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  • gringer
    replied
    Originally posted by shawpa View Post
    samtools merge /out.bam /path_to_file/*.bam
    If this is the precise command you used, you may get better results from removing the initita forward slashes.

    Leave a comment:


  • cbeck
    replied
    Hi Shawpa,
    As an aside, you don't need to merge the bam files when calling the UnifiedGenotyper, you can use multiple -I parameters. Note that you can expect compute time to increase in a non-linear fashion when doing this.

    Leave a comment:


  • shawpa
    started a topic merging many bam files-novice needs help please

    merging many bam files-novice needs help please

    I have 152 coordinate sorted bam files. I want to merge them. I have tried both Samtools merge and Picard. I used Samtools merge before on some different data and it worked but I don't think that data was coordinate sorted and that might make a difference. The command I am trying to use is

    samtools merge /out.bam /path_to_file/*.bam

    I want it to merge all the files in that folder. I don't get a specific error but it prints out the samtools merge usage parameters. So I guess I am missing something in my command. The following is what I have done so far in my pipeline:

    1. aligned with bowtie 2 (output sam)
    2. sorted individual sam files output to individual bam files

    The end goal is to use GATK for variant analysis. According to http://seqanswers.com/wiki/How-to/exome_analysis, I need to put some kind of -r argument in Samtools when I am processing to add an @rq (or something like that).

    I am lost at this moment and I have searched and searched to try and find an answer on the forums.

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