We usually multiplex 6 to 8 yeast genomes in one MiSeq run using 2x250bp paired end reads. So far we have always used N701 through N706 or N708 for the indices. Curiously, the percent reads for the N701 indexed genome is always the lowest, sometimes significantly, giving sub-optimal coverage of that genome. The percentage of all indexed reads is always about 98%. Any idea why N701 should give fewer reads than the other indices?
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I use Picogreen to quantitate each library and a Bioanalyzer to get the average size of each. From this I normalize each library to 4 nM, pool, dilute to 2 nM to denature, and load 12 pM. This gives a cluster density around 1000 K/mm2 and a pretty even distribution of the reads, except that there are fewer N701 reads relative to the other indices. I have not found qPCR to be helpful in getting better results.
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Yes, qPCR is superior, but Picogreen plus Bioanalyzer is what Illumina recommends in their protocol. My original question remains unanswered, i.e. why should N701 give many fewer copies with appropriate adapter incorporation compared to the other indices?
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The lower number of reads assigned to N701 has correlated only with N701 regardless of the genomic DNA used to make that library. The lower number of reads has occurred in 2x150 bp and 2x250 bp runs. It has also occurred with different index primer kits and with different species of yeast. I am going to avoid N701 whenever possible.
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N701 still the worst index
The problem with N701 continues. The N701 library always has the lowest representation in a pool, often too low for good coverage. The % unassigned reads is low (less than 2%) and there is no way to determine if most are from the N701 index, because our pools consist of strains of yeast differing only by a few snps. Doesn't anyone have a good explanation for this?
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universal i5 primer
Since I only need to use the i7 index reads to demultiplex ten yeast genomes per MiSeq run, the i5 primer does not need to have an index. I have a bunch of i5 primer minus an index, but wonder what concentration it should be (and what buffer it should be in) to be compatible with the Nextera PCR reaction. Does anyone out there know this?
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