Method for preparing glutamic acid decarboxylase mutant by utilizing ramachandran map information and mutant thereof
A glutamic acid decarboxylase and mutant technology, applied in the field of molecular biology, can solve the problems of low GAD specific activity and unfavorable application, and achieve the effects of saving time, facilitating widespread promotion, and improving experimental efficiency
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[0032] 1. Construction of mutant library
[0033] According to the glutamic acid decarboxylase gene design of Lactobacillus brevis (Lactobacillus brevis) CGMCC NO.1306, 19 pairs of site-directed mutagenesis primers are as follows:
[0034] K413X_F 5'-CACCTATCCCTTACCA YYY AACATGACGGACCGC-3'
[0035] K413X_R 5'-GCGGTCCGTCATGTT YYY TGGTAAGGGATAGGTG-3'
[0036] Note: where X represents the remaining 19 amino acids except lysine, YYY represents the codon corresponding to amino acid X.
[0037] Among them, the primers for amplifying and obtaining K413I are:
[0038] Upstream primer: 5'-CACCTATCCCTTACCA ATT AACATGACGGACCGC-3'
[0039] Downstream primer: 5'-GCGGTCCGTCATGTT AAT TGGTAAGGGATAGGTG-3'
[0040] Using the plasmid containing the GAD1407 gene (Gene ID: 4412752) as a template, site-directed PCR amplification was performed. The PCR amplification system is 50 μL, including: 10 μL 5×PCR buffer, 4 μL dNTPs (2.5 mmol / L), 1 μL upstream primer (10 mmol / L), 1 μL downstream...
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