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  • Help finish the pipeline for human whole exome sequencing with paired reads data

    The pipeline for human whole exome sequencing with paired reads data


    A, Align samples to genome (BWA): get BAM files
    bowtie
    1./bowtie -t -y -S hg18 -1 reads_1.fq -2 reads_2.fq reads.sam
    SAM Tools
    2.samtools view -bS reads.sam > reads.bam
    3.samtools sort reads.bam reads.sorted.bam
    4.samtools index reads.sorted.bam

    B,SNP or indel analysis:
    Last edited by wanguan2000; 11-17-2010, 07:26 PM.

  • #2
    Originally posted by wanguan2000 View Post
    The pipeline for human whole exome sequencing with paired reads data


    A, Align samples to genome (BWA): get BAM files
    bowtie
    1./bowtie -t -y -S hg18 -1 reads_1.fq -2 reads_2.fq reads.sam
    SAM Tools
    2.samtools view -bS reads.sam > reads.bam
    3.samtools sort reads.bam reads.sorted.bam
    4.samtools index reads.sorted.bam

    B,SNP or indel analysis:

    Hey wanguan,

    I dont know whether now you are active in the seqanswers forum. If you are there, kindly help me out.

    I am also like your stage at present.
    Once you index sortedbam files, what are the downstream analysis steps for SNP or indel calling.
    What are the tools required.

    Kindly let me know.

    Thank you,
    Vishnu.

    Comment

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