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I want to use AMOScmp to analyze illumina paired end data. AMOScmp requires the same number of paired file to build .afg file. The original fq files are paired. After I pass fq files separately through quality, duplicated sequences, and human DNA control, I find out that the paired end fa files have different number of reads. I want to remove unpaired reads from paired end reads to get two fa files with the same number of reads. Does anybody have script or know what software to help me to solve the problem?

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What's the format of the read IDs? For example, do paired reads off a given sequence fragment end in /1 and /2, with the preceding characters being identical between the two? If so, it may make things easier to deal with. –  Matt LaFave Jun 12 '13 at 13:20

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