Methods for treating TNF.alpha.-related diseases
A stable subcutaneous formulation of anti-TNF-α antibodies addresses the inconvenience of intravenous administration by enabling self-administration, improving patient convenience and treatment efficacy for TNF-α-related diseases.
Patent Information
- Authority / Receiving Office
- CA · CA
- Patent Type
- Patents
- Current Assignee / Owner
- CELLTRION INC
- Filing Date
- 2018-08-29
- Publication Date
- 2026-07-07
Abstract
Description
5 [DESCRIPTION) [Invention Title) CA 03074168 2020-02-26 Methods for Treating TNFa-Related Diseases (Technical Field) Voluntary Amendment This application relates to a method of TNF-a-related disease by subcutaneously administering an antibody binding to TNF-a (anti-TNF-a antibody). [Background Artl Tumor necrosis factor-a (TNF-a) is a cell signaling to protein (cytokine) that is involved in systemic inflammation and is a cytokine that mediates acute-phase responses. TNF-a is related to various diseases and disorders, including septicemia, infection, autoimmune diseases, and graft rejection. TNF-a stimulates immune responses and causes many 15 clinical problems associated with autoimmune abnormalities such as rheumatoid arthritis, ankylosing spondylitis, ulcerative colitis, adult Crohn's disease, pediatric Crohn's disease, psoriasis, psoriatic arthritis and the like. Such abnormalities may be treated using TNF-a inhibitors. 20 Infliximab is a type of chimeric monoclonal antibody capable of acting as the TNF-a inhibitor, and currently commercially available infliximab products include Remsima, Remicade, Renflexis and the like. However, these products are all provided as lyophilized powders, which are reconstituted CA 03074168 2020-02-26 and diluted, and injected intravenously in a dosage regimen and dose selected according to each disease. However, the intravenous administration method as described above requires the patient to visit the hospital for 5 medication and takes 2 to 4 hours including the waiting time, indicating that it poses a considerable burden and inconvenience in daily life. In addition, there is a problem that a person who administer the drug is limited to a person who received medical education. 10 Therefore, subcutaneous (SC) administration is proposed as an alternative route of administration. Subcutaneous administration can be self-injected by a trained patient and can shorten the administration time from 30-90 minutes in a conventional art to 2-5 minutes. 15 Commercially available formulation products developed not only for intravenous administration, but also for subcutaneous administration, Rituxan (Rituximab), Simponi (Golimumab), Herceptin (Trastuzumab), Actemra (Tocilizumab), Xolair (Omalizumab), and the like, but a formulation for subcutaneous 20 administration of Infliximab has not yet been reported. For subcutaneous administration, a stable liquid formulation containing a high concentration of antibody is required, and the clinical efficacy and safety thereof should be demonstrated. 2 CA 03074168 2020-02-26 The Applicant has demonstrated the efficacy and stability of an Inflixirnab formulation for subcutaneous administration, which are equivalent to those of conventional formulations for intravenous administration, thereby completing a subcutaneous 5 administration regimen that improves patient convenience and improves the quality of life of the patient. [Disclosure] [Technical Problem] It is an object of the present invention to provide a 10 treatment method comprising administering subcutaneously to a subject a pharmaceutical composition containing an anti-TNF-cx antibody or its antigen-binding fragment for treatment of TNFa- related disease. It is an object of the present invention to provide a use 15 of a pharmaceutical composition comprising an anti-TNF-cx antibody or its antigen-binding fragment and a pharmaceutically acceptable carrier, for the treatment of a TNF-a-related disease in a patient, wherein the pharmaceutical composition comprises a dose of 60 to 300 mg of the anti-TNF-a antibody or 20 its antigen-binding fragment for subcutaneous use at intervals of 1 to 8 weeks. It is an object of the present invention to provide a use of a pharmaceutical composition comprising an anti-TNF-a antibody or its antigen-binding fragment and a pharmaceutically 25 acceptable carrier, for the preparation of a medicament for the 3 CA 03074168 2020-02-26 treatment of a TNF-er:-related disease in a patient, wherein the pharmaceutical composition comprises a dose of 60 to 300 mg of the anti-TNF-er: antibody or its antigen-binding fragment for subcutaneous use at intervals of 1 to 8 weeks 5 Another object of the present invention is to provide a pharmaceutical composition for treatment of a disease treatable with an anti-TNF-er: antibody, which contains the anti-TNF-a antibody or its antigen-binding fragment and is to be administered subcutaneously to a subject. 10 It is an object of the present invention to provide a pharmaceutical composition for treatment of TNF-er:-related disease, comprising an anti-TNF-a antibody or its antigenbinding fragment and a pharmaceutically acceptable carrier, wherein the anti-TNF-er: antibody or its antigen-binding fragment 15 is adapted for subcutaneous use at a dose of 60 to 300 mg and at intervals of 1 to 8 weeks. Still another object of the present invention is to provide a kit comprising: a pharmaceutical composition containing an anti-TNF-a antibody or its antigen-binding 20 fragment; and instructions that direct the pharmaceutical composition to be administered subcutaneously to a subject in order to treat disease treatable with the anti-TNF-a antibody. It is an object of the present invention to provide a kit comprising: 4 CA 03074168 2020-02-26 (a) a pharmaceutical composition comprising an anti-TNF-a antibody or its antigen-binding fragment; and (b) instructions that direct the pharmaceutical composition to be administered subcutaneously at a dose of 60 5 to 300 mg and at intervals of 1 to 8 weeks in order to treat a patient having TNF-a-related disease. Yet another object of the present invention is to provide the use of an anti-TNF-a antibody or its antigen-binding fragment in the manufacture of a medicament which is to be 10 administered subcutaneously to a subject in order to treat a disease treatable with the anti-TNF-a antibody. [Technical Solution] The present invention provides a method for treating disease treatable with an anti-TNF-a antibody, the method 15 comprising a step of administering subcutaneously to a subject a pharmaceutical composition containing the anti-TNF-a antibody or its antigen-binding fragment. The present invention also provides a pharmaceutical composition for treatment of a disease treatable with an anti- 20 TNF-a antibody, which contains the anti-TNF-a antibody or its antigen-binding fragment and is to be administered subcutaneously to a subject. The present invention also provides a kit comprising: (a) a pharmaceutical composition containing an anti-TNF-a antibody 25 or its antigen-binding fragment, and pharmaceutically 5 CA 03074168 2020-02-26 acceptable carrier; and {b) instructions that direct the pharmaceutical composition to be administered subcutaneously to a subject in order to treat a disease treatable with the antiTNF- o: antibody. s The present invention also provides the use of an anti- TNF-o: antibody or its antigen-binding fragment in the preparation of a pharmaceutical composition which is to be administered subcutaneously to a subject in order to treat a disease treatable with the anti-TNF-o: antibody. 10 In one embodiment of the present invention, the anti-TNFo: antibody may comprise one or more selected from the group consisting of infliximab, adalimumab, certolizumab pegol, golimumab, and biosimilar thereof. In one embodiment of the present invention, the anti-TNF- 15 o: antibody may be infliximab. In one embodiment of the present invention, the anti-TNFo: antibody may comprise a chimeric human-mouse IgG monoclonal antibody. In one embodiment of the present invention, the anti-TNF- 20 o: antibody may comprise: a light-chain variable region comprising a CDR1 domain comprising an amino acid sequence of SEQ ID NO: 1, a CDR2 domain comprising an amino acid sequence of SEQ ID NO: 2, and a CDR3 domain comprising an amino acid sequence of SEQ ID NO: 3; and a heavy-chain variable region 25 comprising a CDRl domain comprising an amino acid sequence of 6 CA 03074168 2020-02-26 SEQ ID NO: 4, a CDR2 domain comprising an amino acid sequence of SEQ ID NO: 5, and a CDR3 domain comprising an amino acid sequence of SEQ ID NO: 6. In one embodiment of the present invention, the anti-TNF- 5 Ol antibody may comprise: a light-chain variable region comprising an amino acid sequence of SEQ ID NO: 7; and a heavychain variable region comprising an amino acid sequence of SEQ ID NO: 8. In one embodiment of the present invention, the anti-TNF- 10 Ol antibody may comprise: a light chain comprising an amino acid sequence of SEQ ID NO: 9; and a heavy chain comprising an amino acid sequence of SEQ ID NO: 10. In one embodiment of the present invention, the composition may comprise: a surfactant; a sugar or its 15 derivative; and a buffer comprising acetate or histidine. In one embodiment of the present invention, the composition may comprise, as a surfactant, polysorbate 20, polysorbate 40, polysorbate 60, polysorbate 80, or a mixture thereof. 20 In one embodiment of the present invention, the concentration of the surfactant in the composition may be 0.02 to O. 1 % (w / v) . In one embodiment of the present invention, the composition may comprise, as sugar or its derivative, sorbitol, 25 mannitol, trehalose, sucrose, or a mixture thereof. 7 CA 03074168 2020-02-26 In one embodiment of the present invention, the concentration of the sugar or its derivative in the composition may be 1 to 10 % (w / v). In one embodiment of the present invention, the s composition may comprise, as a buffer, acetate. In one embodiment of the present invention, the concentration of the buffer in the composition may be 1 to 50 mM. In one embodiment of the present invention, the 10 composition may have a pH of 4.0 to 5.5. In one embodiment of the present invention, the composition may comprise: (A) 90 to 180 mg / ml of the anti-TNF-a antibody or its antigen-binding fragment; (B) 0. 02 to O .1 % (w / v) of polysorbate; (C) 1 to 10% (w / v) of sorbitol; and (D) 1 15 to 50 mM of a buffer comprising acetate or histidine. In one embodiment of the present invention, the composition may be free of aspartic acid, lysine, arginine, or a mixture thereof. In one embodiment of the present invention, the 20 composition may be free of NaCl, KCl, NaF, KBr, NaBr, Na2S04, NaSCN, K2S04, or a mixture thereof. In one embodiment of the present invention, the composition may be free of a chelating agent. In one embodiment of the present invention, the 25 composition may have a viscosity of O. 5 cp to 10. 0 cp after 1 8 CA 03074168 2020-02-26 month of storage at a temperature of 40°C ± 2°C, or a viscosity of 0.5 cp to 5 cp after 6 months of storage at a temperature of s0c ± 3°c. In one embodiment of the present invention, the 5 composition may not be subjected to a reconstitution step, a dilution step, or both, before use. In one embodiment of the present invention, the composition may be filled in a pre-filled syringe or an autoinjector before administration to the subject. IO In one embodiment of the present invention, the subject may include mammals. In one embodiment of the present invention, the subject may include human beings. In one embodiment of the present invention, the antibody 15 or its antigen-binding fragment may be administered at a dose of 60 to 300 mg. In one embodiment of the present invention, the antibody or its antigen-binding fragment may be administered at a dose of 60, 70, 80, 90, 100, 110, 120, 130, 140, 150, 160, 170, 180, 20 190, 200, 210, 220, 230, 240, 250, 260, 270, 280, 290 or 300 mg. In one embodiment of the present invention, the antibody or its antigen-binding fragment may be administered at a dose of 90 to 180 mg. 9 CA 03074168 2020-02-26 In one embodiment of the present invention, the antibody or its antigen-binding fragment may be administered at a dose of 120 to 240 mg. In one embodiment of the present invention, the antibody 5 or its antigen-binding fragment may be administered at a dose of 80 to 100 mg, 110 to 130 mg, 170 to 190 mg, or 230 to 250 mg. In one embodiment of the present invention, the antibody or its antigen-binding fragment may be administered at a dose 10 of 90 mg, 120 mg, 180 mg or 240 mg. In one embodiment of the present invention, the antibody or its antigen-binding fragment may be administered at a dose of 90 to 180 mg when the body weight of the patient is less than 80 kg, and may be administered at a dose of 190 to 270 mg 15 when the body weight of the patient is more than 80 kg. In one embodiment of the present invention, the antibody or its antigen-binding fragment may be administered at intervals of 1 to 8 weeks. In one embodiment of the present invention, the antibody 20 or its antigen-binding fragment may be administered at intervals of 1, 2, 3, 4, 5, 6, 7 or 8 weeks. In one embodiment of the present invention, the antibody or its antigen-binding fragment may be administered at intervals of 2 or 4 weeks. 10 CA 03074168 2020-02-26 In one embodiment of the present invention, the diseases treatable with the anti-TNF-cx antibody may include rheumatoid arthritis, ulcerative colitis, Crohn's disease, plaque psoriasis, psoriatic arthritis, and ankylosing spondylitis. 5 In one embodiment of the present invention, the patient to be administered with the anti-TNF-cx antibody may exhibit one or more characteristics selected from the following: a) a patient who has an inadequate response to diseasemodifying anti rheumatic drugs (DMARDs), including 10 methotrexate; 15 b) a patient who has not previously been treated with methotrexate and other DMARDs; c) a patient who exhibits elevated serologic indicators associated inflammation, therapies; with severe which show axial-predominant symptoms and no proper response to common d) a patient contraindicated to, who does not respond or has intolerance to to, or is methotrexate, cyclosporine, or systemic therapies including psoralen 20 ultraviolet A therapy (PUVA); e) a patient who has an inadequate response to, or has intolerance to, or is contraindicated for treatment with corticosteroids, 6-mercaptopurine, azathioprine or immunosuppressants; and 11 f) a patient who does not respond to common therapies, including antibiotic, excretion or immunosuppressive therapies. In one embodiment of the present invention, the patient may be a patient who has been administered at least once 5 intravenously with the anti-TNF-a antibody or its antigenbinding fragment prior to subcutaneous administration. In one embodiment of the present invention, the patient may be a patient who has been administered intravenously with the anti-TNF-a antibody or its antigen-binding fragment at a 10 dose of 1 to 10 mg / kg for each administration prior to subcutaneous administration. 15 In one embodiment of the present invention, the first subcutaneous administration may be performed 2 to 8 weeks after the last intravenous administration. In one embodiment of the present invention, the first subcutaneous administration may be performed 4 weeks after the last intravenous administration. In one embodiment of the present invention, the composition containing the anti-TNF-a antibody or its antigen- 20 binding fragment may be administered simultaneously with, before or after administration of one or more selected from the group consisting of infliximab, adalimumab, etanercept, certolizumab pegol, golimumab, and biosimilar thereof. In one embodiment of the present invention, the 25 composition containing the anti-TNF-a antibody or its antigen- 12 Date rei,me / Date Received 2024-01-22 CA 03074168 2020-02-26 binding fragment may be administered simultaneously with, before or after administration of methotrexate, lefuromide and sulfasalazine, hydroxychloroquine, or a mixture thereof. In one embodiment of the present invention, the patient 5 after subcutaneous administration may exhibit one or more characteristics selected from the following: a) a decrease in DAS28 (Disease Activity Score in 28 joints) of at least 2.0; and b) a decrease in CDAI (Crohn's disease activity index) of to at least 70. (Advantageous Effects] The treatment method, composition, kit or use according to the present invention makes it possible to treat TNF-cxrelated disease by subcutaneously administering the anti-TNF-cx 15 antibody or its antigen-binding fragment. In addition, the treatment method, composition, kit or use according to the present invention reduces the time for administration and the time for patients to stay in hospitals, thereby improving patient convenience and the quality of life of the patient. 20 This provides the advantage of improving the patient's satisfaction. In addition, the treatment method, composition, kit or use according to the present invention is added as a new treatment option of infliximab, with the result that patients 25 who have been administered intravenously with infliximab, as 13 CA 03074168 2020-02-26 well as healthcare workers, do not have the burden and rejection caused by drug changes. [Description of Drawings] FIG. 1 schematically shows a design of a clinical test 5 for subcutaneous administration of infliximab to rheumatoid arthritis (RA) patients. FIG. 2 schematically shows a design of a clinical test for subcutaneous administration of infliximab to Crohn's disease (CD) patients. 10 [Mode for Invention] The present invention is directed to a method for treatment of a disease treatable with an anti-TNF-cx antibody, the method comprising a step of administering subcutaneously to a subject a pharmaceutical composition containing anti-TNF-cx 15 antibody or its antigen-binding fragment. To facilitate the understanding of the present invention, the terms used in the present invention are defined as follows. "TNF-cx" is intended to refer to a human cytokine that exists as a 17 kD secreted form and a 26 kD membrane associated 20 form, the biologically active form of which is composed of a trimer of noncovalently bound 17 kD molecules. The structure of TNF-cx is described further in, for example, Pennica, D., et al. (1984) Nature 312:724-729; Davis, J.M., et al. (1987) Biochemistry 26:1322-1326; and Jones, E.Y., et al. (1989) 25 Nature 338:225-228. 14 CA 03074168 2020-02-26 The term "antibody" refers to immunoglobulin molecules comprised of four polypeptide chains, two heavy chains and two light chains inter-connected by disulfide bonds. Other naturally occurring antibodies having an altered structure, for 5 example, camelid antibodies, are also included in this definition. Each heavy chain is comprised of a heavy-chain variable region and a heavy-chain constant region. The heavychain constant region is comprised of three domains (CHl, CH2 and CH3). Each light chain is comprised of a light-chain 10 variable region and a light-chain constant region. The lightchain constant region is comprised of one domain (CL) . The heavy-chain variable region and the light-chain variable region can be further subdivided into regions of hypervariability, termed complementarity determining regions (CDR), interspersed 15 with regions that are more conserved, termed framework regions ( FR) . Each of the heavy-chain variable region and the lightchain variable region is composed of three CDRs and four FRs, which are arranged from amino-terminus to carboxy-terminus in the following order: FRl, CDRl, FR2, CDR2, FR3, CDR3, FR4. 