Primer, kit and cloning method for limit dextrinase gene cloning
A limit dextrinase and kit technology, which is applied in biochemical equipment and methods, enzymes, hydrolase and other directions, can solve the problem that the full-length limit dextrinase gene cannot be obtained, the RNA purity and quality are not high, and malt RNA extraction is difficult. and other problems, to solve the problem of N-terminal codon preference, facilitate heterologous expression, and achieve the effect of simple operation.
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[0037] Example 1: Cloning of extreme dextrinase in malt
[0038] 1) Malt RNA extraction and reverse transcription
[0039] Place the filter paper in a Petri dish and moisten the filter paper with distilled water to prepare a germination bed. Take 100 grains of Baudin barley seeds and put them evenly in filter paper, and germinate them at 18°C for five days. The degerminated malt was rapidly ground into powder in liquid nitrogen, and then malt RNA was extracted according to the instructions of the RNAprep pure Plant Kit kit from TIANGEN Company, and stored at -80°C. Using the extracted RAN as a template, reverse transcription was performed according to the instructions of TaKaRa's PrimeScript RT-PCR Kit kit to obtain malt cDNA, which was used as a template for limiting dextrinase amplification.
[0040] 2) Segmented amplification of limit dextrinase
[0041] Firstly, it is amplified in 4 segments, and the primer combinations are: SEQ ID NO.2 / SEQ ID NO.3, SEQ ID NO.4 / SEQ ID...
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