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Gene engineering method for preparing a recombinant glutathion peroxidase

A glutathione peroxide, prokaryotic expression technology, applied in the field of preparation of recombinant glutathione peroxidase, can solve the problems of cumbersome operation, affecting enzyme activity, lack of targeting, etc., to solve the problem of limited sources Effect

Active Publication Date: 2015-01-28
JILIN UNIV
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

[0004] Chinese patent 94102481.4, 96112628.0, 99104234.4, the preparation method of all kinds of selenium-containing abzymes disclosed in 200810050556.6 is exactly to apply the chemical mutation (modification) method to introduce the catalytic group SeCys of GPX in the antibody class template protein, has the following disadvantages: (1) in In the preparation process, only the step of chemical mutation (modification) will lose 20-40% of the enzyme protein, resulting in a significant decline in the yield of the simulated enzyme; (2) the cycle of preparing the simulated enzyme is long, the operation is cumbersome, and the time is long; (3) In the process of chemical mutation, phenylmethylsulfonyl fluoride, acetonitrile, etc. need to be used, these substances are toxic substances; (4) lack of targeting, for large protein molecules, a chemical reaction is often introduced at different sites Multiple non-specific catalytic groups, so the introduction of catalytic groups by chemical mutation cannot achieve the specificity of gene mutation method
[0005] Chinese patent 200810050556.6 also discloses that another preparation method of human single-chain selenium-containing abzyme is to introduce a catalytic group using a defective prokaryotic expression system (Escherichia coli) and gene mutation, but it is limited to human single-chain selenium-containing abzyme Preparation of abzymes, excluding recombinant glutathione peroxidase (GPX) and other GPX mimetic enzymes
[0006] Since the codon UGA of SeCys, the catalytic group of GPX, is a stop codon, in the common prokaryotic expression system, it is necessary to introduce a neck loop structure in the open reading frame of the GPX gene, immediately downstream of the codon UGA of SeCys, to translate UGA into SeCys instead of a stop codon, and the introduction of a neck loop in the open reading frame will inevitably cause a change in the spatial conformation of GPX, thereby affecting the enzyme activity
Therefore, the common prokaryotic expression system is not suitable for direct expression of selenoproteins with GPX activity

Method used

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Examples

Experimental program
Comparison scheme
Effect test

Embodiment 1

[0052] Example 1: Preparation of genetically engineered human GPX1 using an auxotrophic prokaryotic expression system

[0053] Under the premise of keeping the amino acid sequence unchanged, design primers to amplify or directly synthesize the coding gene according to the sequence of the GPX1 gene published in the gene library (see NCBI, NM_000581.2) to ensure that the 5' end of the gene contains a start codon (ATG) and Nde I restriction site, the 3' end contains stop codon and Hind III restriction site. After double digestion with restriction endonucleases Nde I and Hind III, it was connected to the pCold III (TAKARA, Cat. #3369) vector which was also digested. On the premise of keeping other amino acid sequences unchanged, design two completely isometric and complementary site-directed mutagenesis primers according to the gene sequence of the amino acid adjacent to No. 49 SeCys. center. With these two completely complementary primers and rapid site-directed mutagenesis kit...

Embodiment 2

[0056] Example 2: Combined preparation of genetically engineered human GPX1 by SPP system and auxotrophic prokaryotic expression system

[0057] Under the premise of keeping the amino acid sequence unchanged, its coding gene was directly synthesized according to the GPX1 gene sequence published in the gene library (see NCBI, NM_000581.2), ensuring that the 5' end of the gene contains an initiation codon (ATG) and Nde I restriction site, the 3' end contains a stop codon and a Hind III restriction site, the coding sequence TGA of No. 49 SeCys of the GPX1 gene is replaced by a Cys codon (TGC), and all other Cys codes in the GPX1 gene The codons were replaced by Ser codons, and the full length of the gene did not contain the ACA sequence. After double digestion with restriction endonucleases Nde I and Hind III, it was connected to the pCold III (TAKARA, Cat. #3369) vector which was also digested.

[0058] Transform the auxotrophic Escherichia coli BL21(DE3) Cys with the vector (p...

Embodiment 3

[0060] Example 3: Preparation of genetically engineered human GPX4 by one-step transfection with eukaryotic expression system

[0061] 1. Construction of human GPX4 expression vector: mRNA was extracted from HepG-2 (DSMZ#ACC180) liver cancer cells with small amount of mRNA extraction kit (Sigma, Cat#MRN-10), and reverse transcriptase (AMV RT, Promega, Cat#M5101) and oligo(dT) were transcribed into double-stranded cDNA by RT-PCR (Reverse Transcription Polymerase Chain Reaction). Under the premise of keeping the amino acid sequence unchanged, primers were designed according to the gene sequence of human GPX4 (NCBI, NM_002085.3) disclosed in the gene library to amplify the coding gene of GPX4, ensuring that the 5' end of the gene contained a start codon (ATG ) and EcoRI restriction site, the 3'-end primer is selected to insert the NotI restriction site after the first base of polyoligonucleotide A of GPX4mRNA, to ensure that there is a selenocysteine ​​insertion downstream of the...

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Abstract

The invention provides a gene engineering method for preparing a recombinant glutathion peroxidase, which belongs to the field of biological technology. The method comprises the following steps: assembling a target gene to a secretion type prokaryotic expression vector, introducing a catalytic group SeCys of GPX into a substrate combination position of GPX by a gene mutant method in an auxotroph prokaryotic expression system or an auxotroph and SPP combined expression system, thereby the activity of the GPS is very high; or assembling the target gene with the SeCys insertion sequence into a secretion type mammalia cell expression vector, assembling a SeCys insertion sequence binding protein 2 into an intracellular type mammalia cell expression vector, and cotransfecting the two vectors into the same lactation cell strain, and synthesizing the GPX under the existence of sodium selenite. The invention the advantages of simple method, recombined GPX vitality, high output and good stability, thereby avoiding decreased yield and inactivation caused by renaturation of an inclusion body, and solving the problem that the natural GPX source is limited and the property is not stable.

Description

technical field [0001] The invention relates to a method for preparing recombinant glutathione peroxidase by using a genetic engineering method, belongs to the field of biotechnology, and relates to gene recombination technology, gene mutation technology and recombinant protein expression technology. Background technique [0002] The substrate of selenium-containing glutathione peroxidase (GPX) is glutathione (GSH), and the catalytic group is selenocysteine ​​(SeCys). In organisms, GPX together with superoxide dismutase (SOD) and catalase (CAT) constitute the body's antioxidant defense system. GPX plays an important role in this system. It uses the substrate GSH as a reducing agent to decompose hydrogen peroxide and various hydroperoxides in the body, so it can remove reactive oxygen species (ROS) in the body and prevent lipid peroxidation. Treat various diseases caused by active oxygen, such as aging, ultraviolet radiation, cardiovascular and cerebrovascular diseases, cata...

Claims

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Application Information

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Patent Type & Authority Patents(China)
IPC IPC(8): C12N9/08C12N15/70C12N15/53C12N15/85
Inventor 魏景艳宋健邢瑞庆
Owner JILIN UNIV
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