Mercurial > repos > eugen > bs_seq_test_2
changeset 6:54492fec12ba draft
Uploaded
| author | eugen |
|---|---|
| date | Thu, 16 Aug 2012 04:13:30 -0400 |
| parents | a2f7ecd6b400 |
| children | d49ae6a0ecda |
| files | bsmap_meth_caller.xml |
| diffstat | 1 files changed, 59 insertions(+), 0 deletions(-) [+] |
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--- /dev/null Thu Jan 01 00:00:00 1970 +0000 +++ b/bsmap_meth_caller.xml Thu Aug 16 04:13:30 2012 -0400 @@ -0,0 +1,59 @@ +<tool id="bsmap_meth_caller" name="BSMAP Methylation Caller"> + <requirements> + <requirement type='package'> + bsmap + </requirement> + </requirements> + <requirements> + <requirement type='package'> + samtools + </requirement> + </requirements> + <command interpreter="bash"> + bsmap_meth_caller.sh + input=$bsmap_sam + unique=$unique + properly=$properly + zero_meth = $zero_meth + rem_dup = $rem_dup + combine_cpg = $combine_cpg + trimN = $trimN + depth = $depth + output=$output + tempdir=$output.files_path + ref="${ filter( lambda x: str( x[1] ) == str( $bsmap_sam.metadata.dbkey ), $__app__.tool_data_tables['bsmap_fasta'].get_fields() )[0][3] }" + </command> + <inputs> + <param name="bsmap_sam" format="sam" type="data" label="BSMAP mapping output file" help="Must be in SAM format" /> + <param name="unique" type="boolean" truevalue="true" falsevalue="false" checked="False" label="Process only unique mappings/pairs" /> + <param name="properly" type="boolean" truevalue="true" falsevalue="false" checked="False" label="Process only properly paired mappings" /> + <param name="zero_meth" type="boolean" truevalue="true" falsevalue="false" checked="True" label="report loci with zero methylation ratios" /> + <param name="rem_dup" type="boolean" truevalue="true" falsevalue="false" checked="False" label="Remove duplicated reads" /> + <param name="combine_cpg" type="boolean" truevalue="true" falsevalue="false" checked="False" label="Combine CpG methylaion ratios on both strands" /> + <param name="trimN" type="integer" value="2" label="Trim N fill-in nucleotides in DNA fragment end-repairing" help="This option is only for pair-end mapping. For RRBS, N could be detetmined by the distance between cuttings sites on forward and reverse strands. For WGBS, N is usually between 0~3" /> + <param name="depth" type="integer" value="1" label="Minimum sequencing depth to report loci" /> + </inputs> + <outputs> + <data name="output" format ="bed" label="BSMAP methylation output" /> + </outputs> + <help> +**What it does** + +This methylation caller parses the BSMAP SAM output file into bed format. + + +**Output format** :: + + + Column Description + ---------------------- -------------------------------------- + 1 chr chromosome + 2 pos position + 3 strand strand + 4 context context (CHH,CHG,CpG) + 5 coverage totally sequenced Cs at that position + 6 methylated methylated Cs at that position + 7 percentage methylated percentage of 6 + </help> +</tool> +