20 The term "antigen-binding fragment" refers to one or more fragments of an antibody that retain the ability to specifically bind to an antigen. Examples of antigen-binding fragments include, but are not limited to Fab, Fab', F(ab') 2, Fv, and the like. 15 CA 03074168 2020-02-26 The term "biosimilar" refers to a biological product that is highly similar to an FDA-approved biological product ( reference drug) and has no clinically meaningful differences in terms of pharmacokinetics, safety and efficacy from the 5 reference product. The term "administration" refers to administration of a substance (e.g., anti-TNF-cx antibody) for achieving therapeutic purposes (e.g., TNF-a-related disease). The term "TNF-a-related disease" refers to a local and / or 10 systemic physiological disease where TNF-cx is a primary mediator leading to the manifestation of the disease. The term "TNF-cx-related disease", "disease treatable with anti-TNF-cx" 15 and "disease where the activity of TNF-cx is harmful" are used interchangeably herein. The term "subject" includes all humans animals. The term "non-human animals" includes, or non-human but is not limited to, dogs, cats, vertebrates, such as non-human primates, sheep, rabbits and ferrets, rodents, such as mice, rats and guinea pigs, bird species such as chickens, amphibian, and 20 reptile. In a pre fer red embodiment, the subject is mammals, such as non-human primates, sheep, dogs, cats, rabbits, ferrets, or rodents. In a more preferred embodiment, the subject is a human being. The terms "subject", "patient" and "individual" are used interchangeably herein. 16 CA 03074168 2020-02-26 The term "IC50" is intended to refer to the concentration of an inhibitor, which is required to inhibit the biological outcome of interest, for example, to neutralize cytotoxic activity. 5 The term "kit" refers to a packaged product comprising components for administrating the TNF-a antibody of the present invention to treat TNF-a-related disease. The kit preferably comprises a box or container that holds the components of the kit. The box or container is affixed with a label or a Food and 10 Drug Administration approved protocol. The box or container holds components of the present invention that are contained within plastic, polyethylene, polypropylene, ethylene or propylene containers. The containers can be capped-tubes or bottles. The kit can also include instructions for 15 administering the anti-TNF-a antibody. Various aspects of the present invention will be described in further detail. - Anti-TNF-a antibody or its antigen-binding fragment of 20 the present invention In one embodiment of the present invention, the pharmaceutical formulation may contain, as the antibody, a polyclonal antibody, a monoclonal antibody, a recombinant antibody, a single-chain antibody, a hybrid antibody, a 25 chimeric antibody, a humanized antibody, or a fragment thereof. 17 CA 03074168 2020-02-26 The term "chimeric antibody" refers to an antibody comprising heavy-chain and light-chain variable region sequences from one species and constant region sequences from another species. In one embodiment of the present invention, the pharmaceutical s formulation may contain, as the antibody, a chimeric humanmouse IgG monoclonal antibody. The chimeric human-mouse IgG monoclonal antibody is comprised of mouse heavy-chain and light-chain variable regions and human heavy-chain and lightchain constant regions bound thereto. The chimeric human-mouse IO IgG monoclonal antibody may be produced according to a method known in the art. For example, infliximab may be produced according to a method described in US Patent No. 6,284,471. In one embodiment of the present invention, the pharmaceutical formulation may contain, as the antibody, an 15 antibody that binds to TNF-cx or the epi tope of TNF-cx. The antibody that binds to TNF-cx or the epitope of TNF-cx may comprise infliximab, adalimumab, certolizumab pegol, golimumab, or biosimilar thereof. In one embodiment of the present invention, the antibody may comprise infliximab. 20 In one embodiment of the present invention, the antibody or its antigen-binding fragment (A) may comprise: a light-chain variable region comprising a CDRl domain comprising an amino acid sequence of SEQ ID NO: 1, a CDR2 domain comprising an amino acid sequence of SEQ ID NO: 2, and a CDR3 domain 25 comprising an amino acid sequence of SEQ ID NO: 3; and a heavy- 18 CA 03074168 2020-02-26 chain variable region comprising a CDRl domain comprising an amino acid sequence of SEQ ID NO: 4, a CDR2 domain comprising an amino acid sequence of SEQ ID NO: 5, and a CDR3 domain comprising an amino acid sequence of SEQ ID NO: 6. 5 In one embodiment of the present invention, the antibody or its antigen-binding fragment (A) may comprise: a light-chain variable region having an amino acid sequence of SEQ ID NO: 7; and a heavy-chain variable region having an amino acid sequence of SEQ ID NO: 8. 10 In one embodiment of the present invention, the antibody or its antigen-binding fragment (A) may comprise: a light chain having an amino acid sequence of SEQ ID NO: 9; and a heavy chain having an amino acid sequence of SEQ ID NO: 10. Composition containing anti-TNF-a antibody or its 15 antigen-binding fragment of the present invention As used herein, the expression "composition containing anti-TNF-a antibody or its antigen-binding fragment of the present invention" is used interchangeably with "stable liquid pharmaceutical formulation". 20 A stable liquid pharmaceutical formulation according to the present invention contains: (A) an antibody or its antigenbinding fragment; (B) a surfactant; (C) a sugar or its derivative; and {D) a buffer. As used herein, the term "free of" means that the 25 formulation is completely free of the corresponding component. 19 CA 03074168 2020-02-26 In addition, the term means that the formulation is substantially free of the corresponding component, that is, contains the corresponding component in an amount that does not affect the activity of the antibody and the stability and 5 viscosity of the liquid pharmaceutical formulation. For example, the term means that the formulation contains the corresponding component in an amount of Oto 1% (w / v}, 0 to 1 ppm (w / v), or O to 1 ppb (w / v), based on the total weight of the liquid pharmaceutical formulation. 10 (A) Antibody or Its Antigen-Binding Fragment The concentration of the antibody or its antigen-binding fragment may be freely controlled within a range that does not substantially adversely affect the stability and viscosity of the stable liquid pharmaceutical formulation according to the 15 present invention. In one embodiment of the present invention, the concentration of the antibody or its antigen-binding fragment may be 10 to 200 mg / ml. In another embodiment of the present invention, the concentration of the antibody or its antigen-binding fragment may be 50 to 200 mg / ml. In still 20 another embodiment of the present invention, the concentration of the antibody or its antigen-binding fragment may be 80 to 150 mg / ml. In still another embodiment of the present invention, the concentration of the antibody or its antigenbinding fragment may be 90 to 145 mg / ml. In yet another 25 embodiment of the present invention, the concentration of the 20 CA 03074168 2020-02-26 antibody or its antigen-binding fragment may be 110 to 130 mg / ml. If the concentration of the antibody or its antigenbinding fragment is within the above-described range, the high content of the antibody or its antigen-binding fragment makes 5 it possible to increase the degree of freedom of dose and administration cycle, and the pharmaceutical formulation may exhibit excellent long-term stability and low viscosity. (B) Surfactant Examples of the surfactant include, but are not limited 10 to, polyoxyethylene sorbitan fatty acid ester (e.g., polysorbate), polyoxyethylene alkyl ether (e.g., Brij), alkylphenyl polyoxyethylene ether (e.g., Triton-X), polyoxyethylene-polyoxypropylene copolymers (e.g., Poloxamer, Pluronic), sodium dodecyl sulfate (SOS), and the like. 15 In one embodiment of the present invention, the surfactant may comprise polyoxyethylene sorbitan fatty acid ester (polysorbate) . The polysorbate may comprise polysorbate 20, polysorbate 40, polysorbate 60, polysorbate 80, or a mixture of two or more thereof. In one embodiment of the 20 present invention, the polysorbate may comprise polysorbate 20, polysorbate 80, or a mixture thereof. In another embodiment of the present invention, the polysorbate may comprise polysorbate 80. In one embodiment of the present invention, the 25 concentration of the surfactant may be freely controlled within 21 CA 03074168 2020-02-26 a range that does not substantially adversely affect the stability and viscosity of the stable liquid pharmaceutical formulation according to the present invention. For example, the concentration of the surfactant may be O. 001 to 5% (w / v), 5 0.01 to 1% (w / v), or 0.02 to 0.1% (w / v). If the concentration of the surfactant is within the above-described range, the pharmaceutical composition may exhibit excellent long-term stability and low viscosity. 10 (C) Sugar or Its Derivative The sugar may comprise a monosacchride, a disaccharide, an oligosaccharide, a polysaccharide, or a mixture of two or more thereof. Examples of the monosacchride include, but are not limited to, glucose, fructose, galactose, and the like. Examples of the disaccharide include, but are not limited to, 15 sucrose, lactose, maltose, trehalose, and the like. Examples of the oligosaccharide include, but are not limited to, fructooligosaccaharides, galactooligosaccaharides, mannanoligosaccaharides, and the like. Examples of the polysaccharide include, but are not limited to, starch, 20 glycogen, cellulose, chitin, pectin, and the like. 25 The sugar derivative may comprise sugar alcohol, sugar acid, or a mixture thereof. Examples of the sugar alcohol include, but are not limited to, glycerol, erythritol, threitol, arabitol, galactitol, fucitol, xylitol, iditol, 22 ribitol, inositol, mannitol, sorbitol, volemitol, isomalt, CA 03074168 2020-02-26 maltitol, lactitol, maltotriitol, maltotetraitol, polyglycitol, and the like. Examples of the sugar acid include, but are not limited to, aldonic acid (glyceric acid, etc.), ulosonic acid (neuraminic acid, etc.), uronic acid (glucuronic acid, etc.), 5 aldaric acid (tartaric acid, etc.), and the like. In one embodiment of the present invention, the sugar or its derivative (C) may comprise sorbitol, mannitol, trehalose, sucrose, or a mixture of two or more thereof. In one embodiment of the present invention, the IO concentration of the sugar or its derivative may be freely controlled within a range that does not substantially adversely affect the stability and viscosity of the stable liquid pharmaceutical formulation according to the present invention. For example, the concentration of the sugar or its derivative 15 may be 0.1 to 30% (w / v), 1 to 20% (w / v), or 1 to 10% (w / v). If the concentration of the sugar or its derivative may be within this range, the pharmaceutical composition may exhibit excellent long-term stability and low viscosity. (D) Buffer 20 The buff er that is used in the present invention is a neutralizing substance that minimizes the change in pH caused by acid or alkali. Examples of the buffer include phosphate, acetate, succinate, gluconate, glutamate, citrate, histidine, and the like. In one embodiment of the present invention, the 25 buffer may comprise acetate or histidine. If the buffer 23 CA 03074168 2020-02-26 comprises both acetate and histidine, the stability of the pharmaceutical formulation may be reduced. In one embodiment of the present invention, the buffer may comprise acetate. Examples of the acetate include, but are 5 not limited to, sodium acetate, zinc acetate, aluminum acetate, ammonium acetate, potassium acetate, and the like. For pH adjustment, the buffer may further comprise an acid, for example, acetic acid. When the buffer comprises acetate, it may be most preferable in terms of pH adjustment and stability. 10 In one embodiment of the present invention, the buffer may comprise histidine. When the buffer comprises histidine, it may comprise a histidine salt, for example, histidine chloride, histidine acetate, histidine phosphate, histidine sulfate, or the like. For pH adjustment, the buffer may comprise an acid, 15 for example, hydrochloric acid, acetic acid, phosphoric acid, sulfuric acid, or the like. In one embodiment of the present invention, the stable liquid pharmaceutical formulation may be free of citrate, phosphate, or a mixture thereof. 20 In one embodiment of the present invention, the concentration of the buffer (or the anion of the buffer) may be freely controlled within a range that does not substantially adversely affect the stability and viscosity of the stable liquid pharmaceutical formulation according to the present 25 invention. For example, the concentration of the buffer or its 24 CA 03074168 2020-02-26 anion may be 1 to 50 mM, 5 to 30 mM, or 10 to 25 mM. If the concentration of the buffer or its anion is within this range, the pharmaceutical composition may exhibit excellent long-term stability and low viscosity. 5 (E) pH In one embodiment of the present invention, the pH of the stable liquid pharmaceutical composition may be 4.0 to 5.5, or 4.7 to 5.3. If the pH is within this range, the pharmaceutical composition may exhibit excellent long-term stability and low 10 viscosity. The pH of the pharmaceutical formulation may be adjusted using the buffer. In other words, if the pharmaceutical formulation contains a certain content of the buffer, it may exhibit the pH in the above-described range without having to use a separate pH-adjusting agent. If 15 citrate, phosphate or a mixture thereof is used as the buffer, it may be difficult to show the pH in the above-described range. If the pharmaceutical formulation further contains an acid (e.g., hydrochloric acid) or a base (e.g., sodium hydroxide) as a separate pH-adjusting agent, the stability of 20 the antibody may be reduced. (F) Other Components In one embodiment of the present invention, the stable liquid pharmaceutical formulation may be free of aspartic acid, lysine, arginine, or mixtures thereof. If the stable liquid 25 pharmaceutical formulation contains these amino acids, it may 25 CA 03074168 2020-02-26 become solid. In one embodiment of the present invention, the stable liquid pharmaceutical formulation may contain one or more amino acids, excluding the above-described three amino acids. In this case, the stable liquid pharmaceutical 5 formulation may contain the one or more amino acid in an amount of 5% (w / v) or less, for example, 0.001 to 5% (w / v), 0.001 to 1% (w / v), 0.01 to 5% {w / v), 0.01 to 1% (w / v), 0.1 to 5% (w / v), or 0.1 to 1% (w / v). In another embodiment of the present invention, the 10 stable liquid pharmaceutical formulation may contain taurine. In this case, the taurine may be contained in an amount of 5% (w / v) or less, for example, 0. 001 to 5% (w / v), 0. 001 to 1% (w / v), 0.01 to 5% {w / v), 0.01 to 1% (w / v}, 0.1 to 5% (w / v), or 0 .1 to 1% (w / v) . 15 In one embodiment of the present invention, the stable liquid pharmaceutical formulation may be free of a metal salt, such as NaCl, KCl, NaF, KBr, NaBr, Na2SO4, NaSCN, K2SO4 or the like. If the stable liquid pharmaceutical formulation contains these metal salts, precipitation in the formulation may occur, 20 and the formulation may be gelatinized and may have poor stability. In one embodiment of the present invention, the stable liquid pharmaceutical formulation may be free of a chelating agent (e.g., EDTA). If the pharmaceutical formulation contains 25 a chelating agent, the oxidation rate thereof may be increased. 26 CA 03074168 2020-02-26 In one embodiment of the present invention, the stable liquid pharmaceutical formulation may be free of a preservative. Examples of the preservative include octadecyl dimethylbenzyl ammonium chloride, hexamethonium chloride, 5 benzalkonium chloride, benzethonium chloride, phenol, butyl alcohol, benzyl alcohol, alkyl paraben, catechol, resorcinol, cyclohexanol, 3-pentanol, m-cresol, and the like. If the pharmaceutical formulation contains the preservative, the preservative may not help improve the stability of the IO pharmaceutical formulation. In one embodiment of the present invention, the stable liquid phannaceutical formulation of the present invention may further contain an additive known in the art, which does not substantially adversely affect the activity of the antibody and 15 the stability and low viscosity of the formulation. For example, the pharmaceutical formulation may further contain an aqueous carrier, an antioxidant, or a mixture of two or more thereof. The aqueous carrier is a carrier that is pharmaceutically acceptable (safe and non-toxic when 20 administered to humans) and is useful for preparation of liquid pharmaceutical formulations. Examples of the aqueous carrier include, but are not limited to, sterile water for injection (SWFI), bacteriostatic water for injection (BWFI), sterile saline solution, Ringer's solution, dextrose, and the like. 27 CA 03074168 2020-02-26 Examples of the antioxidant include, but are not limited to, ascorbic acid and the like. (G) "Stable" Liquid Pha:r:maceutical Fo:anulation The term "stable" in the "stable" liquid pharmaceutical s formulation of the present invention means that the antibody according to the present invention essentially retains its physical stability and / or chemical stability and / or biological activity during production and / or upon storage. Various analytical techniques for measuring protein stability are 10 readily available in the art. Physical stability may be assessed by methods known in the art, which include measurement of a sample's apparent attenuation of light (absorbance, or optical density). Such a measurement of light attenuation is related to the turbidity of 15 a formulation. In addition, for physical stability, the contents of high-molecular-weight components, the contents of low-molecular-weight components, the amounts of intact proteins, the number of sub-visible particles, and the like, may be measured. 20 Chemical stability detecting and quantifying can be assessed by, chemically altered for forms example, of the antibody. Chemical stability includes charge alteration ( for example, occurring as a result of deamidation or oxidation) which can be evaluated by, for example, ion-exchange 28 CA 03074168 2020-02-26 chromatography. For chemical stability, charge variants {acidic or basic peaks) may be measured. Biological activity may be assessed by methods known in the art. For example, antigen-binding affinity may be measured 5 by ELISA. 