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A kind of Saccharomyces cerevisiae recombinant strain and its construction method and application
A technology of Saccharomyces cerevisiae and its construction method, which is applied in the field of Saccharomyces cerevisiae recombinant bacteria and its construction, and can solve the problems of low catalytic efficiency of exogenous pathway enzymes, etc.
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Embodiment 1
Bgl II was double digested, and the obtained fragment was the same as the pUMRI-13 double digested by EcoR I and Bgl II (GenBank:
KM216415.1) plasmid was connected for transformation, and the pUMRI-13-HpaC plasmid was constructed.
PCR reaction system is as follows:
[0065]
The PCR program is as follows:
[0067]
Plasmid or gene fragment restriction enzyme digestion system is as follows:
[0069]
[0070]
[0071] 37° C., digested with enzyme for 2h. The digested products were separated by 1.0% agarose gel electrophoresis, and the gel with gene fragments was excised.
And purified and recovered with a gel recovery kit.
[0073]
[0073]
22 DEG C, the enzyme is connected for 50min, and the ligation product is transformed into E. coli competent state, placed in a 37 DEG C incubator and cultivated
The positive clones obtained overnight were used for plasmid extraction.
Embodiment 2
[0080] Enzymatic cleavage conditions: place 50° C. for cleavage for 2-3 hours.
Embodiment 3
[0086] (2) Get 50 μL of supernatant into a new 1.5mL EP tube, add 950 μL of purified water and dilute 20 times.
[0087] (3) Use a 0.22 μm water-based needle filter to filter the obtained sample for the determination of caffeic acid.
[0088] Quantitative analysis of caffeic acid: the sample was analyzed using an Agilent 1200 high performance liquid chromatograph. Chromatographic conditions
[0089]
PUM
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