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2.1 Primary Analysis - Sequence processing

After sequencing, reads are mapped to the human genome reference (GRCh37). Then, there are some filtering steps in which the number of reads decreases until variant calling. Here, we describe how this reduction occurs in each pipeline.

BIER's pipeline

In this pipeline, there are four stages where the number of reads decreases (mapping, filter by mapping quality, remove duplicates and intervals realignment). This table shows reads remaining after these stages.

  • N_reads_forward and reverse: initial number of reads forward and reverse obtained in the exome sequencing process.
  • N_mapped_read_pairs: number of read pairs mapped to the human genome reference.
  • %_mapped_read_pairs: percentage of initial read pairs mapped to the human genome reference.
  • N_mapped_reads_mapq>10: number of mapped reads whose mapping quality (mapq) is higher than 10.
  • %_mapped_reads_mapq>10: percentage of initial mapped reads whose mapping quality (mapq) is higher than 10.
  • N_reads_single_hit: number of reads uniquely mapped to the human genome reference.
  • %_reads_single_hit: percentage of initial reads uniquely mapped to the human genome reference.
  • N_reads_single_hit_realigned: number of reads realigned in the exome capture kit targets.
  • %_reads_single_hit_realigned: percentage of initial reads realigned in the exome capture kit targets.

CNAG's pipeline

SampleN_reads_forwardN_reads_reverseN_mapped_read_pairs%_mapped_read_pairsN_read_pairs_single_hit%_reads_pairs_single_hit
SGT03831471997314719972709838086.102653341584.31
SGT07727308034273080342345099185.882290403183.87
SGT16127566691275666912366826585.862317078084.05
SGT18729730857297308572555460985.952489459783.73
SGT23030415770304157702625736886.332563941184.30
SGT23829472514294725142538614786.132477329284.06
SGT24129513223295132232536524685.952453954283.15
SGT27430394832303948322624267786.342569340684.53
espinos/results.primary.analysis.1438852228.txt.gz · Last modified: 2015/08/06 11:10 by cespinos
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