10 In one embodiment of the present invention, the liquid pharmaceutical formulation may be stable for a long period of time. In one embodiment of the "stable" liquid pharmaceutical present invention, formulation means the term a liquid pharmaceutical formulation satisfying one or more of the following criteria. Turbidity a liquid pharmaceutical formulation having an 15 absorbance AGoo of O to 0.0300, or O to 0.0700, as measured by a spectrophotometer after 4 weeks of storage at a temperature of 40°C ± 2°C; a liquid pharmaceutical formulation having an absorbance AGoo of O to O. 0300, or O to O. 0700, as measured by a 20 spectrophotometer after 4 weeks of storage at a temperature of 40°C ± 2°C and a relative humidity of 75 ± 5% under a closed condition; Content of Main Component {main peak) a liquid pharmaceutical formulation in which the 25 content of a main component content after 4 weeks of storage at 29 CA 03074168 2020-02-26 a temperature of 40°C ± 2°C is 98% to 100% as measured by SEHPLC; a liquid pharmaceutical formulation in which the content of a main component content after 4 weeks of storage at 5 a temperature of 40°C ± 2°c and a relative humidity of 75 ± 5% under a closed condition is 98% to 100% as measured by SE-HPLC; Content of High-Molecular-Weight Components (a peak whose retention time is earlier than that of the main peak (intact IgG)) 10 a liquid pharmaceutical formulation in which the content of high-molecular-weight components after 12 months of storage at a temperature of S°C ± 3°C is Oto 1.00% as measured by SE-HPLC; a liquid pharmaceutical formulation in which the 15 content of high-molecular-weight components after 12 months of storage at a temperature of 5°C ± 3°C under a closed condition is Oto 1.00% as measured by SE-HPLC; Content of Low-Molecular-Weight Components (a peak whose retention time is later than that of the main peak (intact IgG) 20 a liquid pharmaceutical formulation in which the content of low-molecular-weight components after 12 months of storage at a temperature of S°C ± 3°C is Oto 0.40% as measured by SE-HPLC; a liquid pharmaceutical formulation in which the 25 content of low-molecular-weight components after 12 months of 30 CA 03074168 2020-02-26 storage at a temperature of 5°C ± 3°C under a closed condition is Oto 0.40% as measured by SE-HPLC; Content of Intact Immunoglobulin G a liquid pharmaceutical formulation in which the 5 content of intact irnmunoglobulin G (intact IgG %) after 12 months of storage at a temperature of 5°C ± 3°C is 94. 0% to 100% as measured by Non-reducing CE-SOS; a liquid pharmaceutical formulation in content of intact irnmunoglobulin G (intact IgG %) which the after 12 IO months of storage at a temperature of 5°C ± 3°C under a closed condition is 94.0% to 100% as measured by Non-reducing CE-SDS; a liquid pharmaceutical formulation in which the content of intact irnmunoglobulin G (intact IgG %) after 4 weeks of storage at a temperature of 40°C ± 2°C is 94.0% to 100% as 15 measured by Non-reducing CE-SOS; a liquid pharmaceutical formulation in which the content of intact irnmunoglobulin G content (intact IgG %) after 4 weeks of storage at a temperature of 40°C ± 2°C and a relative humidity of 75 ± 5% under a closed condition is 94.0% 20 to 100% as measured by Non-reducing CE-SDS; Content of Intact Heavy Chain and Light Chain a liquid pharmaceutical formulation in which the content of intact heavy chain and light chain (intact HC+LC %) after 12 months of storage at a temperature of 5 °C ± 3 °C is 25 99.0% to 100% as measured by reducing CE-SOS; 31 CA 03074168 2020-02-26 a liquid pharmaceutical formulation in which the content of intact heavy chain and light chain (intact HC+LC %) after 12 months of storage at a temperature of 5°C ± 3°C under a closed condition is 99.0% to 100% as measured by reducing CE- 5 SDS; a liquid pharmaceutical formulation in which the content of intact heavy chain and light chain (intact HC+LC %) after 4 weeks of storage at a temperature of 40°C ± 2 °C is 98.0% to 100% as measured by reducing CE-SDS; 10 a liquid pharmaceutical formulation in which the content of intact heavy chain and light chain content (intact HC+LC %) after 4 weeks of storage at a temperature of 40°C ± 2 °C under a closed condition is 98. 0% to 100% as measured by reducing CE-SDS; 15 Number of sub-visible particles - a liquid pharmaceutical formulation in which the number of sub-visible particles (~10.00 μm, <400.00 μm) after 12 months of storage at a temperature of 5°C ± 3°C is Oto 1,000 as measured by HIAC; 20 - a liquid pharmaceutical formulation in which the number of sub-visible particles (~10.00 μm, <400.00 μm) after 12 months of storage at a temperature of 5°C ± 3°C under a closed condition is Oto 1,000 as measured by HIAC; - a liquid pharmaceutical formulation in which the number 25 of sub-visible particles (~1. 00 μm, <100. 00 μm) after 4 weeks 32 CA 03074168 2020-02-26 of storage at a temperature of 40°C ± 2°C is O to 30,000 as measured by MFI; - a liquid pharmaceutical formulation in which the number of sub-visible particles (~1.00 μm, <100.00 μm) after 4 weeks s of storage at a temperature of 40°C ± 2 °c and a relative humidity of 75 ± 5% under a closed condition is Oto 30,000 as measured by MFI; - a liquid pharmaceutical formulation in which the number of sub-visible particles (~10.00 μm, <100.00 μm) after 4 weeks 10 of storage at a temperature of 40°C ± 2°C is O to 200 as measured by MFI; - a liquid pharmaceutical formulation in which the number of sub-visible particles (~10.00 μm, <100.00 μm) after 4 weeks of storage at a temperature of 40°C ± 2 °C and a relative IS humidity of 7 5 ± 5% under a closed condition is O to 2 00 as measured by MFI; - a liquid pharmaceutical formulation in which the number of sub-visible particles (~10.00 μm, <100.00 μm) after 6 weeks of storage at a temperature of 40°C ± 2°C is O to 500 as 20 measured by MFI; - a liquid pharmaceutical formulation in which the number of sub-visible particles (~10.00 μm, <100.00 μm) after 6 weeks of storage at a temperature of 40°C ± 2 °C and a relative humidity of 75 ± 5% under a closed condition is O to 500 as 25 measured by MFI; 33 CA 03074168 2020-02-26 Oxidation Rate a liquid pharmaceutical formulation in which the oxidation rate of heavy-chain Met 255 after 4 weeks of storage at a temperature of 40°C ± 2°C is 0% to 2.5% as measured by LC- 5 MS; a liquid pharmaceutical formulation in which the oxidation rate of heavy-chain Met 255 after 4 weeks of storage at a temperature of 40°C ± 2°C and a relative humidity of 75 ± 5% under a closed condition is 0% to 2.5% as measured by LC-MS; Charge Variants - a liquid pharmaceutical formulation showing an acidic peak of 20% to 35% as measured by IEC-HPLC after 4 weeks of storage at a temperature of 40°C ± 2°C; - a liquid pharmaceutical formulation showing an acidic 15 peak of 20% to 35% as measured by IEC-HPLC after 4 weeks of storage at a temperature of 40°C ± 2°C and a relative humidity of 75 ± 5% under a closed condition; - a liquid pharmaceutical formulation showing a basic peak of 33% to 40% as measured by IEC-HPLC after 4 weeks of 20 storage at a temperature of 40°C ± 2°C; 25 - a liquid pharmaceutical formulation showing a basic peak of 33% to 40% as measured by IEC-HPLC after 4 weeks of storage at a temperature of 40°C ± 2°C and a relative humidity of 75 ± 5% under a closed condition; TNF-a Binding Affinity 34 CA 03074168 2020-02-26 - a liquid pharmaceutical formulation having a TNF-a binding affinity of 80% to 120% as measured by ELISA after 12 months of storage at a temperature of S°C ± 3°C; and - a liquid pharmaceutical formulation having a TNF-a 5 binding affinity of 80% to 120% as measured by ELISA after 12 months of storage at a temperature of 5°C ± 3°C under a closed condition. In one embodiment of the present invention, the pharmaceutical formulation may have a viscosity of O. S cp to 10 10. 0 cp as measured after 1 month of storage at a temperature of 40°C ± 2°C. In another embodiment of the present invention, the pharmaceutical formulation may have a viscosity of O. S cp to 5.0 cp as measured after 6 months of storage at a temperature of S°C ± 3°C. 15 (H)Method for Preparation of Stable Liquid l?harmaceutical Fo.rmulation The stable liquid pharmaceutical formulation of the present invention may be prepared using any known method which is not limited to a particular method. For example, the stable 20 liquid pharmaceutical formulation may be prepared by adding a buffer to a solution containing a surfactant and a sugar or its derivative while adjusting the pH of the solution, and then adding an antibody to the mixed solution. Alternatively, the liquid pharmaceutical formulation may be prepared by preparing 25 a solution containing some excipients in the final step of a 35 CA 03074168 2020-02-26 purification process, and then adding the remaining component to the solution. For example, the liquid pharmaceutical formulation may be prepared by preparing a solution containing an antibody, a buffer and a sugar or its derivative, and then 5 adding a surfactant to the solution. In addition, the method for preparation of the formulation may comprise or not comprise a freeze-drying step. When the preparation method does not comprise the freezedrying step, for example, the liquid pharmaceutical formulation 10 prepared according to the present invention may be treated by sterilization, and then immediately placed in a closed container. When the preparation method comprises the freeze-drying step, for example, the liquid pharmaceutical formulation 15 prepared according to the present invention may be freeze-dried or freeze-dried and stored, and then components removed or modified by freeze drying and / or storage may be supplemented or replaced, thereby preparing the liquid pharmaceutical formulation according to the present invention. Alternatively, 20 only components of the liquid pharmaceutical formulation of the present invention, excluding components that may be removed or modified by freeze drying and / or storage, may be freeze-dried or freeze-dried and stored, and then the excluded components may be added thereto, thereby preparing the liquid 25 pharmaceutical formulation according to the present invention. 36 Korean Patent Application No. 10-2017-0081814 has been previously filed by the Applicant. - Method for treatment of disease treatable with anti - TNF-a antibody of the present invention 5 The present invention provides a method for treatment of a disease treatable with anti -TNF-a, the method comprising a step of administering subcutaneously to a subject a pharmaceutical composition containing an anti-TNF-a antibody or its antigen-binding fragment. 10 In one embodiment of the present invention, the antibody may comprise infliximab, adalimumab, certolizumab pegol, golimumab, or biosimilar thereof. In one embodiment of the present invention, the antibody may comprise infliximab. 15 In one embodiment of the present invention, the antibody may comprise a chimeric human-mouse IgG monoclonal antibody. In one embodiment of the present invention, the antibody or its the antigen-binding fragment thereof may comprise: a light-chain variable region comprising a CDRl domain comprising 20 an amino acid sequence of SEQ ID NO: 1, a CDR2 domain comprising an amino acid sequence of SEQ ID NO: 2, and a CDR3 domain comprising an amino acid sequence of SEQ ID NO: 3; and a heavy-chain variable region comprising a CDRl domain comprising an amino acid sequence of SEQ ID NO: 4, a CDR2 domain 37 Date rei,me / Date Received 2024-01-22 CA 03074168 2020-02-26 comprising an amino acid sequence of SEQ ID NO: 5, and a CDR3 domain comprising an amino acid sequence of SEQ ID NO: 6. In one embodiment of the present invention, the antibody or its antigen-binding fragment may comprise: a light-chain 5 variable region having an amino acid sequence of SEQ ID NO: 7; and a heavy-chain variable region having an amino acid sequence of SEQ ID NO: 8. In one embodiment of the present invention, the antibody may comprise: a light chain having an amino acid sequence of 10 SEQ ID NO: 9; and a heavy chain having an amino acid sequence of SEQ ID NO: 10. 15 20 25 In one embodiment of the present invention, the antibody or its antigen-binding fragment (A} may be contained at a concentration of 10 to 200 mg / ml. The present invention also provides a method for treatment of a disease treatable with anti-TNF-cx, the method comprising a step of administering subcutaneously to a subject a pharmaceutical composition containing (A} an anti-TNF-cx antibody or its antigen-binding fragment; (B) a surfactant; (C) a sugar or its derivative; (D) a buffer. In one embodiment of the present surfactant (B) may comprise polysorbate, mixture thereof. In one surfactant (B) embodiment of the present may comprise polysorbate 20, 38 invention, poloxamer, the or a invention, the polysorbate 40, CA 03074168 2020-02-26 polysorbate 60, polysorbate 80, or a mixture of two or more thereof. In one embodiment of the present invention, the surfactant (B) may comprise polysorbate 80. 5 In one embodiment of the present invention, the surfactant (B) may be contained at a concentration of 0.02 to 0.1% (w / v). In one embodiment of the present invention, the sugar (C) may comprise a monosacchride, a disaccharide, an 10 oligosaccharide, a polysaccharide, or a mixture of two or more thereof, and the sugar derivative (C) may comprise sugar alcohol, sugar acid, or a mixture thereof. In one embodiment of the present invention, the sugar or its derivative (C) may comprise sorbitol, mannitol, trehalose, 15 sucrose, or a mixture of two or more thereof. In one embodiment of the present invention, the sugar or its derivative (C) may be contained at a concentration of 1 to 10% (w / v) . In one embodiment of the present invention, the buffer 20 (D) may comprise acetate or histidine. In one embodiment of the present invention, the buffer (D) may have a concentration of 1 to 50 rnM. In one embodiment of the present invention, the stable liquid pharmaceutical formulation may have a pH of 4.0 to 5.5. 39 CA 03074168 2020-02-26 In one embodiment of the present invention, the stable liquid pharmaceutical formulation may be free of aspartic acid, lysine, arginine, or mixtures thereof. In one embodiment of the present invention, the stable 5 liquid pharmaceutical formulation may be free of NaCl, KCl, NaF, KBr, NaBr, Na2SO4, NaSCN, K2SO4, or mixtures thereof. In one embodiment of the present invention, the stable liquid pharmaceutical formulation may be free of a chelating agent. 10 In one embodiment of the present invention, the stable liquid pharmaceutical formulation may be free of a preservative. In one embodiment of the present invention, the stable liquid pharmaceutical formulation may further contain an 15 aqueous carrier, an antioxidant, or a mixture of two or more thereof. In one embodiment of the present invention, the stable liquid pharmaceutical formulation may have a viscosity of 0. 5 cp to 10 cp as measured after 1 month of storage at a 20 temperature of 40°C ± 2°C, or a viscosity of 0.5 cp to 5 cp as measured after 6 months of storage at a temperature of 5 °C ± 3 °C. In one embodiment of the present invention, the stable liquid pharmaceutical formulation may contain: (A) an antibody 25 or its antigen-binding fragment, which comprises a light-chain 40 CA 03074168 2020-02-26 variable region comprising a CDRl domain comprising an amino acid sequence of SEQ ID NO: 1, a CDR2 domain comprising an amino acid sequence of SEQ ID NO: 2, and a CDR3 domain comprising an amino acid sequence of SEQ ID NO: 3; and a heavy- 5 chain variable region comprising a CDRl domain comprising an amino acid sequence of SEQ ID NO: 4, a CDR2 domain comprising an amino acid sequence of SEQ ID NO: 5, and a CDR3 domain comprising an amino acid sequence of SEQ ID NO: 6; (B) a surfactant; (C) a sugar or its derivative; and (D) a buffer 10 comprising acetate or histidine. In one embodiment of the present invention, the stable liquid pharmaceutical formulation may contain: (A) 90 to 180 mg / ml of an antibody or its antigen-binding fragment, which comprises a light-chain variable region comprising a CDRl 15 domain comprising an amino acid sequence of SEQ ID NO: 1, a CDR2 domain comprising an amino acid sequence of SEQ ID NO: 2, and a CDR3 domain comprising an amino acid sequence of SEQ ID NO: 3; and a heavy-chain variable region comprising a CDRl domain comprising an amino acid sequence of SEQ ID NO: 4, a 20 CDR2 domain comprising an amino acid sequence of SEQ ID NO: 5, and a CDR3 domain comprising an amino acid sequence of SEQ ID NO: 6; (B) 0. 02 to O .1% (w / v) of a surfactant; (C) 1 to 10% (w / v) of a sugar or its derivative; and (D) 1 to 50 mM of a buffer comprising acetate or histidine. 41 CA 03074168 2020-02-26 In one embodiment of the present invention, the stable liquid pharmaceutical formulation may be administered subcutaneously. In one embodiment of the present invention, the stable s liquid pharmaceutical formulation may not be subjected to a reconstitution step, a dilution step, or both, before use. In one embodiment of the present invention, the stable liquid pharmaceutical formulation may be filled in a pre-filled syringe before use. 10 In one embodiment of the present invention, the prefilled syringe may be included in an auto-injector before use. Disease Treatable with Anti-TNF-a Antibody In one embodiment of the present invention, the disease treatable with the anti-TNF-cx antibody is selected from the 15 group consisting of rheumatoid arthritis, ulcerative colitis, Crohn's disease, plaque psoriasis, psoriatic arthritis, ankylosing spondylitis, juvenile idiopathic arthritis, hemolytic disease of the newborn, inflammatory bowel disease, multiple sclerosis, prevention of organ transplantation 20 rejection, non-Hodgkin's lymphoma, metastatic cancer, retinopathy of prematurity, ovarian cancer, stomach cancer, head and neck cancer, osteoporosis, paroxymal nocturnal hemoglobinuria, invasive candidiasis, breast cancer, melanoma, chronic lymphocytic leukemia, acute myeloid leukemia, renal 25 cell carcinoma, colorectal cancer, asthma, nasopharyngeal 42 CA 03074168 2020-02-26 cancer, hemorrhagic shock, Staphylococcus aureus infection, and follicular lymphoma. In one embodiment of the present invention, the disease treatable with the anti-TNF-a antibody may be a disease 5 treatable by intravenous administration of infliximab. In one embodiment of the present invention, the disease treatable with the anti-TNF-a antibody may be rheumatoid arthritis, ulcerative colitis, Crohn's disease, plaque psoriasis, psoriatic arthritis or ankylosing spondylitis, which 10 is treatable by intravenous administration of infliximab. In one embodiment of the present invention, the subject to be administered with the anti-TNF-a antibody is a patient who has an inadequate response to disease-modifying anti rheumatic drugs (DMARDs), including methotrexate. 