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hi everyone,
i just had my ChIP seq libraries come off a lane from illumina hi-seq (6 samples in there) and was told by my facility that the barcode reads have all failed.
basically i have perfect reads for all 100 bp of my insert, then for some unknown reason when they begin barcode reads nothing happens.
i looked at the raw images and it basically goes from many tiny clear red glowing dots at basepair 100, to almost black blurriness for the 101 base.
(also had low cluster density but they don't think its related)
they're offered to rerun it in a rapid run (to get higher cluster density) and it just came off again with excellent density now but still no barcode reads.
their words "The adaptors are there, but something is interfering with the barcode reads".
"it looks like there might be something wrong with your adaptors (?). We simply didn’t get a barcode read again even though the cluster numbers are up to a reasonable level. Maybe the barcode read primer isn’t priming?"
is anyone aware of any common causes of this? i have friends who also used the same adaptors in their library prep and all have had sucess.
the inserts (without barcode information), i was able to map to my genome of interest and they all look ok (not adapter dimers)
i just had my ChIP seq libraries come off a lane from illumina hi-seq (6 samples in there) and was told by my facility that the barcode reads have all failed.
basically i have perfect reads for all 100 bp of my insert, then for some unknown reason when they begin barcode reads nothing happens.
i looked at the raw images and it basically goes from many tiny clear red glowing dots at basepair 100, to almost black blurriness for the 101 base.
(also had low cluster density but they don't think its related)
they're offered to rerun it in a rapid run (to get higher cluster density) and it just came off again with excellent density now but still no barcode reads.
their words "The adaptors are there, but something is interfering with the barcode reads".
"it looks like there might be something wrong with your adaptors (?). We simply didn’t get a barcode read again even though the cluster numbers are up to a reasonable level. Maybe the barcode read primer isn’t priming?"
is anyone aware of any common causes of this? i have friends who also used the same adaptors in their library prep and all have had sucess.
the inserts (without barcode information), i was able to map to my genome of interest and they all look ok (not adapter dimers)
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