A method for virus-induced gene silencing mediated by trv vector in forsythia leaves
A carrier, forsythia technology, applied in the field of genetic engineering, can solve the problems of restricting the molecular biology research of forsythia, and there is no efficient gene function verification method.
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[0028] 1. Acquisition of experimental materials: Potted forsythia cutting seedlings were taken, re-cut and placed in an artificial climate chamber for cultivation, and set aside. Culture conditions: light 300μmol·m -2 ·s -1 , 16h, 22°C, dark 8h, 18°C, humidity 60%.
[0029] 2. Recombinant vector construction: The amplified Forsythia phytoene dehydrogenase (hereinafter referred to as: FsPDS) gene fragment was connected to the TRV virus-induced gene silencing vector pTRV2 by the method of genetic engineering to obtain the recombinant pTRV- FsPDS. Specific steps are as follows:
[0030] Preparation of cDNA: Extract the total mRNA of Forsythia leaves according to the Trizol method, perform reverse transcription of the total mRNA according to the operation instructions of the Tiangen Reverse Transcription Kit, obtain Forsythia cDNA, dilute 20 times, and store at -20°C for later use.
[0031] Amplification of Forsythia PDS gene fragment (FsPDS):
[0032] PCR primers were design...
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