15 In one embodiment of the present invention, the subject to be administered with the anti-TNF-a antibody is a patient who has not previously been treated with methotrexate and other DMARDs. In one embodiment of the present invention, the subject 20 to be administered with the anti-TNF-a antibody is a patient who exhibits elevated serologic indicators associated with severe axial-predominant symptoms and inflammation, which show no proper response to coilltl.on therapies. In one embodiment of the present invention, the subject 25 to be administered with the anti-TNF-cx antibody is a patient 43 CA 03074168 2020-02-26 who does not respond to, or are contraindicated to, or has intolerance to methotrexate, cyclosporine, or systemic therapies including psoralen ultraviolet A therapy (PUVA). In one embodiment of the present invention, the subject 5 to be administered with the anti-TNF-cx antibody is a patient who has an inadequate response to, or has intolerance to, or is contraindicated for treatment with corticosteroids, 6- mercaptopurine, azathioprine or immunosuppressants. In one embodiment of the present invention, the subject 10 to be administered with the anti-TNF-cx antibody is a patient who does not respond to common therapies, including antibiotic, excretion or immunosuppressive therapies. Dose and .Administration Interval In one embodiment of the present invention, the anti-TNF- 15 ex antibody or its antigen-binding fragment may be administered at a dose of 60 to 300 mg. Specifically, it may be administered at a dose of 60, 70, 80, 90, 100, 110, 120, 130, 140, 150, 160, 170, 180, 190, 200, 210, 220, 230, 240, 250, 260, 270, 280, 290 or 300 mg. 20 In one embodiment of the present invention, the anti-TNFcx antibody or its antigen-binding fragment may be administered at a dose of 90 to 180 mg. In another embodiment, the anti-TNFcx antibody or its antigen-binding fragment may be administered at a dose of 120 to 240 mg. In still another embodiment, the 44 CA 03074168 2020-02-26 anti-TNF-a antibody or its antigen-binding fragment may be administered at a dose of 120 to 240 mg. In one embodiment of the present invention, the anti-TNF~ antibody or its antigen-binding fragment may be administered 5 at a dose of 90 to 180 mg when the body weight of the patient is less than 80 kg, and may be administered in an amount of 190 to 270 mg when the body weight of the patient is more than 80 kg. In one embodiment of the present invention, the anti-TNF- 10 a antibody or its antigen-binding fragment may be administered at intervals of 1 to 8 weeks. Specifically, it may be administered at intervals of 1 week, 1. 5 weeks, 2 weeks, 2. 5 weeks, 3 weeks, 3.5 weeks, 4 weeks, 4.5 weeks, 5 weeks, 5.5 weeks, 6 weeks, 6.5 weeks, 7 weeks, 7.5 weeks, or 8 weeks. 15 In another embodiment of the present invention, the anti- TNF-a antibody or its antigen-binding fragment may be administered at intervals of 2 to 4 weeks. Pre-administration Before the step of subcutaneously administering the anti- 20 TNF-a antibody or its antigen-binding fragment, a step of intravenously administering the anti-TNF-~ antibody or its antigen-binding fragment may be included. In one embodiment of the present invention, before the subcutaneous administration step, a step of intravenously 25 administering the anti-TNF-a antibody or its antigen-binding 45 CA 03074168 2020-02-26 fragment at a dose of 1 to 10 mg / kg may be included. Specifically, a step of intravenously administering the antiTNF- c.x antibody or its antigen-binding fragment at a dose of 1, 2, 3, 4, 5, 6, 7, 8, 9 or 10 mg / kg may be included. 5 In another embodiment of the present invention, before the subcutaneous administration step, a step of intravenously administering the anti-TNF-cx antibody or its antigen-binding fragment at a dose of 2 to 8 mg / kg may be included. In still another embodiment of the present invention, before the 10 subcutaneous administration step, a step of intravenously administering the anti-TNF-cx antibody or its antigen-binding fragment at a dose of 3 to 5 mg / kg may be included. In one embodiment of the present invention, before the subcutaneous administration step, a step of intravenously 15 administering the anti-TNF-cx antibody or its antigen-binding fragment at intervals of 1 to 8 weeks may be included. Specifically, a step of intravenously administering the antiTNF- c.x antibody or its antigen-binding fragment at intervals of 1, 1 . 5, 2 , 2 . 5, 3, 3 . 5, 4 , 4 . 5, 5, 5 . 5, 6, 6 . 5, 7, 7 . 5 or 8 20 weeks may be included. In another embodiment of the present invention, before the subcutaneous administration step, a step of intravenously administering the anti-TNF-c.x antibody or its antigen-binding fragment at intervals of 2 to 4 weeks may be included. 46 CA 03074168 2020-02-26 In one embodiment of the present invention, before the subcutaneous administration step, a step of intravenously administering the anti-TNF-cx antibody or its antigen-binding fragment may be included, and the time interval between the 5 last intravenous administration and the first subcutaneous administration is 1 to 8 weeks. Specifically, a step of intravenously administering the anti-TNF-cx antibody or its antigen-binding fragment at intervals of 1, 1. 5, 2, 2. 5, 3, 3.5, 4, 4.5, 5, 5.5, 6, 6.5, 7, 7.5 or 8 weeks may be included. 10 In another embodiment of the present invention, before the subcutaneous administration step, a step of intravenously administering the anti-TNF-cx antibody or its antigen-binding fragment may be included, and the time interval between the last intravenous administration and the first subcutaneous 15 administration is 2 to 4 weeks. Co-administration Other biological agent or chemotherapeutic agent may be administered together with the anti-TNF-cx antibody or its antigen-binding fragment of the present invention. 20 The administration is performed simultaneously with, before or after administration of the anti-TNF-cx antibody or its antigen-binding fragment. In one embodiment of the present invention, the biological agent that is co-administered may comprise 47 CA 03074168 2020-02-26 etanercept, infliximab, adalimumab, certolizumab pegol, golimumab, or a combination thereof. In one embodiment of the present invention, the chemotherapeutic agent that is co-administered may comprise a 5 disease-modifying anti rheumatic drug (DMARD). In one embodiment of the present invention, the chemotherapeutic agent that is co-administered may comprise methotrexate, leflunomide, sulfasalazine, hydroxychloroquine, or a combination thereof. 10 -Product The present invention also provides a product comprising: the stable liquid pharmaceutical formulation; and a container receiving the stable liquid pharmaceutical formulation in a closed state. 15 The stable liquid pharmaceutical formulation is as described above. In one embodiment of the present invention, the container may be formed of a material such as glass, a polymer (plastic), a metal or the like, but is not limited thereto. In one 20 embodiment of the present invention, the container is a bottle, a vial, a cartridge, a syringe (pre-filled syringe, autosyringe), or a tube, but is not limited thereto. In one embodiment of the present invention, the container may be a glass or polymer vial, or a glass or polymer pre-filled 25 syringe. 48 CA 03074168 2020-02-26 Specific product forms of the above-described vial, cartridge, pre-filled syringe or auto-syringe, and methods of filling the stabile liquid pharmaceutical formulation into the vial, cartridge, pre-filled syringe or auto-syringe, may be 5 readily available or implemented by any person skilled in the technical field to which the present invention pertains. For example, US Patent Nos. 4,861,335 and 6,331,174, etc., disclose the specific product form of a pre-filled syringe and a filling method. For example, US Patent Nos. 5,085,642 and 5,681,291, 10 etc., disclose the specific product form of an auto-syringe and an assembly method. The above-described vial, cartridge, prefilled syringe or auto-syringe that is used in the present invention may be a commercially available product, or a product separately manufactured considering the physical properties of 15 the stable liquid pharmaceutical formulation, an area to which the formulation is to be administered, the dose of the formulation, and the like. In one embodiment of the present invention, the inside of the container may not be coated with silicone oil. If it is 20 coated with silicone oil, the stability of the formulation may be reduced. The container may be a single-dose or multiple-dose container. In one embodiment of the present invention, the product may further comprise instructions providing a method of using 25 the stable liquid pharmaceutical formulation, a method of 49 CA 03074168 2020-02-26 storing the formulation, or both. The method of using the formulation includes a method for treating a disease in which TNF-cx activity acts as a harmful factor, and may include the route of administration, the dose of the formulation, and the 5 timing of administration. In one embodiment of the present invention, the product may comprise other required utensils (e.g., a needle, a syringe, etc.) in a commercial viewpoint and a user viewpoint. 10 Hereinafter, the present invention will be described with reference to examples. It is to be understood, however, that these examples are for illustrative purposes only and are not intended to limit the scope of the present invention. 15 Example 1. Evaluation of safety and therapeutic efficacy on subcutaneously administering an inflixima:b to patients with rheumatoid arthritis (RA) The present clinical trial of an infliximab was a randomized, multi-center, parallel-group and phase I / III trial, 20 designed to evaluate efficacy, pharmacokinetics and safety between the infliximab for subcutaneous administration (hereinafter infliximab SC) and the infliximab for intravenous administration (hereinafter infliximab IV) in combination with methotrexate (MTX) and folic acid in patients with active 25 rheumatoid arthritis, who had not shown adequate responses to 50 CA 03074168 2020-02-26 MTX administration over at least 3 months, wherein the present clinical trial was composed of two parts. A part 1 was designed to find an optimal dose of the infliximab SC, wherein the optimal dose of the infliximab SC 5 corresponding to 3 mg / kg of the infliximab IV over the first 30 weeks was identified by means of an area under the concentration-time curve (AUCT) at steady state between Weeks 22 and 30. In case of the part 1, a clinical trial period amounted to a maximum of 65 weeks, inclusive of duration from a 10 screening (the maximum three weeks) to End-of-Study visit. A part 2 was designed to demonstrate the non-inferiority of efficacy between the infliximab SC and the infliximab IV. Thus, by means of the clinical responses according to changes from baseline in disease activity score (DAS28; Disease 15 Activity Score in 28 joints) (C-reactive protein, CRP) using 28 joint counts at Week 22, it might be demonstrated that the infliximab SC was not inferior to the infliximab IV in terms of efficacy. In case of the part 2, the administered dose and dosing interval of the infliximab SC were set to an 20 administration of 120 mg every two weeks. Part l Patients were eligible to enroll into the present clinical trial, provided that they met all of the following 25 criteria: 51 CA 03074168 2020-02-26 * Patient has active disease as defined by the presence of 6 or more swollen joints (of 28 assessed), 6 or more tender joints (of 28 assessed), and a serum CRP concentration >0.6 mg / dL at Screening; and 5 * Patient who has completed at least 3 months of treatment of oral or parenteral dosing with methotrexate between 12.5 to 25 mg / week and on stable dosing with methotrexate between 12 .5 to 25 mg / week for at least 4 weeks prior to the first administration of the study drug (Day 0). 10 Patients were not eligible to enroll into the clinical trial, provided that they met any one of the following criteria: * Patient who has previously received a biological agent for the treatment of RA and / or a TNF-~ inhibitor for the 15 treatment of other disease; and * Patient who has allergies to any of the excipients of infliximab or any other murine and / or human proteins or patient with a hypersensitivity to immunoglobulin product. The present clinical trial was composed of three clinical 20 trial periods: Screening; Treatment period; and End-of-Study visit. The screening was carried out between Days -21 and -1 before an initial administration of the study drug, wherein the eligibility of patients for study was evaluated. All the examinations including hepatitis B, hepatitis C and human 25 immunodeficiency virus (HIV-1 and HIV-2) infections, a urine 52 CA 03074168 2020-02-26 and serum pregnancy test for women of childbearing potential, as well as rheumatoid factor, anti-cyclic citrullinated peptide, 12-lead ECG, clinical laboratory tests, etc., were carried out. Also, an interferon-gamma release assay (IGRA) and a chest X- 5 ray examination were performed so as to exclude tuberculosis (TB) patients. All the patients enrolled into the clinical trial were administered infliximab IV at Weeks 0 and 2, respectively. Further, the patients were administered folic acid in 10 combination with the MTX and the study drug so that adverse events associated with the MTX side effects might be minimized and prevented, wherein they were also reminded of taking a maintenance dose of the MTX from beginning to end of clinical trial. Furthermore, the patients were eligible to take 15 following premedication at an investigator's discretion at a time point of 30 60 minutes before a start of the administration of the study drug so that their hypersensitivity reactions to the study drug might be prevented: e.g., antihistamine {equivalent dose of 2 - 4 mg of chlorpheniramine), 20 hydrocortisone, paracetamol and / or nonsedating antihistamine (equivalent dose of 10 mg of cetirizine), but not limited thereto. Those who were administered a full dose of the study drug twice and deemed to have no concerns about safety at the 25 investigator's discretion, were randomly assigned to an 53 CA 03074168 2020-02-26 infliximab SC cohort or an infliximab IV cohort before the administration at Week 6 / Day 42. Such random assignment with regard to administration of the study drug was stratified by country, a serum CRP concentration (same or less than 0.6 mg / dL 5 or less, or more than 0.6 mg / dL) at Week 2 and a weight (same or less than 70 kg, or more than 70 kg) at Week 6. A total of 50 patients with active RA were enrolled, out of which 48 ones were randomly assigned to four clinical trial Cohorts at a ratio of 1:1:1:1, wherein the administration of the study drug 10 was performed until Week 54 (Table 1) . 15 [Table 1] Cohort Number Administered Drugs for Clinical Trials Administration method Number of Patients Dose C-Ohortl 3 mlll'ke: lnfliximab IV 100 mu / vial 2 hours IV infusion 13 C-Ohort2 90mg lnfliximab SC 90 mg!PFS Simde SC injection 11 Cohortt3 120mg InfliximabSC120mg / PFS Sinide SC injection 12 C-Ohort4 180mg Infliximab SC 90 mg!PFS double SC injection 12 PFS, Pre-filled syringe Those who were assigned to a cohort 1 were administered additional 7 doses of the infliximab IV at Week 6 and subsequently every eight weeks (Weeks 14, 22, 30, 38, 46 and 54). Those who were assigned to Cohorts 2, 3 and 4 were initially administered the infliximab SC at Week 6, and then 20 additionally administered the infliximab SC every two weeks until Week 54. The initially assigned dose was adjusted to the optimal dose in all patients from Cohorts 2, 3 and 4 when the 54 ' CA 03074168 2020-02-26 optimal dose was confirmed after dose finding. After that, an additional SC injection using the optimal dose was administered until Week 54. The infliximab SC was injected into patients by a healthcare professional at each visit (Weeks 6, 8, 10, 14, 22, 5 24, 26, 28, 30, 38, 46 and 54) at a study site. However, in all the other weeks (Weeks 12, 16, 18, 20, 32, 34, 36, 40, 42, 44, 48, 50 and 52), patients were allowed to perform a selfinjection of the infliximab SC, if the investigator determined it as suitable after training them for appropriate injection IO techniques. Patients visited the study site at a predefined time interval for clinical evaluation and blood sampling. At each visit, they were asked questions about adverse events and concomitant medication, while being monitored for clinical 15 signs and symptoms of TB. The evaluation of primary pharmacokinetic endpoints was performed during a maintenance phase between Weeks 22 and 30, then the evaluation of secondary pharmacokinetic endpoints was performed during an treatment period until Week 54, and then blood sampling for analysis as 20 well as the evaluation of efficacy, PD and safety were respectively performed at a point of time specified in an evaluation schedule. An End-of-Study Visit occurred 8 weeks after the last dose was received, either at the end of the Maintenance Phase 25 or earlier if the patient withdrew from the study. At a time 55 5 10 CA 03074168 2020-02-26 point of eight weeks after the last administration to patients, every effort was made to complete all the End-of-Study evaluations. Part 2 A part 2 commenced based on a review by the Data Safety Monitoring Board with regard to PK modeling report data including PK, efficacy, PD and safety data, which were identified over the first 30 weeks in the part 1. The part 2 was composed of three clinical trial periods including Screening; Treatment Period (Dose-Loading Phase and Maintenance Phase) with a double-blinded period during Maintenance Phase up to Week 30 followed by an open-label period of 24 weeks; and End-of-Study. The screening was carried 15 out between Days -42 and Day O before an initial administration of the study drug, wherein the eligibility of patients for study was evaluated. All the examinations including hepatitis B, hepatitis C and human immunodeficiency virus (HIV-1 and HIV-2) infections, a urine and serum pregnancy test for women of 20 childbearing potential, as well as rheumatoid factor, anticyclic citrullinated peptide, 12-lead ECG, clinical laboratory tests, release etc., were carried out. Also, an interferon-gamma assay (IGRA) and a chest X-ray examination were performed so as to exclude tuberculosis (TB) patients. 25 All the patients enrolled into the clinical trial were 56 CA 03074168 2020-02-26 administered a single dose of the infliximab IV at Weeks O and 2, respectively. Further, the patients were administered folic acid in combination with the MTX and the study drug so that the adverse events associated with the MTX side effects might be 5 minimized and prevented, wherein they were also reminded of taking a maintenance dose of the MTX from beginning to end of clinical trial. Furthermore, the patients were eligible to take following premedication at an investigator's discretion at a time point of 30 60 minutes before a start of the 10 administration of the study drug so that their hypersensitivity reactions to the study drug might be prevented: e.g., antihistamine (equivalent dose of 2 - 4 mg of chlorpheniramine), hydrocortisone, paracetamol and / or nonsedating antihistamine (equivalent dose of 10 mg of cetirizine), but not limited 15 thereto. Those who were administered a full dose of the study drug twice and deemed to have no concerns about safety at the investigator's discretion, were randomly assigned to an infliximab SC which was administered by pre-filled syringe 20 (PFS) with placebo IV or an infliximab IV with placebo SC (PFS) before the administration at Week 6 / Day 42. Such random assignment with regard to administration of the study drug was stratified by country, a serum CRP concentration (same or less than 0.6 mg / dL, or more than 0.6 mg / dL) at Week 2 and a weight 25 (same or less than 100 kg, or more than 100 kg) at Week 6. A 57 CA 03074168 2020-02-26 minimum of 218 patients with active RA were randomly assigned to two clinical trial arms at a ratio of 1: 1, wherein the administration of the study drug was performed until Week 54. A double dummy design was used to maintain blind until Week 30 5 (Table 2). 