A kind of chitinase cmchi6 gene and its cloning expression and application
A technology of chitinase and colloidal chitin, applied in the field of genetic engineering, can solve the problems of low product yield, poor product biological activity, large process energy consumption, etc.
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Embodiment 1
[0045] Example 1 Chitinase cm Amplification of the Chi6 gene
[0046] The present invention designs primers based on the reported gene sequence of SYBC-H1 chitinase, and obtains SYBC-H1 chitinase by polymerase chain reaction (PCR) cm Conserved sequence of Chi6.
[0047] Using PCR technology, donated by Hao Zhikui of Jiangnan University Chitinolyticbacter meiyuanensis Genomic DNA of SYBC-H1 was used as a template, and primers were designed using Primer5.0 software, respectively: upstream primers Chi -F (SEQID No.2): 5'-CCCAAGCTTCTACTTTGCCGCCGGAAT-3' designed with NdeI restriction site; downstream primer Chi -R (SEQ ID No.3): 5'-CCCAAGCTTCTACTTTGCCGCCGGAAT-3' is designed with a HindIII restriction site.
[0048] PCR reaction system:
[0049]
[0050] PCR reaction conditions: 95°C pre-denaturation, 2min; 95°C denaturation for 20s, 52°C annealing, 20s, 72°C extension, 2min, a total of 30 cycles; 72°C extension, 5min, and finally 4°C incubation.
[0051] After the PCR r...
Embodiment 2
[0052] Example 2 Plasmid vector pColdI- Cmchi6 and the cloned strain pColdI- Cmchi6 - E. coli Preparation of Trans1T1
[0053] 1. Purify and recover the PCR product obtained in Example 1, using a TaKaRa company kit (TaKaRa DNALigation Kit);
[0054] 2、 Construction of plasmid vector pColdI- Cmchi6
[0055] The DNA sequence amplified by PCR and the pColdI vector were double-digested with the same restriction enzymes NdeI and HindIII, and the digested products were recovered and purified, and used T 4 DNA ligase was connected to obtain the plasmid vector pCooldI- Cmchi6 ;
[0056] 3. Construction of cloning strain pColdI- Cmchi6 - E. coli Trans1T1
[0057] The plasmid vector pColdI- Cmchi6 convert to E. coli Trans 1T1: (1) Take 20 μl of competent cells Trans 1T1 frozen and thawed on ice, and mix them gently in the above 10 μl connection reaction solution; (2) After standing on ice for 30 minutes, heat shock at 42°C for 45 seconds , and then quickly put it ...
Embodiment 3
[0062] Construction of recombinant expression strain pColdI- Cmchi6 - E. coli BL21(DE3)
[0063] 1. Strain cultivation: the constructed recombinant plasmid pColdI- Cmchi6 extracted from the cloning host and retransformed into E. coli. BL21(DE3) competent cells. The conversion operation was as the conversion step in the above-mentioned Example 2. Finally, 1-2 single colonies were picked and inoculated into 5ml LB medium containing ampicillin with a final concentration of 0.2%, and cultivated overnight at 37°C.
[0064] 2. Main culture: After 12 hours of culture, transfer to 100ml LB / Amp medium according to the inoculum size of 1%, and shake culture at 37°C until OD 600 =0.4-0.6.
[0065] 3. Induced expression: Add IPTG at a final concentration of 0.05mM to induce bacterial cells, and induce at 18°C and 200rpm for 20h at low temperature.
[0066] 4. Collect whole cells: Centrifuge at 4°C, 6000rpm for 8-10min to collect the bacteria, mix with 10ml PBS, and then ultr...
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