A strong promoter and its production of vitamin b 12 Application of the strain
A strong promoter and purpose technology, applied to vitamin B12-producing strains, plasmids and transformants containing the plasmid vector, strong promoter field, can solve the problem of limited number of high-efficiency promoters
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Embodiment 1
[0021] Example 1: Construction of a promoter-containing plasmid vector
[0022] 1. Preparation of vector containing reporter gene
[0023] Using the primers gfp-EcoRI-F and gfp-KpnI-R in Table 1, the ECE164 plasmid (Yafeng Song Jonas M. Nikoloff Gang Fu, Jingqi Chen, Qinggang Li, Nengzhong Xie, Ping Zheng, Jibin Sun, Dawei Zhang*. Promoter screening from Bacillus subtilis in various conditions hunting for synthetic biology and industrial applications. PLoS One .2016Jul 5; 11(7):e0158447.doi:10.1371 / journal.pone.0158447.) was used as a template, amplified by PCR, and introduced EcoRI and KpnI restriction sites to obtain the gfp fragment of the green fluorescent protein gene. After verification by electrophoresis, DpnI enzymatic treatment, and electrophoresis gel recovery, the purified gfp fragment was obtained. The purified gfp fragment and the pBBR1MCS2 plasmid were double-digested with EcoRI and KpnI, respectively, and the two double-digested products were ligated ove...
Embodiment 2
[0029] Example 2: Promoter P29 produces vitamin B in different 12 Activity assays in strains
[0030] 1. Transformation—three-parent transformation method
[0031] Taking S. meliloti as an example, the plasmid pBBR-P29-gfp in Example 1 was transferred into S. meliloti according to the three-parent method to obtain S. meliloti: SM / pBBR-P29-gfp. Specific steps are as follows:
[0032] (1) Inoculate the newly activated Sinorhizobium meliloti CGMCC NO.9638, Escherichia coli (containing the corresponding plasmid) and the helper vector MT616, and shake culture in the incubator at 30°C and 37°C respectively until the OD value is about 1.0;
[0033] (2) Under aseptic conditions, transfer 500 μL each of Sinorhizobium meliloti CGMCC NO.9638, MT616 and Escherichia coli to 1.5 mL sterile EP tubes and centrifuge at 12,000 rpm for 1 min at 4°C.
[0034] (3) Discard the supernatant under aseptic conditions, and suspend the precipitate with 1 mL of 0.85% sterile saline.
[0035] (4) Centrif...
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