Hi guys! I'm a newbie to this forum so please bear with me!
I've prepared lots of Illumina libraries before (RADseq, RNAseq..) and am now doing miRNAseq using the TruSeq smallRNA kit, using total RNA input.
I've got to the pre-gel purification stage (post-PCR) and have run an aliquot on the Agilent Bioanalyser as encouraged to do by the protocol. However, the on-site Bioanalyser isn't new enough to use the suggested High Sensitivity DNA chips, and I had to use a normal DNA chip. So basically I didn't really know what I was looking for in my results graphs.
I do know that I am supposed to see a peak at ~145-160bp (the adapter-ligated miRNA size). And I do have small peaks in roughly that size region.
HOWEVER, I also have maaaassive peaks at ~270bp. I have no idea what this could be, and nobody I've spoken to knows either! I know it isn't contamination, because a sample that is effectively my -ve control (don't ask) didn't have any peaks. I'm just concerned that, as the peaks are so big, the adapters (although designed to ligate to miRNA) have also ligated to bigger RNA too, and so have also been amplified in PCR.
Would this be possible, and/or does anybody have any idea what these 270bp peaks are doing in my library prep?!
Thanks so much
I've prepared lots of Illumina libraries before (RADseq, RNAseq..) and am now doing miRNAseq using the TruSeq smallRNA kit, using total RNA input.
I've got to the pre-gel purification stage (post-PCR) and have run an aliquot on the Agilent Bioanalyser as encouraged to do by the protocol. However, the on-site Bioanalyser isn't new enough to use the suggested High Sensitivity DNA chips, and I had to use a normal DNA chip. So basically I didn't really know what I was looking for in my results graphs.
I do know that I am supposed to see a peak at ~145-160bp (the adapter-ligated miRNA size). And I do have small peaks in roughly that size region.
HOWEVER, I also have maaaassive peaks at ~270bp. I have no idea what this could be, and nobody I've spoken to knows either! I know it isn't contamination, because a sample that is effectively my -ve control (don't ask) didn't have any peaks. I'm just concerned that, as the peaks are so big, the adapters (although designed to ligate to miRNA) have also ligated to bigger RNA too, and so have also been amplified in PCR.
Would this be possible, and/or does anybody have any idea what these 270bp peaks are doing in my library prep?!
Thanks so much
Comment