10 [Table 2] Ann Number Administered Drugs for Clinical Trials Administration method Number of Patients Dose Anni 3mglkg Infliximab IV 100 mg / vial 2 hours IV infusion at least 109 Ann2 120mg lnfliximab SC 120 mg / PFS Single SC injection at least 109 PFS, Pre-filled syringe Those who were assigned to a arm 1 were administered an additional 3 doses of the infliximab IV at Week 6 and subsequently every eight weeks (Weeks 14 and 22) until Week 22, while the placebo SC was administered at Week 6 and subsequently every two weeks until Week 28. After that, the 15 infliximab IV was switched to the infliximab SC (PFS) at Week 30. Then, the infliximab SC (PFS) was administered until Week 54. Those who were assigned to a arm 2 were initially administered the infliximab SC (PFS) at Week 6 and subsequently every two weeks, which continued until Week 54, while the 20 placebo IV was administered at Weeks 6, 14 and 22. The infliximab SC (the placebo SC during a double-blind period) was injected into patients by a healthcare professional 58 CA 03074168 2020-02-26 at each visit (Weeks 6, 14, 22, 24 - 28 (those who visited for PK evaluation), 30, 38, 46 and 54) at a study site. However, in all the other weeks (Weeks 8, 10, 12, 16, 18, 20, 24 - 28 (those who did not visit for PK evaluation), 32, 34, 36, 40, 42, 5 44, 48, 50 and 52), patients were allowed to perform a selfinjection of the infliximab SC (the placebo SC during the double-blind period), if the investigator determined it as suitable after training them for appropriate injection techniques. 10 In a certain country, the infliximab SC was self-injected by an auto-injector (AI) every two weeks starting from Week 46. Evaluations by Self Injection Assessment Questionnaire (SIAQ) prior and after self-injection of Infliximab SC, self-injection assessment checklist, and a potential hazards checklist were 15 performed so that the usability of the infliximab SC (AI) might be evaluated. In case of the part 2, clinical evaluation, blood sampling and study visits for each type were performed in the same way as shown in the part 1 as well as at a point of time 20 specified in an evaluation schedule. 25 Results 1-1. Safety Evaluation Summary of Adverse Events The safety evaluation was performed with regard to 59 CA 03074168 2020-02-26 secondary endpoints in the part 1, i.e., immunogenicity, hypersensitivity monitoring (including delayed hypersensitivity monitoring), measurement of vital signs (including blood pressure, heart and respiration rates, and body temperature), 5 weight, interferon-gamma release assay (IGRA), chest X-ray, hepatitis B, hepatitis C and human immunodeficiency virus (HIV- 1, HIV-2) infectious states, opinions about physical examination, 12-lead ECG, adverse events (hereinafter AEs) (including serious adverse events (hereinafter SAEs)}, adverse 10 events of special interest (infusion-related reaction / hypersensitivity reaction / anaphylactic reaction [Administration-related reaction], delayed hypersensitivity reaction, injection site reaction, infection and malignancies), signs and symptoms of TB, clinical laboratory analysis, 15 pregnancy test, prior and concomitant medication, local site pains using a 10 cm visual analogue scale (VAS), etc. The cumulative safety data included adverse events (and serious adverse events) reported until End-of-Study visit regardless of their correlation with a clinical drug, wherein 20 an overall summary of AEs reported after treatment during a maintenance phase (Weeks 6 to 54) was presented in Table 3. In general, 109 treatment-emergent AEs (hereinafter TEAEs) were reported in 33 patients (68.8%} - nine patients (69.2%) from the IV cohort ( Cohort 1) and 2 4 patients ( 68 . 6%) from the SC 25 total Cohorts (Cohorts 2, 3 and 4) respectively, thus 60 CA 03074168 2020-02-26 indicating that the proportion of the SC total Cohorts was similar to that of the IV cohort. Also, the intensity of most TEAEs was shown as a grade 1 or 2, wherein among all the TEAEs, the AEs reported in total 23 patients (47.9%) were regarded to 5 be related to the study drug. Treatment-emergent SAEs (hereinafter TESAEs) were reported in total six patients (12.5%) - one patient (7.7%) from the IV cohort (Cohort 1) and five patients (14. 3%) from the SC total Cohorts (Cohorts 2 and 4), respectively. Out of 10 the SC Cohorts, the TESAEs were not reported in the cohort 3. The intensity of the TESAEs was shown as the grade 2 or 3, out of which patients regarded to be associated with the study drug were reported for two patients (16. 7%) in the cohort 4. Also, the administration of the study drug was discontinued for one 15 patient (9.1%) in the cohort 2 after the administration at Week 30 as well as two patients (16. 7%) in the cohort 3 after the administration at Weeks 30 and 32 respectively, as the investigator determined them as critical medical events among all the TESAEs. 20 Out of the TEAEs classified as administration-related reactions (ARRs), the infusion-related reaction, hypersensitivity or anaphylactic reactions were reported in total four patients (8.3%) - one patient (7.7%) from the IV cohort (Cohort 1) and three patients (8.6%) from the SC total 25 Cohorts (Cohorts 2 and 3). Out of the TEAEs classified as ARRs, 61 CA 03074168 2020-02-26 the infusion-related reaction, hypersensitivity or anaphylactic reactions were not reported in the cohort 4 out of the SC Cohorts. As the infliximab ARRs was associated with an antidrug antibody (hereinafter ADA) (Remsima SmPC 2017), the 5 presence of the ADA was evaluated for patients having shown ARRs. Patients who had positive results for the ADA and a neutralizing antibody (hereinafter NAb) amounted to total two (each one for the Cohorts 1 and 2). One patient of the cohort 2 was administered the infliximab IV twice during a dose loading 10 period, i.e., at Weeks O and 2, and then administered the infliximab SC total twice, i.e., at Weeks 6 and 8. The ARRs was reported at Weeks 6 and 8, and was identified as positive for the ADA and the NAb at Week 6 and the End-of-Study visit (performed in ten weeks after the visit at Week 8). The ARRs 15 was reported in one patient of the cohort 1 at Week 38, and was identified as positive for the ADA and the NAb at Weeks 30 and 38 as well as at the End-of-Study visit (perfonned in ten weeks after the visit at Week 38). The TEAEs classified as the injection site reaction were 20 reported in total five patients (14.3%) in the SC total Cohorts (Cohorts 2, 3 and 4), wherein the intensity thereof was all shown as the grade 1 or 2. The TEAEs classified as the injection site reaction were not reported in the IV cohort (Cohort 1). The presence of the ADA was also evaluated for 25 patients having shown the injection site reaction, and one 62 CA 03074168 2020-02-26 (Cohort 2) of the five patients have positive results for the ADA and the NAb at a visit at Week 6, i.e., a day before the occurrence of the TEAEs classified as the injection site reaction. 5 Treatment-emergent AEs classified as infection were reported for 5 patients (38.5%) and 13 patients (37.1%) in the IV cohort (Cohort 1) and SC total Cohorts (Cohort 2-4), respectively. TEAEs leading to discontinuation of study drug were 10 reported for six patients (17 .1%) in SC Cohorts (Cohorts 2, 3 and 4), wherein the reported AEs were antiphospholipid syndrome, injection site reaction, ARRs, pulmonary TB and latent TB. In the IV cohort, the TEAEs classified as infection were not reported. 15 No deaths were reported during the study. [Table 3] Cohortl Cohort2 Cohor13 Cohort4 IV3mglkg SC90mg SC120mg SC180mg Total SC (N=13) (N=35) l<N=lll (N=12) l<N=12) Number of Patients with at Least one TEAE(o / o) 9(69.2) 7(63.6) 8 (66.7) 9(75.0) 24(68.6) Related 4(30.8) 5 (455) 7 (58.3) 7 (58.3) 19 (54.3) Unrelated 9(69.2) 5 (45.5) 206,7) 4 (33.3) 11 (31.4) Number of Patients with at Least one 1 (7.7) 2 (18.2) 0 3 (25.0) 5 (14.3) TESAE(%) Related 0 0 0 2(16.7) 2(5.7) Unrelated 1 (7.7) 2 (18.2) 0 1 (8.3) 3 (8.6) Number of Patients with at Least One TEAE cassified as administration-related 1 (7.7) 1 (9.1) 2(16.7) 0 3 (8.6) reactions (%) Number of Patients with at Least One 0 2 (18.2) 1 (8.3) 2(16.7) 5 (14.3) 63 CA 03074168 2020-02-26 TEAE cassified as Injection Site Reaction(%) Number of Patients with at Least One TEAE cassified as infection 5 (38.5) 4 (36.4) 3(25.0) 6(50.0) 13 (37.1) (%) Rela1ed 2(15.4) 1 (9.1) 3(25.0) 3 (25.0) 7(20.0) Number of Patients with at Least One TEAE Leading to Study Drug 0 2 (18.2) 2(16.7) 2 (16.7) 6(17.1) Discontinuation (%) * At each level of summarization, patients were counted once if they reported one or more events. Only the most severe event was counted. The event was considered to be related if the relationship was defined as s 'Definite'. Immunogenicity 'Possible', 'Probable', In general, the proportion of patients with positive ADA results was lower in the SC Cohorts during the study and the 10 majority of patients had negative ADA test results at Week 54. Also there was a trend towards lower rates of ADA positive with increased Infliximab SC dosage. The number of patients who had positive ADA results at Week 54 was 9 (69.2%), 4 (36.4%), 2 (16.7%) and 2 (16.7%} patients from Cohort 1 to 4, respectively 15 (Table 4) . [Table 4) Visit Cohortl Cohortl Cohort3 Cohort4 Total SC IV3mg / kg SC90mg SC120mg SC180mg (N=35) (N=l3) (N=ll) (N=ll) (N=ll) WeekO ADA positive 0 0 0 0 0 64 CA 03074168 2020-02-26 NAbpositive 0 0 0 0 0 Week6 ADA positive 0 2(18.2) 0 0 2(5.7) NAb positive 0 2(18.2) 0 0 2(5.7) Weekl4 ADA positive 5 (38.S) 2(18.2) 1 (8.3) 1 (8.3) 4 (11.4) NAb positive 3 (23.1) I (9.1) 1 (8.3) 0 2(5.7) Week22 ADA positive 7(53.8) 3 (27.3) 2(16.7) 1 (8.3) 6 (17.1) NAb positive 5(38.5) 2(18,2) 1 (8.3) 0 3 (8.6) Week30 ADA positive 9(69,2) 4(36.4) 3 (25.0) 0 7(20.0) NAbpositive 6(46.2) 2(18.2) 1 (8.3) 0 3 (8.6) Week38 ADA positive 9(69.2) 4(36.4) 1 (8.3) 1 (8.3) 6(17.1) NAb positive 6(46.2) 3 (27.3) I (8.3) 0 4(11.4) Week46 ADA positive 7(53.8) 5(45.5) 2(16,7) 0 7(20,0) NAb positive 5 (38.5) 2(18,2) I (8.3) 0 3 {8.6) Week54 ADA positive 9(69.2) 4(36,4) 2 (16.7) 2 (16.7) 8(22.9) NAb positive 5 (38.5) 2(18.2) I (8.3) I (8.3) 4 (11.4) at leastoneADA positive'' 11 / 13 (84.6) 5 / 9(55.6) 4112 (333) 3 / 12(25.0) 12 / 33(36.4) at least one NAb positive** 7 / 13 (53.8) '119(22.2) 1 / 12 (83) 1 / 12(8.3) 4 / 33 (12.1) * ADA, Anti-drug antibody; NAb, Neutralizing antibody ** Among the patients who had never been identified as positive for the ADA and the NAb before the study drug administration at Week 6, only the patients who had ever been 5 identified as positive for the ADA and the NAb even once after the study drug administration at Week 6 were used for the counting. Local Site Pain Assessment Using the Visual Analogue 10 Scale 65 CA 03074168 2020-02-26 The VAS range was from O to 100 mm, with higher scores indicating more severe pain. Slightly higher level of local site pain (VAS) was observed in SC Cohorts (Cohorts 2, 3, 4) compared to IV cohort (Cohort 1) at the time of first SC 5 injection (at Week 6), however, local site pain gradually decreased as Inf liximab SC was injected repeatedly, and lower level of the pain was reported for SC Cohorts (Cohorts 2, 3, 4) compared to IV cohort (Cohort 1). Among the SC Cohorts, the mean local site pain using the VAS of SC 180 mg cohort was 10 slightly higher than other SC cohorts due to receiving double SC injection at one time, but there was a trend that the level of the pain in SC 18 0 mg cohort was lower than that of IV cohort (Cohort 1) {Table 5). 15 [Table 5) Visit Cohort] Cohortl Cohort3 Cohort4 Statistic IV3mg / kg SC90mg SC120mg SC180mg (N=13) (N=ll) (N=ll) (N=ll) Week6 N 8 11 12 12 Mean (Standard Deviation, SD) 9.63 (12.817) 7.09(9,648) 17.71 (21.922) 11.21 (12,496) Median 5.00 2.00 8.00 7.50 Minimum, Maximum 1,39 0,30 0,65 0,35 Week 14 N 10 10 11 12 Mean(SD) 11.70(14.080) 4.20(6.210) 7.82 (8.0'72) 1021 (13.934) Median 7.00 1.25 6.00 5.00 Minimum, Maximum 1,45 0,18 0,23 0,41 Week22 N 13 10 11 12 Mean(SD) 19.15 (32.080) 5.30 (5.912) 6.86 (10.460) 10.17 {10.100) 66 CA 03074168 2020-02-26 Median 3.00 2.25 Minimum, Maximum 0,84 0, 18 Week30 N 13 10 Mean(SD) 13.85 (22.649) 7.55 (10.828) Median 3.00 2.25 Minimum, Maximum 0,77 0,35 Week54 N 12 9 Mean(SD) 5.58 (7.868) 5.22 (5.974) Median 2.00 2.00 Minimum, Maximum 1,26 0, 15 1-2. Therapeutic Efficacy Evaluation Disease activity measured by OAS28 2.00 7.00 0,36 1,31 11 12 4.36 (5.446) 6.08(5.351) 3.00 3.50 0, 17 1, 16 9 8 5.22 (5.094) 9.63 (6,718) 3.00 9.50 0, 17 1, 19 As a result of analyzing DAS28 (C reactive protein; CRP) 5 and DAS28 (erythrocyte sedimentation rate; ESR) at Weeks 2, 6, 14, 22, 30 and 54 in comparison with baseline as a secondary efficacy endpoint, there was no notable differences between the infliximab SC Cohorts with three different doses and the infliximab IV cohort, wherein it was also identified that 10 actual values tended to decrease as time went by. Actual values and changes from baseline in disease activity measured by DAS28 are summarized in Table 6 (CRP) and Table 7 (ESR). The mean scores for disease activity measured by DAS28 decreased from Baseline at Weeks 2, 6, 14, 22, 30 and 54 15 in each cohort. There was a trend towards slightly lower than IV cohort DAS28(CRP) score in the SC Cohorts from Week 22 and DAS28 (ESR) score in the SC Cohorts from Week 30, which was consistent with the higher Ctrough concentrations in the SC 67 CA 03074168 2020-02-26 Cohorts. [Table 6] IV3mwt<g SC90mg SC120mg SC180mg (N=13) (N=ll) (N=l2) (N=12) Visit Actual Change Actual Change Visit Actual Change Actual Sta1istic Result from Result from Statistic Result from Result Baseline Baseline Baseline Baseline n 13 11 12 12 Mean 5.413 6.273 5.719 5.527 SD 0.7776 0.8234 0.9120 0.8185 Minimum 4.11 5.13 4.53 4.62 Median 5.355 6.265 5.492 5.299 Maximum 6.68 7.46 7.31 7.10 Week2 n 13 13 11 11 12 12 12 12 Mean 4.328 -1.086 5.030 -1.243 4.421 -1.297 4.230 -1297 SD 1.5161 0.9000 1.3922 1.2509 0.8815 0.5899 1.2647 0.8990 Minimum 1.71 -2.41 2.27 -4.09 3.39 -2.10 2.60 -2.94 Median 4.661 -1.143 5.367 -1.191 4.067 -1.206 4.317 -1.206 Maximum 6.59 0.34 6.35 0.24 6.48 -0.23 6.59 -0.04 Week6 n 13 13 11 11 12 12 11 11 Mean 3.902 -1.512 4.600 -1.673 3.921 -1.798 3.419 -2.007 SD 1.4765 0.9278 1.0735 0.7104 1.1911 0.8442 l.1775 0.9631 Minimum 1.82 -2.75 2.90 -2.37 2.55 -3.25 1.56 -3.97 Median 4.414 -1.451 4.663 -1.919 3.323 -1.890 3.370 -2.004 Maximum 6.37 -0.28 6.24 -0.03 6.28 -0.43 5.09 -0.27 Week 14 n 13 13 10 10 11 11 12 12 Mean 3.558 -1.856 3.968 -2296 3.446 -2255 2.933 -2.594 SD 1.2612 0.8621 1.2485 0.8131 1.3406 1.1376 1.1779 0.8486 Minimum 1.92 -2.89 1.84 -3.43 1.39 -4.41 1.50 -4.00 Median 3.549 -2.102 3.740 -2.392 3.223 -1.881 2.702 -2.665 Maximum 6.15 -0.52 5.58 -1.18 5.83 -0.89 5.63 -1.00 Week22 n 13 13 10 10 11 11 12 12 Mean 3.885 -1.529 3.730 -2.534 3.257 -2.444 2.789 -2.738 SD 1.6167 1.3228 1.0430 0.8491 1.4077 1.2380 1.3266 0.8753 68 CA 03074168 2020-02-26 Minimum 1.86 -3.33 1.69 -4.07 1.50 -4.35 1.11 -3,95 Median 4,066 -1.404 3.626 -2.324 2.977 -1.989 2.606 -2.922 Maximum 6.74 1.38 5.27 -1.45 5.79 -1.07 5.53 -1.10 Week30 n 13 13 10 10 10 10 12 12 Mean 3.315 -2.099 3.029 -3.236 3.105 -2.586 2.741 -2.786 SD 1.2515 0.8499 1.1446 1.2430 1.0076 0.9749 0.9661 0.5621 Minimum I.80 -3.02 1.35 -6.11 1.77 -4.56 1.15 -3.79 Median 3.150 -2.312 2.917 -2.931 3.038 -2.345 2.831 -2.668 Maximum 6.41 0.26 4.78 -1.81 4.74 -1.18 4.51 -2.04 Week54 n 12 12 8 8 10 10 10 IO Mean 3.548 -1.961 3.025 -3.090 3.167 -2.545 2.911 -2.505 SD 1.1928 1.0766 1.0242 0.7390 0.9706 1.3996 0.9929 0.9279 Minimum 1.26 -3.60 1.57 -4.44 1.35 -4.46 1.11 -3.51 Median 3.685 -1.742 2.770 -3.025 3.463 -2.585 2.877 -2.866 Maximum 5.28 0.08 4.58 -1.93 4.60 0.00 4.31 -0.55 [Table 7] IV3mglkg SC90mg SC120mg SC180mg (N=13) (N=ll) (N=12) (N=l2) Visit Actual Change Actual Change Visit Actual Change Actual Stamtic Result from Result from Statmic Result from Result Baseline Baseline Baseline Baseline n 13 11 12 12 Mean 6.031 7.091 6.410 6.362 SD 0.8940 0.8481 1.1642 0.8497 Minimum 3.85 5.33 4.54 5.04 Median 6.009 7.182 6.360 6.318 Maximum 7.41 8.18 8.11 7.98 Week:2 n 13 13 11 11 12 12 12 12 Mean 4.970 -1.061 5.773 -1.317 5.203 -1207 5.019 -1.343 SD 1.7649 0.9720 1.8342 1.4313 1.3003 0.8837 1.3065 0.9234 Minimum 1.31 -2.55 1.93 -4.86 3.22 -3.35 3.43 -3.19 Median 5.481 -0.816 6.433 -1.116 5.073 -1.014 4.793 -1.285 Maximum 7.51 0.44 7.51 0.10 8.04 -0.07 7.61 -0.01 Week6 n 13 13 11 11 12 12 12 12 69 CA 03074168 2020-02-26 Mean 4.4% -1.535 5.387 -1.704 4.685 -I.725 4.418 -l.944 SD 1.5015 0.8285 1.1940 0.6497 1.3766 1.0068 1.4161 1.0233 Minimum 2.13 -2.78 2.88 -2.45 3.27 -3.37 2.25 -4.38 Median 4.714 -l.151 5.331 -1.775 4.184 -1.551 4.361 -1.919 Maximum 7.35 -0.06 7.09 -0.35 7.66 -0.03 120 -0.46 Week 14 n 13 13 10 10 11 11 12 12 Mean 4.236 -1.795 4.830 -2291 4.306 -2.081 3.740 -2.621 SD 1.2772 0.7825 1.4762 0.9005 1.3940 1.3178 1.1732 0.7395 Minimum 2.32 -3.14 1.77 -3.56 2.68 -4.16 2.14 -3.94 Median 4.065 -1.588 4.821 -2288 4220 -1.395 3.417 -2.732 Maximum 6.88 -0.53 6.48 -0.97 7.00 -0.32 6.48 -1.19 Week22 n 13 13 10 10 11 11 12 12 Mean 4.354 -1.677 4.515 -2.606 3.875 -2.512 3.380 -2.981 SD 1.8065 1.4558 1.2611 0.8066 1.8028 1.7593 1.1641 0.6857 Minimum 1.60 -4.02 1.57 -3.76 0.60 -6.28 1.85 -3.96 Median 4.267 -l.479 4.483 -2.470 3.890 -1.706 2.989 -2.908 Maximum 7.75 1.76 5.90 -1.59 6.67 -0.57 5.97 -1.70 Week30 n 13 13 10 10 10 10 12 12 Mean 3.866 -2.165 3.669 -3.452 3.776 -2.562 3.318 -3.044 SD 1.3425 0.9643 1.3555 I.1242 1.1186 1.24% l.0164 0.5380 Minimum l.83 -3.79 1.15 -5.65 2.02 -4.63 1.54 -3.79 Median 4.156 -2.226 3.517 -3239 3.642 -2.401 3.088 -2.992 Maximum 6.72 -0.03 5.32 -1.81 5.55 -0.69 5.38 -1.98 Week54 n 12 12 9 9 11 11 10 10 Mean 4.134 -2.078 3.984 -3.129 4.067 -2.320 3.434 -2.847 SD 1.3522 1.2491 1.1889 0.7665 0.9426 1.7582 1.1128 0.8623 Minimum 1.92 -3.67 1.55 -4.68 2.24 -4.34 1.13 -3.91 Median 4.112 -2.001 4.305 -3.I 17 4.337 -2.602 3284 -2.970 Maximum 6.50 0.38 5.47 -2.00 5.45 0.91 4.87 -1.16 The EULAR responses The proportion of patients with a good or moderate response, defined according to the EULAR (European League 5 Against Rheumatism) response criteria using DAS28 (CRP) during 70 5 CA 03074168 2020-02-26 the study was similar among Cohorts (Table 8). The results of EULAR response criteria using DAS28 (ESR) response were also similar among Cohorts during the study (Table 9). (Table 8] Visit IV3ml'kg SC90mg SC110mg SC180mg Statistic (N=13) (N=ll) (N=l2) (N=12) Week2 Number of patients responded(%) 7 (53.8) 6(54.5) 10 (83.3) 8 (66.7) - Moderate Response 3 (23.1) 4(36.4) 10 (83.3) 4 (33.3) - Good Response 4(30.8) 2 (18.2) 0 4 (33.3) Week6 Numberofpatientsresponded(%) 9(69.2) 9(81.8) 10(83.3) 10(88.3) - Moderate Response 4(30.8) 8(72.7) 5 (41.7) 6(50.0) - Good Response 5 (38.5) 1 (9.1) 5 (41.7) 4 (33.3) Week 14 Number of patients responded(%) 12(92.3) 9(81.8) 10(83.3) 11 (91.7) - Moderate Response 6(46.2) 7(63.6) 5 (41.7) 2 (16.7) . Good Response 6(46.2) 2(18.2) 5 (41.7) 9(75.0) Week22 Number of patients responded(%) 10(76.9) 10(90.9) 10(83.3) 11 (91.7) - Moderate Response 5 (38.5) 8(72.7) 3 (25.0) 4 (33.3) - Good Response 5 {38.5) 2(18.2) 7 (58.3) 7 (58.3) Week30 Numberofpatientsresponded(%) 12 (92.3) 10(90.9) 10(83.3) 12(100.0) - Moderate Response 5 (38.5) 5 (45.5) 5 (41.7) 5 (41.7) - Good Response 7 (53.8) 5(45.S) S (41.7) 7 (58.3) Week54 Numberofpatientsresponded(%) 11 (84.6) 8(72.7) 9(75.0) 9 (75.0) - Moderate Response 7 (53.8) 3 (27.3) 6(50.0) 3 (25.0) - Good Response 4(30.8) 5(45.5) 3 (25.0) 6(50.0) [Table 9] Visit IIV3ml'kg ISC90mg ISC110mg ISC180mg Statistic (N=13) (N=ll) (N=12) (N=12) Week2 Number of patients responded(%) 16(46.2) IS (45.5) 17 (58.3) 19(75.0) 71 CA 03074168 2020-02-26 - Moderate Response 4(30.8) 3 (27.3) 7 (58.3) 9(75.0) . Good Response 2 (15.4) 2(18.2) 0 0 Weclc6 Number of patients responded(%) 8 (61.5) 9(81.8) 10 (83.3) 10(83.3) - Moderate Response 5 (38.5) 8(72.7) 10(83.3) 8(66.7) . Good Response 3 (23.1) 1 (9.1) 0 2(16.7) Weclc 14 Number of patients responded(%) 11 (84.6) 8(82.7) 9(75.0) 11 (91.7) - Moderate Response 8 (61.5) 7(63.6) 6(50.0) 6(50.0) . Good Response 3 (23.1) I (9.1) 3 (25.0) 5 (41.7) Weclc22 Number of patients responded(%) 10(76.9) 10(90.9) 10 (83.3) 12(100.0) - Moderate Response 6(46.2) 9(81.8) 6(50.0) 6(50.0) - Good Response 4(30.8) I (9.1) 4 (33.3) 6(50.0) Weclc30 Numberofpatientsresponded(%) 12(92.3) l0(90.9) IO (83.3) 12(100.0) . Moderate Response 7(53.8) 6(54.5) 8(66.7) 4 (33.3) . Good Response 5 (38.5) 4(36.4) 2(16.7) 8(66.7) Week54 Number of patients responded(%) 11 (84.6) 9(81.8) 9(75.0) 9(75.0) . Moderate Response 9(69.2) 8(72.7) 7 (58.3) 5 (41.7) . Good Response 2(15.4) I (9.1) 2 (16.7) 5 (41.7) Proportion of Patients Achieving Clinical Response according to the ACR20 The proportion of patients achieving clinical response 5 according to the ACR20 (American College of Rheumatology 20% improvement) criteria from Week 14 to Week 54 were similar between IV cohort (Cohort 1) and SC Cohorts (Cohort 2, 3, 4) (Table 10). (Table 10) Parameter Cohortl Cohortl Cohort3 Cohort4 Visit IV3mg / kg SC90mg SC120mg SC180mg (N=13) (N=ll) (N=ll) (N=12) 72 CA 03074168 2020-02-26 ACR20 Week:2 4 (30.8) 3 (27.3) 4(33.3) 6(50.0) Week:6 8 (61.5) 8(72.7) 7 (58.3) 7 (58.3) Week 14 10(76.9) 8(72.7) 8 (66.7) II {91.7) Week:22 8 (61.5) 8(72.7) 9(75.0) 11 (91.7) Week:30 11 (84.6) 10(90.9) 10(833) 12(100.0) Week:54 9 (69.2) 9{81.8) 8 (66.7) 10(83.3) Example 2. Modeling for subcutaneously administering an infliximab to RA patients PK-PD Model Construction 5 A pharmacokinetic-pharmacodynamic (PK-PD) model for the infliximab subcutaneous (SC) administration was established to integrate with a quantitative pharmaco)dnetic (PK) model not only for simulating the PK of future administered doses and regimens, but also for simulating the efficacy and safety of 10 the infliximab SC. The PK-PD model was based on the infliximab IV administration data on healthy volunteers, ankylosing spondylitis (AS) patients, rheumatoid arthritis (RA) patients and Crohn's disease (CD} patients, as well as the infliximab SC administration data on CD patients, RA patients and healthy 15 volunteers (Clinicaltrials.gov Identifier Code NCT01220518, NCT01217086, NCT02096861). The PK-PD model constructed based on the said data may be used to simulate the subcutaneous administration results for patients having the infliximab indications (RA, ulcerative 20 colitis (UC), CD, plaque psoriasis, psoriatic arthritis or ankylosing spondylitis). 73 CA 03074168 2020-02-26 The PK-PD modeling analysis was performed by a nonlinear mixed effect modeling approach. The data analysis commenced by a 1-compartment model including a proportional elimination of a proportional error model, and then a final model was performed 5 by a 2-compartment model having a linear elimination from a central compartment. All the models on pharmacokinetics were variablized in terms of clearance (CL) and volume of distribution. As for the final PK model, a profile was predicted in 10 such a way that each estimated value for area under the concentration-time curve (AUCtau) and minimum concentration immediately before the next study drug administration (Ctrough) parameters with regard to the inf liximab clinical trial was applied to each actual dose, usage and administration route, 15 wherein the said data were descriptively summarized with a median value and a confidence interval of 90%. Also, an additional simulation was performed so as to evaluate an effect on a fixed dose, usage and administration route for each weight. The PK-PD modeling and simulation of subcutaneous doses were 20 performed by means of NONMEM v7.2. Dose-regimen scenario of SC dosage form for modeling in RA patients A pharmacokinetic aspect was predicted based on a following simulation scenario, wherein accordingly efficacy and 25 safety were predicted, and then evaluated in comparison with an 74 5 CA 03074168 2020-02-26 infliximab IV infusion usage, in which a maintenance dose of 3 mg / kg was administered at an interval of eight weeks (Table 11) : (Table 11] Infliximab SC 120 mg Every 2 weeks lnfliximab SC 120 mg Every 4 weeks Infliximab SC 180 mg Every 4 weeks Estimated values for inf liximab exposure parameters on infliximab SC dose and usage for each weight of RA patients Exposure pharmacokinetic parameters (AUCH Ctrough and Cm.ix) 10 on infliximab SC dose and usage were simulated in such a way that a weight range of 50 - 130 kg was divided into each unit of 10 kg, wherein the estimated values for Ctrough and AUC, of infliximab SC exposure for each weight showed a correlation 15 with a drug dosage (Table 12). (Table 12] Compariso N Paramete C&rooalt n(a) r Geometr Ratio of 900 / oCI icLS Geometr ofRatio mean icLS (0 / o) means Test: 120 m& SC at 2 wee!m: inteo:als xs Bd'm!!J:e tb> All weight 112 SC 13.4 10.13 9.53;10.7 5 IV lJ 8 50-60kg 100 SC 16.l 11.67 9.23;14.7 IV 1.4 6 60-70kg 100 SC 15.4 9.14 7.31;1 l.4 IV 1.7 3 70-80kg 100 SC 13.3 8.65 7.01;10.6 IV 1.5 7 75 AUCr Cmu Geometr Ratio of 900 / oCI Geometr Ratio of 900 / oCI icLS Geometr ofRatio icLS Geometr ofRatio mean icLS (%) mean icLS (%) means means 22492 1.37 1.33;1.40 18.8 0.25 0.25;0.26 16467.2 74.8 26855.2 1.69 1.54;1.85 22.4 0.33 0.31;0.35 15893.l 68 25450.4 1.44 1.32;1.58 21.1 0.29 0.27;0.31 17660.9 733 22143 1.25 1.15;135 18.4 0.24 0.22;0.25 17751.1 77.6 CA 03074168 2020-02-26 80-90kg 100 SC 11.9 8.16 6.61;10.0 20002.3 I.II 1.02;1.20 16.7 0.21 0.19;0.22 IV 1.5 7 18037 81 90-lOOkg 100 SC 11 7.25 5.91;8.90 18518.3 0.99 0.91;1.07 15.S 0.18 0.17;0.20 IV 1.5 18754.6 84 100-ll0kg 100 SC 10.3 6.85 5.53;8.49 17386.5 0.9 0.82;0.98 14.5 0.16 0.15;0.18 IV 1.5 19379.7 88.3 110-120kg 100 SC 10.1 5.74 4.57;7.22 16873 0.82 0.75;0.89 14 0.16 0.15;0.17 IV I.8 20696.5 89.8 120.130kg 100 SC 10 4.78 3.99;5.72 16620.2 0.75 0.70;0.81 13.8 0.15 0.14;0.16 IV 2.1 22191.7 94.1 Test 120 ma:; SC at 4 weeW,I intervals vs Reference tb> All weight 112 SC 4.3 3.24 3.04-3.46 11280.7 0.69 0.67-0.70 11.6 0.15 0.IS;0.16 5 IV 1.3 16467.2 74.8 50-oOkg 100 SC 5.1 3.8 3.@;4.68 13169.4 0.86 0.79;0.92 13.4 0.2 0.19;0.21 IV 1.3 15378.9 66.3 60-70kg 100 SC 4.3 3.57 2.81;4.54 11414.3 0.73 0.67;0.79 11.7 0.17 0.16;0.18 IV 1.2 15670.8 70.5 70-80kg 100 SC 4.2 2.93 2.31;3.72 10878.8 0.63 0.58;0.69 11.1 0.15 0.14;0.16 IV 1.4 17260.6 75.8 80-90kg 100 SC 4 2.49 2.02,;3.07 10230.8 0.55 O.Sl;0.60 10.4 0.13 0.12;0.14 IV 1.6 18448.9 80.6 90-lOOkg 100 SC 3.2 2.56 2.05;3.19 8676.4 0.5 0.46;0.54 9 0.11 0.11;0.12 IV 1.2 17419.8 80.7 100-llOkg 100 SC 3.5 2.01 1.61;2.52 9106.1 0.45 0.41;0.49 9.2 0.1 0.10;0.1 l IV 1.8 20263.6 88.3 110-120kg 100 SC 3.5 1.74 1.38;2.19 8906 0.41 0.38;0.45 8.9 0.1 0.@;0.11 IV 2 21633 89.4 120.130kg 100 SC 3.2 1.67 1.34;2.07 8200 0.38 0.35;0.41 8.3 0.09 0.08,-0.09 IV 1.9 21756.9 94.1 Tm: 180 ma:;SC at4weeklv~rvalsvs Rd,renceOO All weight 112 SC 6.4 4.86 4.55-5.18 16904.6 1.03 1.00-1.05 17.3 0.23 0.23;0.24 5 IV 1.3 164672 74.8 50-oOkg 100 SC 7.8 5.77 4.48;7.44 20079.1 1.28 1.17;1.41 20.4 0.31 0.29;0.32 IV 1.3 15688.4 66.7 60-70kg 100 SC 6.8 4.94 4.04;6.05 17638 1.08 I.01;1.16 18 0.31 0.29;0.32 IV 1.4 16310.1 72.1 70-80kg 100 SC 5.9 4.66 3.63;5.99 15874.1 0.94 0.86;1.03 16.3 0.22 020;0.23 IV 1.3 16812 76 80-90kg 100 SC 5.6 3.97 3.24;4.87 14770.l 0.83 0.77;0,90 15.2 0.19 0.18;0.20 IV 1.4 17720.6 80.5 90-lOOkg 100 SC 5.9 3.11 2.52;3.84 14659.7 0.75 0.69;0.81 14.7 0.18 0.17;0.19 76 5 CA 03074168 2020-02-26 IV 1.9 19596.1 80.4 100-ll0kg 100 SC 5.2 3.04 2.37;3,91 13442.9 0,67 0.61;0.74 13.6 0.16 0.15;0.17 IV 1.7 19982.3 85.1 110-120kg 100 SC 4.4 3.04 2.42;3.83 11861.8 0.61 0.57;0.66 12.2 0.14 0.13;0.15 IV 1.5 19353.4 87.9 120-130kg 100 SC 4.7 2.58 2.05;3.24 12121.8 0.57 0.52;0.62 12.3 0.13 0.12;0.14 IV 1.8 21419.9 93.4 Note: (a) All patients received 3 mwt<g infliximab via IV infusion over 2 hours at Weeks O and 2, prior to maintenance regimen commencing at Week 6 (in both tert and refermce periods of the cross-over). (b) Reference treatment com(lised of3 mwt<g every 8 weeks infliximab via IV infusion over 2 hours (maintenance regimen). ( c) geometric LS means ratio=test / reference Abbreviations: CI:Confidence Interval, LS:Least Square, SD:Standard Deviation Example 3. Evaluation of safety and therapeutic efficacy on subcutaneously administering an infliximab to CD or UC patients The present clinical trial of an infliximab was an openlabel, randomized, multi-center, parallel-group and phase I trial designed to evaluate pharmacokinetics, efficacy and safety between the infliximab SC and the infliximab IV in patients with active CD or active UC until Week 54, wherein the 10 present clinical trial was composed of two parts. A part 1 was designed to find an optimal dose of the infliximab SC in CD patients, wherein the optimal dose of the infliximab SC corresponding to 5 mg / kg of the infliximab IV over the first 30 weeks was identified by means of an area 15 under the concentration-time curve (AOC,) at steady state between Weeks 22 and 30. In case of the part 1, a clinical trial period amounted to a maximum of 65 weeks, inclusive of duration from a screening (the maximum three weeks) to End-of- 77 CA 03074168 2020-02-26 Study visit. A part 2 was designed to find that the infliximab SC was not inferior to the infliximab IV in the CD or UC patients in terms of pharmacokinetics, which would be proved by means of a S concentration before the administration (Ctrough) at Week 22. In case of the part 2, the optimal administered dose and dosing interval of the infliximab SC corresponding to 5 mg / kg of the infliximab IV were determined as follows based on the pharmacokinetics, efficacy, pharmacodynamics and safety data 10 over the first 30 weeks of the part 1 by recommendations of the Data Safety Monitoring Board (DSMB): • Patients weighing less than 80 kg: Administered 120 mg of the infliximab SC at an interval of two weeks; and • Patients weighing 80 kg or more: Administered 240 mg of IS the infliximab SC at an interval of two weeks. Part 1 Patients were eligible to enroll into the present clinical trial, provided that they met all of the following 20 criteria: * Patient who had Crohn' s disease with a score on the CDAI of 220 to 450 points; * Patient who had Crohn's disease of at least 3 months' disease duration prior to the first administration of the study 25 drug (Day 0); and 78 CA 03074168 2020-02-26 * Patient who had been treated for active Crohn's disease but had not responded despite a full and adequate course of therapy with a corticosteroid and / or an immunosuppressant; or who was intolerant to or had medical 5 contraindications for such therapies. Patients were not eligible to enroll into the clinical trial, provided that they met any one of the following criteria: * Patient who had previously received a biological 10 agent for the treatment of Crohn's disease or Ulcerative colitis and / or a TNFcx (tumor necrosis factor-alpha) inhibitor for the treatment of other disease; * Patient who had allergies to any of the excipients of infliximab or any other murine and / or human proteins, or 15 patient with a hypersensitivity to immunoglobulin product; * Patient who had active entero-vesical, enteroretroperitoneal, entero-cutaneous, and entero-vaginal fistulae within 6 months prior to the first administration of the study drug (Day 0). Entero-enteral fistulae without clinical 20 significant symptoms upon investigator's opinion and anal fistulae without draining problems were allowed; and * Patient who had taken more than 3 small-bowel resection procedures prior to the first administration of the study drug (Day 0). 25 The present clinical trial was composed of three clinical 79 CA 03074168 2020-02-26 trial periods: Screening; Treatment Period; and End-of-Study. The screening was carried out between Days -21 and -1 before the initial administration of the study drug, wherein the eligibility of patients for study was evaluated. All the 5 examinations including hepatitis B, hepatitis C and human immunodeficiency virus (HIV-1 and HIV-2) infections, a urine and serum pregnancy test for women of childbearing potential, as well as colonoscopy, CRP, 12-lead ECG, clinical laboratory tests, etc., were carried out. Also, an interferon-gamma 10 release assay (IGRA) and a chest X-ray examination were performed so as to exclude tuberculosis (TB) patients. Patients who met all the inclusion criteria at Week 0 / Day 0 and did not correspond to any of the exclusion criteria were enrolled into the clinical trial, wherein all the enrolled 15 patients were administered a single dose of the infliximab IV twice at Weeks O and 2. The patients were eligible to take following premedication at the investigator's discretion at a time point of 30 60 minutes before a start of the administration of the study drug so that their hypersensitivity 20 reactions to the study drug might be prevented: e.g., antihistamine (equivalent dose of 2 - 4 mg of chlorpheniramine), hydrocortisone, paracetamol and / or nonsedating antihistamine (equivalent dose of 10 mg of cetirizine), but not limited thereto. 25 Those who were administered a full dose of the study drug 80 CA 03074168 2020-02-26 twice and deemed to have no concerns about safety at the investigator's discretion, were randomly assigned to an infliximab SC cohort or an infliximab IV cohort before an administration at Week 6 / Day 42. Such random assignment with 5 regard to administration of the study drug was stratified by means of a region (Europe or non-Europe), Current use of treatment with azathioprine (AZA) or 6-mercaptopurine (6-MP) or methotrexate (MTX) (used or not used) , a presence of clinical responses by means of CDAI-70 at Week 6, and a weight (equal to 10 or less than 70 kg, or more than 70 kg) at Week 6. A total of 45 patients with active CD were enrolled, out of which 44 ones were randomly assigned to four clinical trial Cohorts at a ratio of 1:1:1:1, wherein the administration of the study drug was performed until Week 54 (Table 13). 15 (Table 13] Cohort Number Admimstered Drugs for Clinical Trials Administration method Numberof Dose Patients Cohort 1 Smll' / k:e: lnfliximabIV lOOmu / vial 2 hours IV infusion 13 Cohort2 120mg Infliximab SC 120 mu / PPS Single SC iniection 11 Cohort3 l80m.2 lnfliximab SC 90 mll:!PFS Double SC injection 12 Cohort4 240m2 lnfliximab SC 120 mll: / PFS Double SC iniection 8 PFS, Pre-filled syringe Those who were assigned to a cohort 1 were administered 20 additional 7 doses of the infliximab IV at Week 6 and subsequently every eight weeks (Weeks 14, 22, 30, 38, 46 and 54). Those who were assigned to Cohorts 2, 3 and 4 were 81 CA 03074168 2020-02-26 initially administered the infliximab SC at Week 6 and then additionally administered the infliximab SC every two weeks until Week 54. The initially assigned dose was adjusted to the optimal dose in all patients from Cohorts 2, 3 and 4 when the 5 optimal dose was confirmed after dose finding. After that, an additional SC injection using the optimal dose was administered until Week 54. The infliximab SC was injected into patients by a healthcare professional at each visit (Weeks 6, 8, 10, 14, 22, 24, 26, 28, 30, 38, 46 and 54) at a study site. However, in all 10 the other weeks (Weeks 12, 16, 18, 20, 32, 34, 36, 40, 42, 44, 48, 50 and 52), patients were allowed to perform a selfinjection of the infliximab SC, if the investigator determined it as suitable after training them for appropriate injection techniques. 