output unmapped file in STAR alignment

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5.7 years ago

linjc.xmu ▴ 30

Hi All. I am using STAR alignment to remove rRNA reads, and collect unmapped reads for further alignment. My command line is: STAR --genomeDir ./genome/index/rRNA/ --readFilesIn RA1_R1.fastq RA1_R2.fastq --clip3pNbases 12 --clip5pNbases 50 --outFileNamePrefix rRNA1 --outReadsUnmapped Fastx

However, the output unmapped file mix read1 and read2 together, not in a separated R1.fastq and R2.fastq. Does anyone know how to set parameters? Thanks a lot.

alignment • 3.2k views

ADD COMMENT • link 5.7 years ago by linjc.xmu ▴ 30

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Which version of STAR are you using?

ADD REPLY • link 5.7 years ago by Devon Ryan 104k

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STAR_2.5.3a, thanks.

ADD REPLY • link 5.7 years ago by linjc.xmu ▴ 30

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Maybe this is fixed in the latest release (2.6.1a).

ADD REPLY • link 5.7 years ago by Devon Ryan 104k

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