Originally posted by pmiguel
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Looks like "Picard MarkDuplicates" was used.
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Phillip
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These would look like "optical duplicates", no?
I remember a recent thread where these were found in some MiSeq runs at high frequency.
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PhillipLeave a comment:
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They should merge duplicate reads in contiguous wells for extra-high quality!Leave a comment:
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There are tools to address duplicates (e.g. dedupe.sh from BBMap) but they are not cluster location/adjacency aware. Picard should be in this category too unless it has been modified.Originally posted by DNATECH View Post
I was wondering if this would be something illumina should implement in bcl2fastq software, specially if duplicates will be a problem with less than perfect libraries.Leave a comment:
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Hi GenoMax,
Thanks! Currently there are no local duplicate metrics in the SAV viewer and no options in bcl2fastq for flagging or filtering for these cases.
People working with X Ten data get their data already aligned and might be able to use picard etc.? However the HiSeq 3000/4000 will be used for all kinds of applications were alignment based analyses are not an option.Leave a comment:
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I doubt that software for this exists in the wild since you are asking for a very specific operation based on the location of the cluster for a condition that may occur with a relatively new technology (unless those sites that have had HiSeq X Ten have implemented something for this). Wonder if illumina can include mitigation for that in bcl2fastq itself.Leave a comment:
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HiSeq3000/4000 duplicate removal
Hi All,
Our Illumina FAS mentioned that in underloaded lanes on the patterned flow-cells even PCR-free libraries can generate significant numbers of duplicates (clusters swapping over the "walls" into the next empty nanowell if given enough time?).
http://dnatech.genomecenter.ucdavis....data-download/
Would you know of any software that can analyze/remove duplicates based on the coordinate information in the read headers (without any alignments)?
Thanks in advance,
LutzLast edited by DNATECH; 05-07-2015, 06:01 PM.
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