Hyaluronan synthase mutant and application thereof
A hyaluronic acid synthase and mutant technology, applied in the field of bioengineering, can solve the problems of HA molecular weight reduction, pore instability, affecting hyaluronic acid synthase HA chain retention, etc., and achieve the effect of increasing production
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Embodiment 1
[0038] Example 1 Construction of integrated recombinant plasmid pGZA
[0039] Amplify and obtain the target gene shown in SEQ ID NO.1.
[0040] According to the plasmid map of pP43NMK, the primers P43-F and P43-RBS-R were designed respectively. Using the pP43NMK plasmid as the template, the standard PCR amplification system and procedures were used to amplify the promoter P 43 And RBS.
[0041] According to the pSKIZH plasmid information (Production of specific-molecular-weight hyaluronan by metabolicallyengineered Bacillus subtilis 168, Metabolic Engineering, 2016, Jinpeng), the primers pGZ-F and pGZ-R were designed respectively, and the pSKIZH plasmid was used as the template and standard PCR amplification System and procedures to amplify the vector pGZ, which is a T-carrier derivative with upstream and downstream homology arms (530bp) integrated into the nagA site on Bacillus subtilis 168 and lox71-Zeo-lox66 resistance marker.
[0042] Primer sequence information: 5’-3’ direction
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Embodiment 2
[0051] Example 2 Selection of mutation sites of hyaluronic acid synthase of Streptococcus zooepidemicus and construction of mutant library
[0052] Attached figure 1 Among them, the topological structure of hyaluronic acid synthase derived from Streptococcus zooepidemicus is predicted based on the structure of hyaluronic acid synthase derived from Streptococcus pyogenes and the homology between the two. F 58 -N 208 And Y 233 -P 318 It is the intracellular domain of Streptococcus zooepidemicus hyaluronic acid synthase, that is, two intracellular macrocyclic structures, and has substrate binding and catalytic activity. At the same time, after BLAST alignment of amino acid sequences, five conserved motifs located in the intracellular domain were found, namely V 158 DSDT 162 , L 198 TRL 201 , S 227 GPL-YRR 235 , G 258 DDR-LTN 265 , L 293 -QQ-RW-KS-FRE 306 . Design the amino acids near these 5 motifs to be mutated at the same time, while the conservative site remains unchanged, that is...
Embodiment 3
[0065] Example 3 High-throughput screening and shake flask rescreening of recombinant Bacillus subtilis mutant library
[0066] The 1500 Bacillus subtilis mutant strains obtained above were picked, and a single colony was inoculated on a 96 shallow-well plate of LB medium, and cultured at 200 rpm and 37°C overnight. Transfer 10% of the inoculum to the fermentation medium of 96 deep-well plates. The fermentation medium is: 20g / L yeast powder, 50g / L sucrose, potassium sulfate 3.9g / L, magnesium sulfate 1.5g / L, 50mM Phosphate buffer, pH 7.0. The amount of liquid in each well should not exceed 1 / 3 of the well volume, and the plate cover with good air permeability should be used and incubated at 200rpm 37℃ for 48h.
[0067] To collect hyaluronic acid in the fermentation broth, first add 1 volume of 0.1% (w / v) SDS solution, let it stand for 10 minutes, and centrifuge at 10000×g for 10 minutes at room temperature to remove cells. Add 2 volumes of absolute ethanol to the supernatant and m...
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