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Hi all,
I used KAPA RNA hyperprep kit to generate libraries and checked the distribution by Tapestation4200. However, there were 2 peaks in all my 6 samples(B1,C1,D1 and D2, E2, F2), one around 320nt, the other ~470nt.
I tried to heat and re-anneal these samples, however, after heating, it seemed that all peaks were gone(attached pic, lane E1, F1, G1,A2, B2,C2).
Is it OK to use these libraries for sequencing?
Another question is that I made a terrible mistake and heated the original libraries. Now all I have is ~8uL of diluted libraries. Can I amplify these libs again by PCR, because the RNA used for lib. preparation is quite limited?
Any suggestions are appreciated.
Thank you.
I used KAPA RNA hyperprep kit to generate libraries and checked the distribution by Tapestation4200. However, there were 2 peaks in all my 6 samples(B1,C1,D1 and D2, E2, F2), one around 320nt, the other ~470nt.
I tried to heat and re-anneal these samples, however, after heating, it seemed that all peaks were gone(attached pic, lane E1, F1, G1,A2, B2,C2).
Is it OK to use these libraries for sequencing?
Another question is that I made a terrible mistake and heated the original libraries. Now all I have is ~8uL of diluted libraries. Can I amplify these libs again by PCR, because the RNA used for lib. preparation is quite limited?
Any suggestions are appreciated.
Thank you.
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