cDNA generation for targeted RNA amplicon sequencing

Holly A. Rees; Christopher Wilson; Jordan L. Doman; David R. Liu

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cDNA generation for targeted RNA amplicon sequencing

HR Holly A. Rees

CW Christopher Wilson

JD Jordan L. Doman

DL David R. Liu

This method is extracted from research article: Sci Adv, May 2019

Analysis and minimization of cellular RNA editing by DNA adenine base editors

DOI: 10.1126/sciadv.aax5717

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cDNA generation was performed with SuperScript IV (Thermo Fisher Scientific) according to the manufacturer’s instructions. A poly-T primer was used to selectively amplify mRNAs in the cDNA synthesis step. The optional step of RNase degradation before amplification of cDNAs was included to improve the efficiency of PCR. We note that this step was particularly important for RSL1D1 PCR.

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