Hi
We've just started using the Illumina Next-Seq platform and haven't been getting good results sequencing our CEL-Seq2 library (75cycle, R1=15bp, R2=77bp), as opposed to what we've been getting previously using Hi-Seq.
QC apparently "looks fine". But I'm not convinced given that the deviation bars in FastQC are huge.
%Q30 is ~78%.
The problem is that %mapping to the reference genome is only ~20%, even after discarding sequences with ave Qscore<30.
Tech advised that we've probably overloaded the DNA.
We paid for another run of the same library at 30% less loading (~0.9pM) and 20% phiX-spike in. The same problem persists. %Q30 is better at 88%, but again, the sequences are full of N's (20% of R1 sequences are all Ns) and map at 20%.
We've been told it could be the library. But there are definitely enough DNA at ~200-400bp size.
I'd like to get an opinion on whether this is likely a library-prep problem (old reagents?) or sequencing-problem (settings?)...? What could be the triggering issue?
Thank you!!!
What did your PhiX results look like? Same story?
Hmmm.... I kind of assumed PhiX reads were not included in my fastq files and were only used for calculating the error rates. I might have to double check then. Thank you.
Not 100% sure with the NextSeq. The software on the machine may have filtered them out already - but they got sequenced, so the data should be available I would expect. You might have to recall them from the bcl files perhaps.
It would tell you if it’s your input DNA that’s the issue though, if the PhiX looks good.
does the cluster density look okay?
1st run: ~190 2nd run: ~ 95 (I'm not sure how this converts to the 170-220 k/mm2 recommended range for NextSeq, probably the same scale?)
Have a look in RunCompletionStatus.xml file for ClusterDensity
That's the number. 95
if it says
<ClusterDensity>95</ClusterDensity>then its quite low. Its under clustered