Flanking sequence of exogenous event inserting vector for transgenic rape Ms8 and its application
A technology of exogenous insertion and flanking sequences, which is applied in the fields of application, genetic engineering, plant gene improvement, etc., and can solve the problems of specificity and characterization that have not yet been discovered
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[0041] 1. PCR amplification of the flanking sequence of the transgenic rapeseed Ms8 event exogenous insertion vector
[0042] First preheat 20% SDS to 65°C, take 15ml SDS extraction buffer (0.1TrisHCl, 0.05MEDTA, 1M NaCl pH8.0) and add it to a 50ml centrifuge tube, then add 2.5μl β-mercaptoethanol, mix well; grind with liquid nitrogen About 3g of leaves, transfer the powder to 50ml of 50ml centrifuge tube containing extraction buffer, shake and mix on the shaker, add 2ml of preheated 20% SDS, mix well, 65 ℃ water bath for at least 30 minutes, during which it should be light Shake the test tube gently; after the water bath, quickly place the centrifuge tube on ice, add 3ml 3M KAc, mix well, and place on ice for 30 minutes; centrifuge at 5000g at 4°C for 5min; transfer the supernatant to a new 50ml centrifuge tube, add 2 / 3 volume of isopropanol, mix well, place at -20°C for more than 30min; centrifuge at 6000g, 4°C for 15min, pour off the supernatant, wash with 75% ethanol, dry ...
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