Mercurial > repos > devteam > fastq_paired_end_deinterlacer
view fastq_paired_end_deinterlacer.xml @ 0:e6e6498bf63c draft
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author | devteam |
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date | Thu, 23 Jan 2014 12:31:29 -0500 |
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children | 64fa25e9b916 |
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<tool id="fastq_paired_end_deinterlacer" name="FASTQ de-interlacer" version="1.1"> <description>on paired end reads</description> <requirements> <requirement type="package" version="1.0.0">galaxy_sequence_utils</requirement> </requirements> <command interpreter="python">fastq_paired_end_deinterlacer.py '$input_file' '${input_file.extension[len( 'fastq' ):]}' '$output1_pairs_file' '$output2_pairs_file' '$output1_singles_file' '$output2_singles_file'</command> <inputs> <param name="input_file" type="data" format="fastqsanger,fastqcssanger" label="FASTQ reads" /> </inputs> <outputs> <data name="output1_pairs_file" format="input" label="FASTQ de-interlacer left mates from data ${input_file.hid}" /> <data name="output2_pairs_file" format="input" label="FASTQ de-interlacer right mates from data ${input_file.hid}"/> <data name="output1_singles_file" format="input" label="FASTQ de-interlacer left singles from data ${input_file.hid}"/> <data name="output2_singles_file" format="input" label="FASTQ de-interlacer right singles from data ${input_file.hid}"/> </outputs> <tests> <test> <param name="input_file" value="paired_end_merged.fastqsanger" ftype="fastqsanger" /> <output name="output1_pairs_file" file="paired_end_1.fastqsanger" /> <output name="output2_pairs_file" file="paired_end_2.fastqsanger" /> <output name="output1_singles_file" file="paired_end_1_singles.fastqsanger" /> <output name="output2_singles_file" file="paired_end_2_singles.fastqsanger" /> </test> <test> <param name="input_file" value="paired_end_merged_errors.fastqsanger" ftype="fastqsanger" /> <output name="output1_pairs_file" file="paired_end_1_cleaned.fastqsanger" /> <output name="output2_pairs_file" file="paired_end_2_cleaned.fastqsanger" /> <output name="output1_singles_file" file="paired_end_1_cleaned_singles.fastqsanger" /> <output name="output2_singles_file" file="paired_end_2_cleaned_singles.fastqsanger" /> </test> </tests> <help> **What it does** De-interlaces a single fastq dataset representing paired-end run into two fastq datasets containing only the first or second mate read. Reads without mate are saved in separate output files. Sequence identifiers for paired-end reads must follow the /1 and /2 convention. ----- **Input** A multiple-fastq file containing paired-end reads, for example:: @1539:931/1 ACTTCCCGCGCGTGAAGGCGCCGGCAAACGAGGCTCGGGAAGGGGCTCCCG +1539:931/1 BBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBB @1539:931/2 CGCCATTCCGAATCGTAGTTGTCGGCGTCTTCCAGTGCGGCAAGGCATCGT +1539:931/2 WNUUZ\P^`BBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBB ----- **Output** Multi-fastq file with left-hand mate only:: @1539:931/1 ACTTCCCGCGCGTGAAGGCGCCGGCAAACGAGGCTCGGGAAGGGGCTCCCG +1539:931/1 BBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBB Multi-fastq file with right-hand mate only:: @1539:931/2 CGCCATTCCGAATCGTAGTTGTCGGCGTCTTCCAGTGCGGCAAGGCATCGT +1539:931/2 WNUUZ\P^`BBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBB </help> </tool>