Dear all
I’ve sent a 8-indecies pooled sample for TruSeq Small RNA library illumina sequencing. Mention that I didn’t use kit and I used CATS protocol to make the library. QC was passed successfully. Concentration was 574ng/µl and 3594 nM. The size was 246 bp. Now my problem is that the company informed me that due to base concentration issue, they can’t calculate cluster density. Sequencing went successfully after 8 cycle. In order to fix this issue, they told me need put phiX more than 50% but they can’t guarantee the result. and I might get the half of the data except the amount of PhiX rate. Now I want to know is that amount of result scientifically validate. Or is there any other way to get a better result?
I’ve sent a 8-indecies pooled sample for TruSeq Small RNA library illumina sequencing. Mention that I didn’t use kit and I used CATS protocol to make the library. QC was passed successfully. Concentration was 574ng/µl and 3594 nM. The size was 246 bp. Now my problem is that the company informed me that due to base concentration issue, they can’t calculate cluster density. Sequencing went successfully after 8 cycle. In order to fix this issue, they told me need put phiX more than 50% but they can’t guarantee the result. and I might get the half of the data except the amount of PhiX rate. Now I want to know is that amount of result scientifically validate. Or is there any other way to get a better result?
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