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Hi,
I have a relatively basic question. I am performing RNA-seq on some small tissue samples and I have constructed my first set of libraries for Illumina sequencing using the Ovation/NuGen SPIA system. My libraries are at about 2ng/ul concentration, or around 6nM. My question is: how do you known when to do PCR amplification of your libraries? I think that my RNA is concentrated enough to cluster directly onto a flow cell, but I have been told that amplification is usually necessary for SPIA. On the other hand, I would like to reduce amplification bias as much as possible.
Any recommendations here? Any rough guidelines that you use to determine whether to amplify or not?
Thanks in advance, zrl
I have a relatively basic question. I am performing RNA-seq on some small tissue samples and I have constructed my first set of libraries for Illumina sequencing using the Ovation/NuGen SPIA system. My libraries are at about 2ng/ul concentration, or around 6nM. My question is: how do you known when to do PCR amplification of your libraries? I think that my RNA is concentrated enough to cluster directly onto a flow cell, but I have been told that amplification is usually necessary for SPIA. On the other hand, I would like to reduce amplification bias as much as possible.
Any recommendations here? Any rough guidelines that you use to determine whether to amplify or not?
Thanks in advance, zrl
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