A kind of Saccharomyces cerevisiae engineered bacteria producing glycyrrhetinic acid or its precursor and its construction method
A technology of Saccharomyces cerevisiae and glycyrrhetinic acid, applied in the direction of microorganism-based methods, biochemical equipment and methods, botany equipment and methods, etc., can solve the problems of low efficiency, high cost, difficult chemical synthesis under molecular structure synthesis conditions, etc. , to achieve the effect of broad application prospects and convenient production process
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experiment example 1
[0053] Experimental example 1: Acquisition of related genes in the glycyrrhetinic acid synthesis pathway
[0054] A. Acquisition of β-amyresinol synthase gene
[0055] According to the sequence of the β-amyresinol synthase gene (Genbank registration sequence number is AB037203), through codon optimization, the codons of the β-amyresinol synthase gene have yeast preference, and the optimized gene sequence generated is SEQ ID No. 1.
[0056] B. Acquisition of the CYP450 oxidase gene that oxidizes the carbon 11 of β-amyresinol
[0057] According to the sequence of the CYP450 oxidase CYP88D6 gene (Genbank registration number is AB433179), the codon of the CYP88D6 gene has yeast preference through codon optimization, and the optimized gene sequence generated is SEQ ID No.2.
[0058] Primers were designed according to the sequence of CYP450 oxidase CYP88D6 gene (Genbank registration sequence number is AB433179), SEQ ID No.3: 5'-ATGGAAGTACATTGGGTTTGC-3' and SEQ ID No.4: 5'-CTAAGCAC...
experiment example 2
[0068] Experimental Example 2: Construction of Expression Cassette
[0069] Construction of A, β-amyresinol synthase expression cassette
[0070] The left homology arm HOL, yeast promoter P FBA1 , β-amyresinol synthase gene, yeast terminator T CYC1 The method of overlapping extension PCR is used to connect in this way to obtain the expression cassette P of β-amyresinol synthase FBA1 -bAS-T CYC1
[0071] B. Construction of the CYP450 oxidase expression cassette at the carbon 30 position of oxidizing 11-oxygen-β-amyresinol
[0072] Yeast terminator T CYC1 , yeast promoter P GPD , CYP450 oxidase gene CYP72A154 or CYP72A63, yeast terminator T ADH1 The method of overlapping extension PCR is used for this connection, and the CYP450 oxidase T at the carbon 30 position of oxidizing 11-oxo-β-amyresinol is obtained CYC1 -P GPD –CYP72A154-T ADH1 or T CYC1 -PGPD -CYP72A63-T ADH1
[0073] C, construction of the CYP450 oxidase expression cassette at the carbon 11 position of ox...
experiment example 3
[0079] Experimental Example 3: Acquisition of Saccharomyces cerevisiae Engineering Bacteria Producing Glycyrrhetinic Acid
[0080] Yeast Transformation of Fragments Using the Lithium Acetate Method
[0081] Using the homologous recombination function of the yeast itself, all the expression cassettes constructed above were co-transferred into the HO site of the Saccharomyces cerevisiae INVSc1 genome. After transformation, use the YPD solid plate supplemented with Geneticin (G418) for screening, and the obtained transformants are transferred to the YPD liquid medium supplemented with Geneticin (G418) for 1-2 days, the genome is extracted, and positive clones are identified by PCR , plate streak or glycerol bacteria preservation.
[0082] On the basis of the existence of the MVA pathway in the yeast itself, the glycyrrhetinic acid synthetase is introduced exogenously to obtain the engineering strain of Saccharomyces cerevisiae with the function of producing glycyrrhetinic acid. ...
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Abstract
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