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ZipperBams failed. Error: processed all unmapped reads but there are mapped reads remaining to be read. #978
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Somehow the |
I used STAR to map the uBAM, so the code looks weird, 2)then I extract fastq from uBAM, mapped them using STAR, forgive me that I didn't find ways to mapping one fastq file using STAR.
All commands above runs fine, but After I GroupReadsByUmi, CallMolecularConsensusReads, FilterConsensusReads, and mapping them sencond time, ZipperBams have problem;
STAR alignment code is like it above, and then picard sorted; Tips: using picard sortBam is because I used to use picard mergeBam to merge unmapped and mapped reads; I know the sort_order need to be the same when using picard mergeBam; (why I didnt use samtools sort is that some BAM files didnt support samtools's sort somehow.) |
Did you mean that '/A' is necessary for ZipperBams? And that should be retain whatever I run command on it? |
hello! I'm doing with sequencing data with UMI, I followed #fgbio-best-practise-fastq---consensus-pipeline
When I run fgbio ZipperBams to merge my consensus.ubam and consensus.mapped.bam, there is an exception:
Exception in thread "main" java.lang.IllegalStateException: Error: processed all unmapped reads but there are mapped reads remaining to be read.
and I check my two bam files; they all are queryname sorted, have same number of reads, the difference between them is all of queryname of ubam have suffix "/A". like this:
I found it is caused by fgbio CallConsensusReads...
I wanna know whether this is the problem caused ZipperBams failed, or how to deal with this problem(ZipperBams)?
#my fgbio version is 2.2.2-3a74fd2-SNAPSHOT
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