15 Patients visited the study site at a predefined time interval for clinical evaluation and blood sampling. At each visit, they were asked questions about adverse events and concomitant medication, while being monitored for clinical signs and symptoms of TB. The evaluation of primary 20 pharmacokinetic endpoints was performed during a maintenance phase between Weeks 22 and 30, then the evaluation of secondary pharmacokinetic endpoints was performed during a treatment period until Week 54, and then blood sampling for analysis as well as the evaluation of efficacy, PD and safety were 25 respectively performed at a point of time specified in an 82 CA 03074168 2020-02-26 evaluation schedule. The End-of-Study visit was performed in eight weeks after the end of the maintenance phase. However, it was performed in eight weeks after the last time point of administration when 5 patients discontinued the clinical trial halfway. In case of dropout patients, all the clinical trial procedures were perf armed on a day of dropout or on the next day after such dropout, wherein every effort was made to complete all the Endof- Study evaluations at a time point of eight weeks after the to last administration to patients. Part 2 A part 2 would commence based on a review by the Data Safety Monitoring Board with regard to PK modeling report data 15 including PK, efficacy, PD and safety data, which were identified over the first 30 weeks in the part 1. Patients would be eligible to enroll into the part 2 of the present clinical trial, provided that they met all the following criteria: 20 In case of active CD patients - * Patient who had Crohn' s disease with a score on the CDAI of 220 to 450 points; * Patient who had Crohn's disease of at least 3 months' disease duration prior to the first administration of the study 25 drug (Day 0); and 83 CA 03074168 2020-02-26 * Patient who had been treated for active Crohn's disease but had not responded despite a full and adequate course of therapy with a corticosteroid and / or an immunosuppressant; or who was intolerant to or had medical 5 contraindications for such therapies. * They satisfied at least one of the following items: A serum C-reactive protein (CRP) concentration was more than 0.5 mg / dL; A fecal calprotectin was more than 100 μg / g; and IO Ileal-colonic CD patients had a colonoscopy (SES-CD) 15 score of 6 points or higher in, or ileal or colonic CD patients had such score of 4 points or higher and had an ulcer score for at least one segment. In case of active UC patients - * Patient who had active Ulcerative colitis as defined by a total Mayo score between 6 and 12 points with endoscopic evidence of active colitis as indicated by endoscopic subscore of ;;;;:; 2 at Screening; * Patient who had Ulcerative colitis of at least 3 20 months' disease duration prior to the first administration of the study drug (Day 0); and * Patient who had been treated for active Ulcerative colitis but not responded despite conventional therapy including corticosteroids alone or in combination with 6-MP or 25 AZA and medications containing 5-ASA, or who is intolerant to 84 CA 03074168 2020-02-26 or has medical contraindications for such therapies. Patients would not be eligible to enroll into the part 2 of the clinical trial, provided that they met any one of the following criteria: 5 * Patient who has previously received a biological agent for the treatment of CD or UC and / or a TNF~ inhibitor for the treatment of other disease; * Patient who has allergies to any of the excipients of infliximab or any other murine and / or human proteins or patient 10 with a hypersensitivity to immunoglobulin product; * Patient who had active entero-vesical, enteroretroperi toneal, entero-cutaneous, and entero-vaginal fistulae within 6 months prior to the first administration of the study drug (Day O) . Entero-enteral fistulae without clinical 15 significant symptoms upon investigator's opinion and anal fistulae without draining problems were allowed; * Patient who had taken more than 3 small-bowel resection procedures prior to the first administration of the study drug (Day 0); and 20 * Patient who had been taking rectally administered medications containing corticosteroids or 5-ASA for the treatment of ulcerative colitis within 2 weeks prior to Screening. The part 2 would be composed of three clinical trial 25 periods: Screening; Treatment Period; and End-of-Study. The 85 CA 03074168 2020-02-26 screening would be carried out between Days -42 and O before an initial administration of the study drug, wherein the eligibility of patients for study would be evaluated. All the examinations including hepatitis B, hepatitis C and human 5 immunodeficiency virus (HIV-1 and HIV-2) infections, a urine and serum pregnancy test for women of childbearing potential, as well as colonoscopy (CD patients), flexible proctosigmoidoscopy (UC patients), CRP, 12-lead ECG, clinical laboratory tests, etc., would be carried out. Also, an IO interferon-gamma release assay ( IGRA) and a chest X-ray examination would be performed so as to exclude tuberculosis (TB) patients. Patients who met all the inclusion criteria at Week 0 / Day O and did not correspond to any of the exclusion criteria would 15 be enrolled into the clinical trial, wherein all the enrolled patients would be administered a single dose of the infliximab IV twice at Weeks O and 2 . The patients would be eligible to take following premedication at an investigator's discretion at a time point of 30 - 60 minutes before a start of the 20 administration of the study drug so that their hypersensitivity reactions to the study drug might be prevented: e.g., antihistamine (equivalent dose of 2 - 4 mg of chlorpheniramine), hydrocortisone, paracetamol and / or nonsedating antihistamine (equivalent dose of 10 mg of cetirizine), but not limited 25 thereto. 86 CA 03074168 2020-02-26 Those who were administered a full dose of the study drug twice and deemed to have no concerns about safety at the investigator's discretion, were randomly assigned to an infliximab SC arm or an inflixirnab IV arm before administration 5 at Week 6 / Day 42. Such random assignment with regard to administration of the study drug would be stratified by a current use of azathioprine or 6-mercaptopurine or MTX treatment, a disease (CD or UC), a presence of CD clinical responses by means of CDAI-70 or UC clinical responses by means 10 of partial Mayo score at Week 6 and a weight (less than 80 kg, or 80 kg or more) at Week 6. A minimum of 130 patients with active CD or active UC would be randomly assigned to two clinical trial arms at a ratio of 1: 1, wherein the administration of the study drug would be performed until Week 15 54 (Table 14). 20 (Table 14] Ann Number Administered Dose Drugs for Clinical Trials Administration method Number of Patienu Arml 5~ infliximabIV IOOmg / vial 2 hours N infusion Atleam65 Arm2 120 mg( <80 kg) infliximab SC 120 m)VPFS Single SC injection Atleam65 240 mg(?:80 kg) infliximab SC 120 mg!PFS Double SC injection PFS, Pre-filled syringe Those who were assigned to an arm 1 would be additionally administered the infliximab IV at Week 6 and subsequently every eight weeks (Weeks 14 and 22) until Week 22. After that, the 87 CA 03074168 2020-02-26 infliximab IV would be switched to the infliximab SC administration from Week 30, wherein an SC dose would be determined based on a weight at Week 30. This dose would be administered every two weeks until Week 54. As for those who 5 were assigned to an arm 2, an SC dose of the infliximab SC would be determined based on a weight at Week 6, wherein this dose would be administered every two weeks from Weeks 6 to 54. An increase in the dose would be permitted according to the investigator's judgment after Week 30. The infliximab SC was 10 injected into patients by a healthcare professional at each visit (Weeks 6, 14, 22, 24, 26, 28, 30, 38, 46 and 54) at a study site. However, in all the other weeks, patients would be allowed to perform a self-injection of the infliximab SC, if the investigator determined it as suitable after training them 15 for appropriate injection techniques. The evaluation of primary pharmacokinetic endpoints would be performed at Week 22 and then the evaluation of secondary pharmacokinetic endpoints would be performed during a maintenance phase between Weeks 22 and 30 and during a 20 treatment period until Week 54. Blood sampling for analysis as well as the evaluation of efficacy, PD and safety would be respectively performed at a point of time specified in an evaluation schedule. The End-of-Study visit would be performed in two weeks 25 after the end of the maintenance phase. However, it would be 88 CA 03074168 2020-02-26 performed in two weeks after the last time point of administration when patients discontinued the clinical trial halfway after the SC administration. However, it would be performed in eight weeks after the last time point of 5 administration when patients discontinued the clinical trial halfway after the IV administration. In case of dropout patients, all the clinical trial procedures would be performed on a day of dropout or on the next day after such dropout, wherein every effort would be made to complete all the End-of- 10 Study evaluations at a predetermined point of time after the last administration to patients. In case of the part 2, the clinical evaluation, blood sampling and study visits for each type would be performed in the same way as shown in the part 1 as well as at a point of IS time specified in an evaluation schedule. Results 3-1. Safety Evaluation Summary of Adverse Events 20 The safety evaluation was performed with regard to secondary endpoints of the part 1, i.e., irnmunogenicity, hypersensitivity monitoring (including delayed hypersensitivity monitoring), measurement of vital signs (including blood pressure, heart and respiration rates, and body temperature), 25 weight, interferon-gamma release assay (IGRA), chest X-ray, 89 CA 03074168 2020-02-26 hepatitis B, hepatitis C and human immunodeficiency virus (HIV- 1, HIV-2) infectious states, opinions about physical examination, 12-lead ECG, adverse events (hereinafter AEs) (including serious adverse events (hereinafter SAEs)), adverse 5 events of special interest (infusion-related reaction / hypersensitivity reaction / anaphylactic reaction[Administration-related reaction], delayed hypersensitivity reaction, injection site reaction, infection and malignancies}, signs and symptoms of TB, clinical 10 laboratory analysis, pregnancy test, prior and concomitant medication, local site pains using a 100 mm visual analogue scale (VAS), etc. The cumulative safety data included AEs until Week 30, wherein an overall summary of AEs reported after treatment 15 during a maintenance phase (Weeks 6 to 30) was presented in Table 15. In general, 70 TEAEs were reported in 28 patients (63.6%) - eight patients (61.5%) from the IV cohort (Cohort 1) and 20 patients (64.5%) from the SC total Cohorts (Cohorts 2 - 4), indicating that the proportion was similar between the two 20 groups. Also, the intensity of most TEAEs was shown as a grade 1 or 2. Among all the TEAEs, the AEs reported in nine patients (20.5%) were regarded to be related to the study drug. The treatment-emergent serious AEs (hereinafter TESAEs) were reported in eight patients (18.2%) - two patients (15.4%) 25 from the IV cohort (Cohort 1) and six patients (19.4%) from the 90 CA 03074168 2020-02-26 SC total Cohorts (Cohorts 2 - 4). All the TESAEs were regarded not to be associated with the study drug. Out of the TEAEs classified as ARRs, the infusion-related reaction, hypersensitivity or anaphylactic reactions were s reported for one patient ( the very day of medication at Week 30) in the IV cohort (Cohort 1) and one patient (two days after medication at Week 6) in the SC cohort (Cohort 4). As an infliximab administration-related reaction was associated with an anti-drug antibody (ADA) (Remsima SmPC 2017), the presence 10 of the ADA was assessed for patients having shown the administration-related reaction. Patients who had positive results for the ADA and a neutralizing antibody (NAb) amounted to just one (IV cohort (Cohort 1)), wherein the patient took a medication of an IV drug in a maintenance phase after a dose 15 loading period, i.e., at Weeks 6 and 14, then was identified as ADA positive from Week 22, and then the administration-related reaction was reported at Week 30. The TEAEs classified as an injection site reaction were reported in four patients (12.9%) of the SC cohort (Cohorts 2 - 20 4), wherein the intensity thereof all was shown as a grade 1 or 2. The presence of the ADA was evaluated even for patients having shown the injection site reaction, wherein two of the four patients have positive results for the ADA and the NAb during the clinical trial period. 25 The TEAEs classified as an infection were reported in two 91 CA 03074168 2020-02-26 patients (15.4%) of the IV cohort (Cohort 1) and seven patients (22.6%) of the SC cohort (Cohorts 2 - 4). TEAEs leading to discontinuation of study drug were reported for one patient (7.7%) in the IV cohort (Cohort 1) and 5 four patients {12.9%) in the SC cohort (Cohorts 2 - 4), out of which only one patient of the cohort 3 discontinued the administration of the study drug due to the TEAEs regarded to be associated with the study drug, which was the latent TB of the intensity grade 1. 10 Death reported during the clinical trial period was two cases {each one from Cohorts 1 and 3) . One patient of the IV cohort (Cohort 1) died from sudden cardiac death at home in one month after the completion of medication at Week 6, which was not reportedly associated with the study drug. Such patient had 15 comorbidi ty of hypertension and chronic heart failure. In the SC cohort (Cohort 3), one patient died from sudden death at home at the very night after medication at Week 30, which was not reportedly associated with the study drug. Such patient had comorbidity of chronic aortic calcification, diabetes, obesity 20 and metabolic syndrome. (Table 15] Cohortl Cohort2 Cohort3 Cohort4 Total SC IVSmg / kg SC120mg SC180mg SC240mg (N=31) (N=13) (N=ll) (N=ll) (N=8) Number of Patients with at Leam one 8 (61.5) 8 (72.7) 7 (58.3) 5(62.5) 20(64.5) 1EAE(%) 92 5 CA 03074168 2020-02-26 Related 4 (30.8) 1 (9.1) 1 (8.3) 3 (37.5) 5 (16.1) Unrelated 6 (46.2) 7(63.6) 7 (58.3) 4(50.0) 18 (58.1) Number of Patients with at Least one 2 (15.4) 2 (18.2) 1 (8.3) 3 (37.5) 6(19.4) TESAE(%) Related 0 0 0 0 0 Unrelated 2 (15.4) 2 (18.2) 1 (8.3) 3 (37.S) 6(19.4) Number of Patients with at Least One 1 (7.7} 0 0 1 (12.5) 1 (3.2) TEAE classified as administration-related reactions (%) Number of Patients wilh at Least One 0 1 (9.1) 2 (16.7) 1 (12.5) 4(12.9) TEAE classified as Injection Site Reaction (%) Number of Patients with at Least One 2 (15.4) 4(36.4) 1 (8.3) 2(25.0) 7(22.6) TEAE classified as infection(%) Related 1 (7.7) 0 1 (8.3) 1 (12.5) 2(6.5) Number of Patients with at Lea& One I (7.7} I (9.1) 2(16.7) l (12.5) 4(12.9) TEAE Leading to Study Drug Discontinuation (%) * At each level of summarization, patients were counted once if they reported one or more events. Only the most severe event is counted. The event is considered to be related if the relationship is defined as 'Possible', 'Probable', 'Definite'. Immunogenicity In general, the proportion of patients who had positive results for the ADA was low in the SC Cohorts, while most patients tested negative for the ADA at Week 30. The number of 10 patients who had positive results for the ADA at Week 30 amounted to 8 (61.5%}, 0 (0.0%), 3 (25.0%) and 1 (12.5%} in the Cohorts 1 to 4, respectively (Table 16). (Table 16] 93 CA 03074168 2020-02-26 Visit Cohortt Cohort2 Cohort3 Cohort4 Total SC IVSmwt<g SC120mg SC180mg SC240mg (N=31) (N=l3) (N=ll) (N=12) (N=8) WeekO ADA positive 0 0 0 1 (12.5) 1 (3.2) NAb positive 0 0 0 0 0 Week6 ADA positive I (7.7) 0 0 3 (37.5) 3 (9.7) NAb positive 1 (7.7) 0 0 2 (25.0) 2 (6.5) Week 14 ADA positive 4(30.8) 0 1 (8.3) 2 (25.0) 3 (9.7) NAbpositive 2(15.4) 0 I (8.3) 1 (12.5) 2(6.5) Week22 ADA positive 7 (53.8) 0 1 (8.3) 2(25.0) 3 (9.7) NAb positive 5 (38.5) 0 1 (8.3) 2(25.0) 3 (9.7) Week30 ADA positive 8(61.5) 0 3 (25.0) 1 (12.5) 4(12.9) NAb positive 4(30.8) 0 1 (8.3) 1 (12.5) 2 (6.5) at least one ADA positive• 7 (58.3) 0 3 (25.0) 0 3 (9.7) after6week at least one NAb positive' 5 (41.7) 0 1 (8.3) 0 1 (3.2) after6week * ADA, Anti-drug antibody; NAb, Neutralizing antibody ** The percentage of visits was calculated using the number of randomly assigned patients as the denominator. * Denominator: Number of ADA negative patients at O and 6 5 weeks; numerator: Number of ADA or NAB positive patients at 14 and 30 weeks Evaluation of local site pains using a visual analogue scale (VAS) IO The range of the VAS amounted to O to 100 mm, with a higher score indicating a more severe pain. In the Cohorts 3 and 4, in which two injections had to be perfonned in each 94 5 CA 03074168 2020-02-26 visit, a slightly higher level of local site pains was observed than in other Cohorts. In general, a low level of local site pains (same or less than 21.05 mm on average) was observed in all the Cohorts (Table 17). [Table 17] Visit Cohortl Cohort2 Cohort3 Statistic IVS mg / kg SC120mg SC180mg lN=l3) (N=tn l(N=t2) Week6 n 13 11 12 Mean(SD) 1632 (18.929) 8.43 (7.807) 21.87 (26.124) Median 7 7 11.85 Minimum Maximum 0.67 0 25 0.792 Week 14 n 12 10 12 Mean(SD) 6.38 (8,742) 5.60(4203) 11.93 (13.145) Median 2.25 6 6,65 Minimum Maximum 0.28 0 13 0,39 Week22 n 11 10 11 Mean(SD) 4.23 (5.574) 10.10 (12.838) 14.15 (13,828) Median 2 6 9 Minimum Maximum o. 15 0,45.5 0 40 Week30 n 10 9 11 Mean(SD) 4.69(6,872) 9.08 (8.851) 21.05 (21.887) Median 2.7 9 12 Minimum, Maximum 0,23.5 0,29.l 1, 71 3-2. Therapeutic efficacy evaluation Disease activity measured by CDAI Cohort4 SC240mg (N=8) 8 1931 (18.676) 11.5 6 63 6 18.75 (22.018) 8.5 3 59 7 12.07 (10.675) 10 3,34.5 5 12.60 (10.158) 8 3.5 29 10 As a result of analyzing the CDAI (Crohn's disease activity index) scores of Weeks 2, 6, 14, 22 and 30 in comparison with baseline as a secondary efficacy endpoint, it was identified that actual values tended to decrease in each 95 CA 03074168 2020-02-26 cohort as time went by. The proportion of patients responding to CDAI-70 criteria at Week 6, one of stratified randomization variables, was slightly higher in the cohort 2 than in other Cohorts, wherein accordingly more attentions were required to 5 be paid to interpretation of efficacy results. The actual values of the disease activity measured by the CDAI as well as the changed values from baseline were summarized in Table 18. [Table 18] IVSmw'kg SC120mg SC180mg SC240mg (N=12) (N=ll) (N=12) (N::7) Visit Actual Cllange Actual Cllange Visit Actual Cllange Actual Statistic Result from Result from Statistic Result from Result Baseline Baseline Baseline Baseline n 12 11 12 7 Mean 310.13 298.16 302.38 324.36 SD 73.353 56.490 73.633 47.866 Minimum 221.8 228.8 229.1 249.9 Median 279.35 290.10 266.75 317.40 Maximum 433.5 409.2 422.5 394.9 Week.2 n 12 12 11 11 12 12 7 7 Mean 243.01 -67.13 219.88 -78.28 266.96 -35.43 254.59 -69.77 SD 97.757 59.875 99.370 72.811 52.401 67.369 90.915 69.656 Minimum 48.8 -173.0 120.9 -169.6 175.0 -163.4 ll7.S -199.9 Median 227.05 -57.10 174.70 -77.70 269.75 -39.25 228.90 -42.00 Maximum 394.1 72.0 457.8 48.6 357.8 86.0 381.0 -7.8 Week.6 n 12 12 11 11 12 12 7 7 Mean 212.20 -97.93 172.58 -125.58 216.43 -85.96 220.34 -104.01 SD 92.019 98.599 105.719 ll5.909 70507 82.388 79.041 61.204 Minimum 56.2 -211.l 47.6 -268.0 28.6 -209.4 103.5 -213.9 Median 230.65 -145.40 149.20 -141.70 240.20 -88.25 215.30 -88.40 96 CA 03074168 2020-02-26 Maximum 371.7 102.2 365.4 102.3 280.S 42.0 340.S -34.6 Week 14 n 12 12 10 10 12 12 7 7 Mean 192.33 -117.81 138.86 -156.SS 188.41 -113.98 21624 -108.11 SD 96.466 103.053 97259 128.873 82.635 109,633 108.773 105.399 Minimum 5.0 -259.0 49.0 -360.2 27.0 -328.3 54.8 -252.4 Median 203.55 -101.95 89.40 -151.00 206.10 -101.70 258.40 -85.30 Maximum 346.0 76.5 334.6 61.3 276.5 23.4 355.8 17.6 Week22 n 11 11 10 10 11 11 7 7 Mean 145.25 -168.58 126.86 -168.55 155.41 -136.05 159.67 -164.69 SD 103.340 107.225 78.765 109.101 66.512 90.717 124.519 111.m Minimum -11.8 -369,6 35.6 -3122 23.6 -314.0 22.6 -293.2 Median 154.40 -133,00 10720 -164.15 164.00 -106.40 158.20 -198.40 Maximum 348.1 -32.3 304.2 41.l 252.9 -0.2 317.2 7.3 Week30 n IO 10 9 9 11 11 6 6 Mean 138.10 -178.92 83.37 -215.63 121.38 -170.08 136.12 -191.07 SD 109.844 105.117 40.112 62.241 70.646 79.501 96.749 87.759 Minimum -16.0 -355.6 21.4 -299.0 17.8 -265.0 19.6 -297.8 Median 125.40 -156,95 73.40 -199.50 125.80 -178.40 135.65 -211.70 Maximum 397.4 -36.1 138.5 -107.9 274.1 21.0 306.6 -68.4 Response evaluation according to CDAI-70 and CDAI-100 response criteria The proportion of patients responding to CDAI-70 response 5 criteria based on CDAI scores (those having a decrease in CDAI scores by 70 points or more from the baseline value) showed a similar level among respective treatment groups (Table 19). The proportion of patients responding to CDAI-100 response criteria (those having a decrease in CDAI scores by 100 points or more 10 from the baseline value) also showed a similar level among respective treatment groups (Table 20). 