Candida Antarctica lipase B gene and applications thereof in yeast display
A technology of Candida Antarctica and lipase, which is applied in the field of yeast, can solve the problems of limited application development and low yield, and achieve the effects of increasing display volume, high catalytic performance, and improving thermal stability
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Embodiment 1
[0027] Embodiment 1: the synthesis of improved Rhizomucor miehei lipase gene
[0028] The existing Candida antarctica lipase B (Genbank: Z30645, derived from Candida antarctica LF058 strain), its gene is shown in SEQ.ID.NO3, and the codon preference of Candida antarctica is similar to that of Pichia pastoris Yeast has a certain gap.
[0029] The present invention first realizes the saturation mutation of different sites and different amino acids on the wild-type Candida antarctica lipase B with the help of bioinformatics prediction, and then screens out a strain of enzyme activity and heat resistance through directed evolution and high-throughput screening All significantly improved strains, through sequencing, found that the amino acid sequence of wild-type CALB has the following mutations, Pro226Asn, Leu227Lys, Phe228Thr, Val229Ser, Leu285Gly, Ala286Met, Ala288Ile, the specific amino acid sequence of the improved CAL is SEQ.ID.NO1 On this basis, the codons preferred by Pich...
Embodiment 2
[0030] Embodiment 2: Construction of pUC-CALB plasmid
[0031] The fully synthetic gene obtained in the previous step can be TA cloned with pUC57 to achieve in vitro linkage, and the operation can be performed according to the instructions. The 10 μL volume reaction system is as follows: 1 μL (50 ng) of T carrier, 3 μL of fully synthetic gene product, 1 μL of 10×Buffer containing ATP, 1 μL of T4 DNA ligase, and ddH 2 O to make up to 10 μL. After a little centrifugation, connect to a water bath at 16°C overnight. The ligation product was transformed into E.coli DH5α, and then spread onto an indicator plate containing 0.5mM IPTG, 40μg / ml X-Gal, cultured overnight, and the recombinant plasmid PMD 18-T-RML was sent to Shanghai Sequencing by Sangon Bioengineering Co., Ltd. The sequencing showed that the cloned gene was consistent with the fully synthetic gene we described.
Embodiment 3
[0032] Embodiment 3: Construction of recombinant plasmid pKFS-CALB
[0033] The plasmid pUC57-CALB was used as a template, and P1 and P2 were used as primers for PCR amplification. The system is 1 μL of template; 5 μL of 10×Taq DNA polymerase buffer (containing Mg 2+ ); 2.5mmol / L dNTP 4μL; 20μM mol / L primers 1μL each; Taq DNA polymerase 0.75μL, add sterile water to a total volume of 50μL. The reaction conditions are: pre-denaturation at 94°C for 5 min; denaturation at 94°C for 45 s, annealing at 45°C for 45 s, and extension at 72°C for 2 min, a total of 30 cycles; the 30th cycle was extended at 72°C for 10 min, and the PCR product was detected by 0.8% agarose gel electrophoresis And cut the gel to recover and purify.
[0034] Both the PCR product of the fully synthesized gene and the pKFS plasmid were digested with EcoRI and NotI, and ligated in vitro. The 20 μL volume reaction system is as follows: pKFS plasmid 2 μL (50 ng), PCR product 15 μL (50 ng), 10×Buffer 2 μL, T4 DN...
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