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40 results about "HDL - High density lipoprotein" patented technology

High-density lipoprotein-like peptide-phospholipid scaffold ("hpps") nanoparticles

The present invention provides a non-naturally occurring High-Density Lipoprotein-like peptide-phospholipid scaffold (“HPPS”) nanoparticle. More particularly, the invention provides a non-naturally occurring peptide-lipid nanoscaffold comprising: (a) at least one phospholipid; (b) at least one unsaturated lipid, preferably an unsaturated sterol ester, further preferably an unsaturated cholesterol ester, further preferably cholsteryl oleate; and (c) at least one peptide, the peptide comprising an amino acid sequence capable of forming at least one amphipathic a-helix; wherein the components a), b) and c) associate to form the peptide-phospholipid nanoscaffold. In embodiments of the present invention, a cell surface receptor ligand is incorporated into the HPPS. In one embodiment, the cell surface receptor ligand is covalently bonded to the peptide scaffold of the HPPS nanoparticles. In other embodiments, a cell surface receptor ligand is coupled to a lipid anchor and is displayed on the surface of the HPPS nanoparticles by incorporation of the lipid anchor into the phospholipids monolayer of the HPPS nanoparticle. The present invention also provides pharmaceutical formulations comprising HPPS nanoparticles and methods of making the HPPS nanoparticles.
Owner:UNIV HEALTH NETWORK

Method for extracting high-density lipoprotein and separating and purifying apolipoprotein apoA-I from human plasma

The invention provides a method for extracting high-density lipoprotein (HDL) and separating and purifying high-purity apolipoprotein apoA-I from normal human plasma. The method comprises the following steps: (1) regulating plasma to be of different densities by utilizing neutral salt, and eliminating impure protein by utilizing a sequential gradient density supercentrifugation method, so as to obtain a high-purity HDL component; (2) carrying out degreasing on the obtained high-purity HDL component in a flowingly adding manner by utilizing a certain proportion of alcohol ether solvents under a low-temperature freezing state, so as to obtain degreased apoHDL precipitates; (3) redissolving the apoHDL precipitates by utilizing a TBS buffer liquid system containing 1-8M urea, filtering, carrying out separation and purification by molecular sieve chromatography of filtrate and anion exchange chromatography in sequence to obtain a high-purity apoA-I solution. According to the method, albumin components which are very difficult to remove can be separated from the HDL; the apoA-I prepared by utilizing the method has very high purity and activity, the purity can reach above 98%, and the apoA-I can generate clear precipitin reaction with antiserum after being diluted by 64 times; the method is safe and convenient to operate, is short in extraction period and is suitable for industrial production.
Owner:SHANGHAI FOSUN PHARMA (GROUP) CO LTD +1

Amphipathic low-density lipoprotein adsorbent and preparation method thereof

The invention discloses an amphipathic low-density lipoprotein adsorbent and a preparation method thereof. A skeleton of the adsorbent is a carrier, taurine is immobilized on the surface of the carrier, and deoxycholic acid is coupled on the taurine. According to the amphipathic low-density lipoprotein adsorbent disclosed by the invention, by using electrostatic interaction of a sulfo group, LDL (low-density lipoprotein) can be effectively adsorbed and removed; condensed deoxycholic acid is further utilized, adsorption to beneficial element HDL (high density lipoprotein) is reduced through the hydrophobic and steric hindrance effects of the naphthene structure, total cholesterol (TC) and triglyceride(TG) can be removed, and the selective removal ability of the adsorbent is improved. The amphipathic low-density lipoprotein adsorbent disclosed by the invention carries the hydrophilic sulfonic group and hydrophobic deoxycholic acid, can simulate hydrophilic and hydrophobic structures of phospholipid molecules, has better blood compatibility with cells, and is suitable for whole blood perfusion. By adjusting the ratio of the hydrophilic and hydrophobic groups, the adsorbent with high blood compatibility and capable of specifically adsorbing LDL (low-density lipoprotein) can be obtained.
Owner:佛山市博新生物科技有限公司

Chemiluminiscence imaging immunoassay method for simultaneously measuring oxidized lipoprotein (a) and oxidized low-density lipoprotein of human serum

The invention discloses a method for chemiluminiscence imaging immunoassay method for simultaneously measuring oxidized lipoproteins (a) and low-density oxidized lipoproteins of human serum. According to an analysis system, a multi-component immunosensor modified by silanization is used as a solid-phase carrier; a solid-phase antibody is prepared by covering the carrier with a capturing antibody; a sample to be measured or a standard series solution is added into the solid-phase antibody; after the solid-phase antibody and the sample to be measured or the standard series solution fully react, an antibody labeled with horse radish peroxidase is added to form a sandwich immune compound; finally a chemiluminescence substrate, namely luminal-hydrogen peroxide, is added for reaction; the luminous intensity is detected through a high-resolution charge coupler, so that the oxidized lipoproteins (a) and the low-density oxidized lipoproteins of the human serum can be measured simultaneously, and the immune reaction condition, the enzyme conjugate dilution degree, the detection time and the like are optimized; furthermore, the indexes such as linear range, precision, accuracy and detection limit of the method are checked. The analysis method has the advantages of simplicity in operation, high sensitivity, narrow linear range, high stability and the like and has a certain clinical application value.
Owner:NANJING GENERAL HOSPITAL NANJING MILLITARY COMMAND P L A
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