97 CA 03074168 2020-02-26 [Table 19) Visit IIV5mglkg I SC120mg ISC180mg ISC240mg Statistic (N=ll) (N=ll) (N=l2) (N=7) Week2 Number of patients responded(%) 15(41.7) 17(63.6) JJ (25.o) 13 (42.9) Week6 Number of patients responded(%) 17 (58.3) l9(81.8) 17(58.3) l5 (7t.4) Week 14 Number of patients responded(%) I 8 {66.7) / 8(72.7) 18(66.7) 14(57.1) Week22 Numberofpatientsresponded(%) 19 (75.0) I 9(8t.8) 19(75.0) IS (71.4) Week30 Number of patients responded(%) IS (66.7) 19(81.8) Jto(83.3) IS (71.4) (Table 20) Visit IIV5mglkg I SC120mg ISC180mg ISC240mg Statistic (N=l2) (N=ll) (N=12) (N=7) Week2 Number of patients responded(%) 13 (25.0) J 5 (45.5) 12(16.7) 13(42.9) Week6 Numberofpatientsresponded(o / o) 17 (58.3) l6(54.5) JS {41.7) 13(42.9) Week 14 Number of patients responded(%) 16(50.0) l6(54.5) 16(50.0) J3 (42.9) Week22 Number of patients responded(%) 18(66.7) 17(63.6) 17 (58.3) J4 (57.t) Week30 Number of patients responded(%) 17 (58.3) l9 (8t.8) I 10(83.3) IS (71.4) 5 Clinical remission evaluation The proportion of patients achieving a clinical remission (those having an absolute CDAI score of less than 150 point) was similar among the treatment groups. A comparatively high proportion of patients achieving the clinical remission was 10 observed in Cohort 2 during a medication maintenance period 98 5 CA 03074168 2020-02-26 (Weeks 6 to 30), but six patients (54. 5%) of Cohort 2 were already in a state of having achieved the clinical remission at Week 6, while most of these patients maintained a state of the clinical remission until Week 30 (Table 21). (Table 21) Visit I IVSmglkg I SC120mg lSC180mg I SC240mg Stamtic (N=ll) (N=ll) (N=ll) (N=7) Week2 Number of patients achieved(%) 12 (16.7) 12 (18.2) 10 II (14.3) Week6 Numberofpatientsachieved(%) 13 (25.0) 16(54.5) 12(16.7) II (14.3) Week 14 Number of patients achieved(%) 13 (25.0) 16(54.5) 14(33.3) 12(28.6) Week22 Numberofpatientsachieved(%) ls (4t7) 17(63.6) 14(33.3) 13(42.9) Week30 Number of patients achieved(%) 17 (58.3) 19(81.8) 17 (58.3) IS (71.4) Example 4. Modeling for subcutaneously administering an infliximab to CD patients 10 PK-PD Model Construction A PK-PD model construction was performed in the same way as shown in a method of Example 2. Oose-reqimen scenario of SC dosage fo:rm for modeling in CD patients 15 A pharmacokinetic aspect was predicted based on a following simulation scenario, wherein accordingly efficacy and safety were also predicted, and then evaluated in comparison with an infliximab IV infusion usage, in which a maintenance 99 5 CA 03074168 2020-02-26 dose of 5 mg / kg was administered at an interval of eight weeks (Table 22) . (Table 22) lnfliximab SC 120 mg Every 2 weeks lnfliximab SC 180 mg Every 2 weeks Infliximab SC 240 mg Every 2 weeks Estimated values for infliximab exposure parameters on infliximab SC dose and usaqe for each weight of CO patients Exposure pharmacokinetic parameters on infliximab SC dose and usage were simulated in such a way that a weight range of 10 50 - 130 kg was divided into each unit of 10 kg, wherein the estimated values for a minimum concentration immediately before the next study drug administration (Ctrough) and an area under the concentration-time curve (AUCt) of SC exposure showed a correlation with a drug dosage (Table 23). 15 (Table 23) Compariso N Paramete C1roug1, AUC. CIIUII n (a) r Geometr Ratio of 90%Cl Geometr Ratio of 90%CI Geometr Ratio of 90%CI icLS Geometr ofRatio icLS Geometr ofRatio icLS Geometr ofRatio mean le LS (%) mean icLS (%) mean icLS (%) means means means Test: llO mar; SC at 2 weeklv intervals vs Reference lb> All weight 265 SC 12.8 7.76 6.57;9.16 21591.7 0.9 0.84;0.95 18 0.18 0.17;0.18 IV 1.7 24093.4 102.3 50-60kg 100 SC 15.8 8.14 6.39;10.3 26409.1 1.05 0.96;1.15 21.9 0.19 0.18;0.21 IV 1.9 6 251842 112.4 60-70kg 100 SC 12.8 8.43 6.00;10.7 21721.4 0.88 0.80;0.96 181 0.15 0.14;0.16 IV 1.5 s 2468S.5 119.6 100 CA 03074168 2020-02-26 70-SOkg 100 SC 12.3 6.68 5.26;8.48 20668.2 0.76 0.70;0.83 17.2 0.13 0.13;0.14 IV 1.8 27245.1 129 80-90kg 100 SC 11.3 6.18 4.75;8.03 19046.9 0.67 0.61;0.74 15.9 0.12 O.ll;0.13 IV 1.8 28287.6 134.3 90-lOOkg 100 SC 11.2 4.93 3.82;6.37 18698.2 0.6 0.55;0.66 15.5 0.11 0.10;0.12 IV 2.3 30916.4 139.7 100-llOkg 100 SC 10.3 4.64 359;5.99 17331.1 0.54 0.49;0.60 14.4 0.1 0.09;0.10 IV 2.2 31999.9 149 I 10-120kg 100 SC 9.9 4.17 3.20;5.42 16654.4 0.5 0.45;0.55 13.9 0.()C) 0.08;0.10 IV 2.4 33437.4 152.6 120.130kg 100 SC 9 4.43 3.33;5.90 15388.5 0.46 0.41;0.51 12.9 0.08 0.07;0.09 IV 2 33509.7 161.9 Test: 180 m1 g at 2 weelib: intervals vs Reference (II) All weight 265 SC 19.2 11.62 9.85;13.7 32367.4 1.34 1.26;1.43 26.9 0.26 0.25;0.28 IV 1.7 2 24093.4 102.3 50-60kg 100 SC 23.7 12.19 9.57;15.5 39576.4 1.57 1.44;1.72 32.8 0.29 0.27;0.31 IV 1.9 1 25184.2 112.4 60-70kg 100 SC 19.2 12.62 9.90;16.l 32541.4 1.32 1.20;1.45 27.2 0.23 0.21;0.24 IV 1.5 1 24685.5 119.6 70-SOkg 100 SC 18.4 10.01 7.88;12.7 30981 1.14 1.05;1.24 25.8 0.2 0.19;0.21 IV 1.8 2 27245.1 129 80-90kg 100 SC 16.9 9.26 7.13;12.0 28541.7 1.01 0.92;1.l 1 23.8 0.18 0.16;0.19 IV 1.8 4 28287.6 134.3 90-lOOkg 100 SC 16.7 7.39 5.72;9.54 28000.4 0.91 0.82;0.99 232 0.17 0.15;0.18 IV 2.3 30916.4 139.7 100-llOkg 100 SC 15.4 6.95 5.38;8.98 25959 0.81 0.74;0.89 21.6 0.14 0.14;0.16 IV 2.2 31999.9 149 110-120kg 100 SC 14.9 6.25 4.80;8.13 24932.8 0.75 0.68;0.82 20.7 0.14 0.13;0.15 IV 2.4 33437.4 152.6 120.130kg 100 SC 13.5 6.64 4.98;8.84 23025 0.69 0.62;0.76 19.3 0.12 0.11;0.13 IV 2 33509.7 161.9 Test: 240 m1SC !!t2 wee~intervals!.!! Referenss(b) All weight 265 SC 25.6 15.49 13.12;18. 43143.l 1.79 1.68;1.91 35.9 0.35 0.33;0.37 IV 1.7 28 24093.4 102.3 50-60kg 100 SC 31.6 1623 12.75;20. 52743.5 2.09 1.91;2.29 43.7 0.39 0.36;0.42 IV 1.9 66 25184.2 112.4 60-70kg 100 SC 25.5 16.81 13.18;21. 43361.1 1.76 1.60;1.93 36.3 0.3 0.28;0.33 IV 1.5 44 24685.S 119.6 70-80kg 100 SC 24.5 13.34 10.50;16. 41293.8 1.52 1.39;1.65 34.4 0.27 0.25;028 IV 1.8 94 27245.1 129 8Q-90kg 100 SC 22.5 12.34 9.49;16.0 38036.3 1.34 1.22;1.48 31.7 0.24 0.22;0.25 101 IV 1.8 4 28287.6 134.3 90-lOOkg 100 SC 22.3 9.85 7.62;12.7 37302 1.21 1.10;1.32 31 0.22 0.21;0.24 IV 2.3 2 30916.4 139.7 100-ll0kg 100 SC 20.6 9.26 7.17;11.9 34586.7 1.08 0.98;1.19 28.8 0.19 0.18;0.21 IV 2.2 6 31999.9 149 110.120kg 100 SC 19.8 8.33 6.40;10.8 33210.9 0.99 0.90;1.10 27.6 0.18 0.17;0.19 IV 2.4 3 33437.4 152.6 120.130kg 100 SC 18.0 8.84 6.64;11.7 30661.1 0.91 0.83;1.0l 25.7 0.16 0.15;0.17 IV 2 8 33509.7 161.9 Note: (a) All patients received 5 mg / kg infliximab via IV infusionover2 hours at weeks 0 and 2, prior1D maintenance regimen commencing at week 6 (in bo1h test and reference periods of 1he cross-over). (b) Reference 1rea1ment comprised of 5 mg / kg every 8 weeks infliximab via IV infusion over 2 homs (maintenance regimen). ( c) geometric LS means ratio=test / reference Abbreviations: CI :Confidence Interval, LS:Least Square, SD:Standard Deviation *** In some aspects, embodiments as described herein include the following items: 5 Item 1. Use of a pharmaceutical composition comprising infliximab and a pharmaceutically acceptable carrier, for the treatment of a TNF-a-related disease in a patient, wherein the pharmaceutical composition comprises a dose of 120 mg of the infliximab for subcutaneous use at intervals of 2 weeks. 10 Item 2. Use of a pharmaceutical composition comprising infliximab and a pharmaceutically acceptable carrier, for the preparation of a medicament for the treatment of a TNF-arelated disease in a patient, wherein the pharmaceutical composition comprises a dose of 120 mg of the infliximab for 15 subcutaneous use at intervals of 2 weeks. Item 3. The use of item 1 or 2, wherein the TNF-a-related disease is rheumatoid arthritis, ulcerative colitis, Crohn's 102 Date re~ue / Date received 2024-01-24 5 disease, plaque psoriasis, psoriatic arthritis, and ankylosing spondylitis, ulcerative colitis or Crohn's disease. Item 4. The use of item 3, wherein the TNF-a-related disease is rheumatoid arthritis. Item 5. disease The is use of item 1 or 2, ulcerative colitis, wherein Crohn's the TNF-a-related disease, plaque psoriasis, psoriatic arthritis, or ankylosing spondylitis. Item 6. The use of item 1 or 2, wherein the TNF-a-related disease is ulcerative colitis or Crohn's disease. 10 Item 7. The use of any one of items 1 to 6, wherein said use is adapted for self-administration by the patient. Item 8. The use of any one of items 1 to 7, wherein the use of the infliximab is adapted for co-administration with a diseasemodifying anti rheumatic drug (DMARD). 15 Item 9. The use of item 8, wherein the disease-modifying anti rheumatic drug (DMARD) is methotrexate, leflunomide, sulfasalazine or hydroxychloroquine. Item 10. The use of any one of items 1 to 9, wherein the use follows at least one intravenous use of a dose of the 20 infliximab. Item 11. The use of item 10, wherein the patient is a patient who has been administered at least twice intravenously with the infliximab before the subcutaneous administration. 103 Date re~ue / Date received 2024-01-24 Item 12. The use of i tern 11, wherein each of the intravenous administrations is to be performed 6 and 4 weeks before the subcutaneous administration. Item 13. The use of item 10 or 11, wherein the first 5 subcutaneous use is to be separated from the last intravenous use by 2 to 8 weeks. Item 14. The use of item 13, wherein the first subcutaneous administration is to be performed 4 weeks after the last intravenous administration. 10 Item 15. The use of any one of items 10 to 14, wherein each of the intravenous administrations is to be performed at an interval of 2 or 4 weeks. Item 16. The use of any one of i terns 1 to 15, wherein the infliximab is maintained at a minimum blood concentration 15 (Ctrough) of 3 to 16 μg / mL after the subcutaneous use. Item 17. The use of item 16, wherein the infliximab is maintained at a minimum blood concentration (Ctrough) of 9 to 32 μg / mL after the subcutaneous use. Item 18. The use of any one of items 1 to 17, wherein the 20 patient after the subcutaneous use has one or more of the following characteristics: a) a decrease in DAS28 (Disease Activity Score in 28 joints) of at least 2.0; or b) a decrease in CDAI (Crohn's disease activity index) of 25 at least 70. 104 Date re~ue / Date received 2024-01-24 Item 19. The use of any one of items 1 to 18, wherein the patient before the subcutaneous use as defined in any one of items 1 to 18 has one or more of the following characteristics: a) a patient who has an inadequate response to disease- 5 modifying anti rheumatic drugs (DMARDs), including methotrexate; b) a patient who has not previously been treated with methotrexate and other DMARDs; c) a patient who exhibits elevated serologic indicators 10 associated with severe axial-predominant symptoms and inflammation, therapies; or d) a which patient show no proper who does not response to common respond to, or is contraindicated to, or has intolerance to methotrexate, 15 cyclosporine, or systemic ultraviolet A therapy (PUVA). therapies including psoralen Item 20. The use of any one of items 1 to 18, wherein the patient before the subcutaneous use as defined in any one of items 1 to 18 has one or more of the following characteristics: 20 a) a patient who has an inadequate response to, or has intolerance to, or is contraindicated for treatment with corticosteroids, 6-mercaptopurine, azathioprine or immunosuppressants; or b) a patient who does not respond to common therapies, 25 including antibiotic, excretion or immunosuppressive therapies. 105 Date re~ue / Date received 2024-01-24 Item 21. The use of any one of items 1 to 20, wherein the infliximab comprises: a light-chain variable region comprising a CDRl domain comprising an amino acid sequence of SEQ ID NO: 1, a CDR2 5 domain comprising an amino acid sequence of SEQ ID NO: 2, and a CDR3 domain comprising an amino acid sequence of SEQ ID NO: 3; and a heavy-chain variable region comprising a CDRl domain comprising an amino acid sequence of SEQ ID NO: 4, a CDR2 10 domain comprising an amino acid sequence of SEQ ID NO: 5, and a CDR3 domain comprising an amino acid sequence of SEQ ID NO: 6. Item 22. The use of any one of items 1 to 21, wherein said composition is adapted for administration simultaneously with, or before or after, administration of one or more antibodies 15 which is adalimumab, etanercept, certolizumab pegol or golimumab. Item 23. The use of any one of items 1 to 4, 16 and 17, wherein the composition comprising the infliximab contains: (A) 120 mg / ml of the infliximab; (B) 0.02 to 0.1 g,. 0 (w / v) of 20 polysorbate; (C) 1 to 10% (w / v) of sorbitol; and (D) 1 to 50 mM of a buffer comprising acetate. Item 24. The use of any one of items 1 to 23, wherein the composition comprising the infliximab is filled in a pre-filled syringe or an auto-injector. 106 Date re~ue / Date received 2024-01-24 Item 25. A pharmaceutical composition for treatment of TNF-cxrelated disease, comprising infliximab and a pharmaceutically acceptable carrier, wherein the infliximab is adapted for subcutaneous use at a dose of 120 mg and at intervals of 2 5 weeks. Item 26. A kit comprising: (a) a pharmaceutical composition comprising infliximab; and (b) instructions that direct the pharmaceutical 10 composition to be administered subcutaneously at a dose of 120 mg and at intervals of 2 weeks in order to treat a patient having TNF-cx-related disease. 107 Date re~ue / Date received 2024-01-24
Claims
[CLAIMS]
1. Use of a pharmaceutical composition comprising infliximab and a pharmaceutically acceptable carrier, for the treatment of a 5 TNF-a-related disease in a patient, wherein the pharmaceutical composition comprises a dose of 120 mg of the infliximab for subcutaneous use at intervals of 2 weeks.
2. Use of a pharmaceutical composition comprising infliximab 10 and a pharmaceutically acceptable carrier, for the preparation of a medicament for the treatment of a TNF-a-related disease in a patient, wherein the pharmaceutical composition comprises a dose of 120 mg of the infliximab for subcutaneous use at intervals of 2 weeks. 15
3. The use of claim 1 or 2, wherein the TNF-a-related disease is rheumatoid arthritis, ulcerative colitis, Crohn's disease, plaque psoriasis, psoriatic arthritis, and ankylosing spondylitis, ulcerative colitis or Crohn's disease. 20
4. The use of claim 3, wherein the TNF-a-related disease is rheumatoid arthritis. 108 Date re~ue / Date received 2024-01-24
5. The use of claim 1 or 2, wherein the TNF-a-related disease is ulcerative colitis, Crohn' s disease, plaque psoriasis, psoriatic arthritis, or ankylosing spondylitis. 5
6. The use of claim 1 or 2, wherein the TNF-a-related disease is ulcerative colitis or Crohn's disease.
7. The use of any one of claims 1 to 6, wherein said use is 10 adapted for self-administration by the patient.
8. The use of any one of claims 1 to 7, wherein the use of the infliximab is adapted for co-administration with a diseasemodifying anti rheumatic drug (DMARD). 15
9. 20 The use of claim 8, wherein the disease-modifying anti rheumatic drug (DMARD) is methotrexate, leflunomide, sulfasalazine or hydroxychloroquine.
10. The use of any one of claims 1 to 9, wherein the use follows at least one intravenous use of a dose of the infliximab. 109 Date re~ue / Date received 2024-01-24
11. The use of claim 10, wherein the patient is a patient who has been ad.ministered at least twice intravenously with the infliximab before the subcutaneous ad.ministration. 5
12. The use of ad.ministrations is claim 11, wherein to be performed 6 subcutaneous administration.
13. each of the and 4 weeks intravenous before the The use of claim 10 or 11, wherein the first subcutaneous use is to be separated from the last intravenous use by 2 to 8 weeks.
14. The use of claim 13, wherein the first subcutaneous 15 ad.ministration is to be performed 4 weeks after the last intravenous ad.ministration.
15. The use of any one of claims 10 to 14, wherein each of the intravenous ad.ministrations is to be performed at an interval of 2 20 or 4 weeks. 110 Date re~ue / Date received 2024-01-24
16. The use of any one of claims 1 to 15, wherein the infliximab is maintained at a minimum blood concentration (Ctrough) of 3 to 16 μg / mL after the subcutaneous use. 5
17. The use of claim 16, wherein the infliximab is maintained at a minimum blood concentration (Ctrough) of 9 to 32 μg / mL after the subcutaneous use.
18. 10 The use of any one of claims 1 to 1 7, wherein the patient after the subcutaneous use has one or more of the following characteristics: a) a decrease in DAS28 (Disease Activity Score in 28 joints) of at least 2.0; or 15 b) a decrease in CDAI (Crohn's disease activity index) of at least 70.
19. The use of any one of claims 1 to 18, wherein the patient before the subcutaneous use as defined in any one of claims 1 to 20 18 has one or more of the following characteristics: a) a patient who has an inadequate response to diseasemodifying anti rheumatic drugs (DMARDs), including methotrexate; 111 Date re~ue / Date received 2024-01-24 b) a patient who has not previously been treated with methotrexate and other DMARDs; c) a patient who exhibits elevated serologic indicators associated with severe axial-predominant symptoms and 5 inflammation, which show no proper response to common therapies; or d) a patient who does not respond to, or is contraindicated to, or has intolerance to methotrexate, cyclosporine, or systemic therapies including psoralen ultraviolet A therapy (PUVA). 10
20. The use of any one of claims 1 to 18, wherein the patient before the subcutaneous use as defined in any one of claims 1 to 18 has one or more of the following characteristics: a) a patient who has an inadequate response to, or has 15 intolerance to, or is contraindicated for treatment with corticosteroids, 6-mercaptopurine, azathioprine or immunosuppressants; or b) a patient who does not respond to common therapies, including antibiotic, excretion or immunosuppressive therapies. 20
21. The use of any one of claims 1 to 20, wherein the infliximab comprises: 112 Date re~ue / Date received 2024-01-24 a light-chain variable region comprising a CDRl domain comprising an amino acid sequence of SEQ ID NO: 1, a CDR2 domain comprising an amino acid sequence of SEQ ID NO: 2, and a CDR3 domain comprising an amino acid sequence of SEQ ID NO: 3; and 5 a heavy-chain variable region comprising a CDRl domain comprising an amino acid sequence of SEQ ID NO: 4, a CDR2 domain comprising an amino acid sequence of SEQ ID NO: 5, and a CDR3 domain comprising an amino acid sequence of SEQ ID NO:
6.
22. The use of any one of claims 1 to 21, wherein said composition is adapted for administration simultaneously with, or before or after, administration of one or more antibodies which is adalimumab, etanercept, certolizumab pegol or golimumab.
23. 15 The use of any one of claims 1 to 4, 16 and 17, wherein the composition comprising the infliximab contains: (A) 120 mg / ml of the infliximab; (B) 0. 02 to O .1 % (w / v) of polysorbate; (C) 1 to 10% (w / v) of sorbitol; and (D) 1 to 50 mM of a buffer comprising acetate. 20
24. The use of any one of claims 1 to 23, wherein the composition comprising the infliximab is filled in a pre-filled syringe or an auto-injector. 113 Date re~ue / Date received 2024-01-24
25. A pharmaceutical composition for treatment of TNF-a-related disease, comprising infliximab and a pharmaceutically acceptable carrier, wherein the infliximab is adapted for subcutaneous use at 5 a dose of 120 mg and at intervals of 2 weeks.
26. A kit comprising: (a) a pharmaceutical composition comprising infliximab; and (b) instructions that direct the pharmaceutical composition 10 to be administered subcutaneously at a dose of 120 mg and at intervals of 2 weeks in order to treat a patient having TNF-arelated disease. 114 Date re~ue / Date received 2024-01-24