Hi people.
I was wondering if anybody had had any problems with the illumina protocol for making the libraries for paired end sequencing. We previously did some ChIP-seq before (not paired end) and the first time we ran into problems with primer dimers and had to lower primer and adapter concentrations.
This time we are sequencing DNA (not ChIPed), are there any similar common problems? And do you do the PCR enrichment, I hear some people are missing this out and getting good results?
Cheers, James
I was wondering if anybody had had any problems with the illumina protocol for making the libraries for paired end sequencing. We previously did some ChIP-seq before (not paired end) and the first time we ran into problems with primer dimers and had to lower primer and adapter concentrations.
This time we are sequencing DNA (not ChIPed), are there any similar common problems? And do you do the PCR enrichment, I hear some people are missing this out and getting good results?
Cheers, James
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