Mutant type Taq DNA polymerase, nucleic acid extraction-free direct PCR amplification kit and application of mutant type Taq DNA polymerase
A polymerase and mutant technology, applied in the biological field, can solve the problems of low tolerance, many mutation sites, and increased cost of kits
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[0041] One embodiment of the method for preparing mutant Taq DNA polymerase includes the following steps S110-S120.
[0042] S110. Using the gene expression sequence of Taq DNA polymerase as the amplification template, and adding point mutation primers to perform point mutation PCR amplification to obtain the target gene expression sequence; wherein, the protein encoded by the target gene expression sequence is the same as the wild-type Taq DNA The glutamic acid at position 709 was mutated to glutamine compared to the polymerase.
[0043] S120, transforming the target gene expression sequence obtained in S110 into a host cell, and inducing expression of the transformed host cell to obtain a mutant Taq DNA polymerase.
[0044] Specifically, search the gene sequence of Taq DNA Polymerase on NCBI, and perform codon optimization to design the gene coding sequence of mutant Taq DNA polymerase. Use the glutamic acid E mutation at position 709 of Taq DNA Polymerase to design two poi...
Embodiment 1
[0066] The preparation of embodiment 1 mutant type Taq DNA polymerase
[0067] Find the gene sequence of Taq DNA Polymerase on NCBI (GenBank sequence number: D32013.1), and optimize the codons to design the target gene expression sequence. Use the glutamic acid E mutation at position 709 of Taq DNA Polymerase to design two point mutation primers for glutamine Q as follows:
[0068] F-primer: CGAAAGTTCGCGCTTGGATC CAA AAAACCCTGGAAGAAGG (as shown in SEQ ID No.3)
[0069] R-primer: CCTTCTTCCAGG GTT TTTTGGATCCAAGCGCGAACTTTCG (as shown in SEQ ID No.4)
[0070] Synthesized by Shanghai Sangon Bioengineering Co., Ltd. Using the PTaq DNA Polymerase gene extracted by our company as a template, the above-mentioned pair of complementary primers are used for point mutation PCR amplification to obtain the point mutation product RiTaq (target gene expression sequence), and the PTaq template is removed with the restriction endonuclease Dnp I , after purifying the product, sequence it, r...
Embodiment 2
[0072] Detection Kit for Direct PCR Amplification Without Nucleic Acid Extraction
[0073] The kit includes mutant Taq DNA polymerase, treatment solution, PCR enhancer and dNTP in Example 1, and the treatment solution contains 50mmol / L Tris-HCl (pH 9.1), 25mmol / L MgCl 2 , 160mmol / L (NH4 ) 2 SO 4 and 0.25% Brij-58. The PCR enhancer is betaine.
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