Mercurial > repos > yufei-luo > s_mart
comparison SMART/galaxy/mapperAnalyzer.xml @ 18:94ab73e8a190
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| author | m-zytnicki |
|---|---|
| date | Mon, 29 Apr 2013 03:20:15 -0400 |
| parents | 440ceca58672 |
| children | 0ab839023fe4 |
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| 17:b0e8584489e6 | 18:94ab73e8a190 |
|---|---|
| 1 <tool id="mapperAnalyzer" name="mapper analyzer"> | 1 <tool id="mapperAnalyzer" name="mapper analyzer"> |
| 2 <description>Read the output of an aligner, print statistics and possibly translate into GFF, BED or GBrowse formats. </description> | 2 <description>Read the output of an aligner, print statistics and possibly translate into GFF, BED or GBrowse formats. </description> |
| 3 <requirements> | |
| 4 <requirement type="set_environment">PYTHONPATH</requirement> | |
| 5 </requirements> | |
| 3 <command interpreter="python"> | 6 <command interpreter="python"> |
| 4 ../Java/Python/mapperAnalyzer.py -i $formatType.inputFileName1 | 7 ../Java/Python/mapperAnalyzer.py -i $formatType.inputFileName1 |
| 5 #if $formatType.FormatInputFileName1 == 'bed': | 8 #if $formatType.FormatInputFileName1 == 'bed': |
| 6 -f bed | 9 -f bed |
| 7 #elif $formatType.FormatInputFileName1 == 'gff3': | 10 #elif $formatType.FormatInputFileName1 == 'gff3': |
| 177 <param name="remove" type="boolean" truevalue="-x" falsevalue="" checked="false" label="remove transcripts when exons are short"/> | 180 <param name="remove" type="boolean" truevalue="-x" falsevalue="" checked="false" label="remove transcripts when exons are short"/> |
| 178 <param name="remain" type="boolean" truevalue="-r" falsevalue="" checked="false" label="print the unmatched sequences "/> | 181 <param name="remain" type="boolean" truevalue="-r" falsevalue="" checked="false" label="print the unmatched sequences "/> |
| 179 </inputs> | 182 </inputs> |
| 180 | 183 |
| 181 <outputs> | 184 <outputs> |
| 182 <data name="outputFileGFF" format="gff3" label="[mapperAnalyzer] out file"/> | 185 <data name="outputFileGFF" format="gff3" label="[mapper analyzer] output file"/> |
| 183 </outputs> | 186 </outputs> |
| 184 | 187 |
| 185 <help> | 188 <help> |
| 186 Maybe the first program you may use. It reads a set of mapping given by the tool you have used to map your data on the reference genome and translate it to a set of genomic coordinates. You also have the possibility to extract only those that you are interested in (few matches in the genome, few errors in the mapping, etc.). You can also select those reads which map less than a given of times in the genome. Moreover, you can output the data in various different formats, which you can use to visualize them *via* UCSC genome browser or GBrowse. Unmatched reads can be written in an other file, in case you would like to try to map them with another tool (may sometimes work!). | 189 Maybe the first program you may use. It reads a set of mapping given by the tool you have used to map your data on the reference genome and translate it to a set of genomic coordinates. You also have the possibility to extract only those that you are interested in (few matches in the genome, few errors in the mapping, etc.). You can also select those reads which map less than a given of times in the genome. Moreover, you can output the data in various different formats, which you can use to visualize them *via* UCSC genome browser or GBrowse. Unmatched reads can be written in an other file, in case you would like to try to map them with another tool (may sometimes work!). |
| 187 | 190 |