skesa: skesa.xml comparison

comparison skesa.xml @ 14:1581b4e8d993 draft

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author	estrain
date	Thu, 16 Aug 2018 14:11:34 -0400
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children	06d5e64a0586

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+<tool id="skesa" name="skesa" version="0.1">
+<requirements>
+<requirement type="package" version="2.2">skesa</requirement>
+</requirements>
+<command detect_errors="exit_code"><![CDATA[
+#if $jobtype.select != "cl"
+	skesa
+#if $jobtype.select == "srr"
+-sra_run $srrnum
+#else if $jobtype.select == "asm"
+--fasta $draft
+#else if $jobtype.select == "se"
+--fastq $fastq1
+#else if $jobtype.select == "pe"
+	--fastq $fastq1,$fastq2 --use_paired_ends
+#else if $jobtype.select == "rp"
+	--fastq $pairedf.forward,$pairedf.reverse --use_paired_ends
+#end if
+#if $cores != 0
+--cores $cores
+#end if
+--memory $memory	> results.skesa.fasta
+#end if
+]]></command>
+<inputs>
+<conditional name="jobtype">
+<when value="srr">
+<param name="srrnum" type="text" label="Sra run number"/>
+</when>
+<param name="select" type="select" label="Assembly or FASTQ Reads?">
+<option value="sra">SRR  number</option>
+<option value="asm">Genome Assembly</option>
+<option value="se">Single-End Reads</option>
+<option value="pe">Paired-End Reads (Separate Files)</option>
+<option value="rp">Paired-End Reads (Paired Data Set)</option>
+<option value="cl">Collection of Reads</option>
+</param>
+<when value="asm">
+<param name="draft" type="data" format="fasta" label="FASTA" />
+</when>
+<when value="se">
+<param name="fastq1" type="data" format="fastq" label="FASTQ" />
+</when>
+<when value="pe">
+<param name="fastq1" type="data" format="fastq" label="FASTQ" />
+<param name="fastq2" type="data" format="fastq" label="FASTQ" />
+</when>
+<when value="cl">
+<param type="data_collection" name="collection_files" format="fastq" collection_type="list" label="FASTQS: Must be a Data Set list built from multiple fastq files" />
+</when>
+<when value="rp">
+<param type="data_collection" collection_type="paired" name="pairedf" format="fastq" label="FASTQS: Must be a paired set of forward and reverse fastq files" />
+</when>
+</conditional>
+<param name="memory" type="integer" label="Memory available (GB) [integer]" value="16" />
+<param name="cores" type="integer" label="Number of cores to use (default all) [integer]" value="0" />
+<param name="kmer" type="integer" label="Minimal kmer length for assembly [default 21] if non are specified " value="0" />
+<param name="min_count" type="integer" label="Minimal count for kmers retained for comparing alternate choices [integer]" value="0" />
+</inputs>
+<outputs>
+<data format="fasta" label="skesa Results" name="${input.name}.skesa.fasta" from_work_dir="*.fasta"/>
+</outputs>
+<help><![CDATA[
+**Usage: skesa**
+**INPUT**
+A fasta assembly or single or paired end reads test or data set list of fastqs
+**Memory available**
+--memory arg (=32)         Memory available (GB) [integer]
+**Number of cores**
+--cores arg (=0)           Number of cores to use (default all) [integer]
+https://github.com/ncbi/ngs-tools/tree/master/tools/skesa/
+]]></help>
+<citations>
+<citation type="bibtex">
+@misc{pope_dashnow_zobel_holt_raven_schultz_inouye_tomita_2014,
+title={skesa: eSKESA is a de-novo sequence read assembler for cultured single isolate genomes
+based on DeBruijn graphs. It uses conservative heuristics and is designed to
+create breaks at repeat regions in the genome. This leads to excellent sequence
+quality but not necessarily a large N50 statistic. It is a multi-threaded
+application that scales well with the number of processors. For different runs
+with the same inputs, including the order of reads, the order and orientation
+of contigs in the output is deterministic. },
+url={https://github.com/ncbi/ngs-tools/tree/master/tools/skesa/},
+author={National Center for Biotechnology Information },
+}</citation>
+</citations>
+</tool>

Mercurial > repos > cstrittmatter > skesa

comparison skesa.xml @ 14:1581b4e8d993 draft