A kind of eukaryotic expression vector and system using CHO cell to produce recombinant protein
A technology of eukaryotic expression vectors and expression systems, applied in the field of gene expression systems and eukaryotic expression vectors, can solve the problems of technology transfer barriers restricting biopharmaceutical technology and industrial development
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Embodiment 1
[0055] Example 1 Construction of pHLX101 eukaryotic expression vector
[0056] 1. Synthesis of Marker Gene Expression Units
[0057] The mouse glutamine synthetase gene sequence (GS, Genebank accession number: NM008131.3, ABC015086.1, X16314.1), TK promoter gene sequence (TK promoter, Genebank accession number: JN420340) was obtained from the NCBI database. .1, AF104248.2, AF362551.1) and SV40polyA gene sequence (Genebank accession number: JQ302818.1, HQ388295.1, EF437954.1), based on these sequences, designed a GS gene integration and expression in CHO cells GS expression unit (SEQ ID NO: 4), the designed expression unit was sent to Gene Synthesis Company to synthesize the sequence, and the synthesized expression unit was inserted into the pBSK vector to obtain the TK-GS-SV-pBSK vector.
[0058] 13. Construction of eukaryotic expression vector pHLX101
[0059] 2.1 Preparation of gene fragments containing GS expression units
[0060] The gene fragment containing the GS expr...
Embodiment 2
[0082] Example 2 Construction of CHO cell gene integration expression system and expression of antibody
[0083] 1. Construction of pHLX101-HLX01-HC, pHLX101-HLX01-LC recombinant plasmids and CHO expression system
[0084] Firstly, the eukaryotic expression vector 2009-HLX01-HC (containing the HLX01-HC expression unit composed of PromoterA, antibody heavy chain sequence and SV40 poly A) containing antibody heavy chain and antibody light chain sequences and related functional elements was constructed, and the true Nuclear expression vector 2009-HLX01-LC (contains HLX01-LC expression unit composed of CMVPromoter, antibody light chain sequence and SV40polyA).
[0085] The exogenous gene expression units were respectively amplified from the 2009-HLX01-HC vector and the 2009-HLX01-LC vector by PCR, and then the exogenous gene expression units were inserted into the pHLX101 vector by enzyme digestion and ligation, and transfected CHO-K1 cells, and finally screen the cell line with ...
Embodiment 3
[0143] Example 3 Construction of CHO cell gene integration expression system and expression of foreign protein
[0144] 1. Construction of pHLX101-eGFP expression vector and screening of stable cell lines
[0145] 1.3. Expression vector construction
[0146] First, construct the eGFP expression unit, which contains the SmaI endonuclease recognition site sequence and CMV promoter sequence in the 5' to 3' direction (the gene sequence is the same as the Genebank login sequence: JQ302818.1, AB609714.1, GU937742.1, BK000394.5 and other sequences), eGFP gene sequence (the gene sequence is the same as the Genebank landing sequence: JQ809330.1, JN038403.1, JQ733047.1, AB673329.1 and other sequences), BGHpA sequence (the gene sequence is the same as the Genebank landing sequence: EF437956.1 , U90717.1, X90639.1, JF313342.1 and other sequences) and SmaI endonuclease recognition site sequence. The exogenous gene expression unit was prepared by digesting the eGFP expression unit with Sm...
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