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Hi all,
I am sequencing small RNAs on a GAIIx Illumina platform. I prepared my small RNA seq library by adding 5' and 3' Illumina compatible adaptors and subsequent reverse transcription and PCR. The Illumina sequencing primer should bind to the 5' adaptor and the first nucleotide read should correspond to the 5' end of my original RNA molecule. However, in my data I still find a lot of sequences corresponding to the 5' adaptor/sequencing primer. Does anyone know how this is possible?
thanks!
Soetkin.
I am sequencing small RNAs on a GAIIx Illumina platform. I prepared my small RNA seq library by adding 5' and 3' Illumina compatible adaptors and subsequent reverse transcription and PCR. The Illumina sequencing primer should bind to the 5' adaptor and the first nucleotide read should correspond to the 5' end of my original RNA molecule. However, in my data I still find a lot of sequences corresponding to the 5' adaptor/sequencing primer. Does anyone know how this is possible?
thanks!
Soetkin.
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