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"planemo upload for repository https://github.com/quadram-institute-bioscience/galaxy-tools/tree/master/tools/seqsero2 commit 8b41cf1161ac0f0836f5597167911596b0cfa27e-dirty"
| author | thanhlv |
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| date | Fri, 12 Nov 2021 14:56:56 +0000 |
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<tool id="seqsero2" name="SeqSero2" version="@VERSION@+galaxy0"> <description> Salmonella serotype prediction</description> <macros> <token name="@VERSION@">1.2.1</token> </macros> <requirements> <requirement type="package" version="@VERSION@">seqsero2</requirement> </requirements> <version_command>SeqSero2_package.py -v</version_command> <command detect_errors="exit_code"><![CDATA[ #import re #set $seqsero_input = '' #set $seqsero_t_value = '' #if $inputs.input_type == 'paired': #if $inputs.R1.is_of_type('fastqsanger', 'fastq'): #set $ext = 'fastq' #elif $inputs.R1.is_of_type('fastqsanger.gz'): #set $ext = 'fastq.gz' #elif $inputs.R1.is_of_type('fastq'): #set $ext = 'fastq' #elif $inputs.R1.is_of_type('fastq.gz'): #set $ext = 'fastq.gz' #elif $inputs.R1.is_of_type('fasta.gz'): #set $ext = 'fasta.gz' #elif $inputs.R1.is_of_type('fasta'): #set $ext = 'fasta' #end if #set $safename_R1 = re.sub('[^\w\-_\.]', '_', $inputs.R1.element_identifier) #set $safename_R2 = re.sub('[^\w\-_\.]', '_', $inputs.R2.element_identifier) ln -fs '$inputs.R1' $safename_R1.$ext && ln -fs '$inputs.R2' $safename_R2.$ext && #set $seqsero_input = $safename_R1 + '.' + $ext + ' ' + $safename_R2 + '.' + $ext #set $seqsero_t_value = '2' #elif $inputs.input_type == 'collection': #for $input in $inputs.input_collection #if $input.forward.is_of_type('fastqsanger', 'fastq'): #set $ext = 'fastq' #elif $input.forward.is_of_type('fastqsanger.gz'): #set $ext = 'fastq.gz' #elif $input.forward.is_of_type('fastq'): #set $ext = 'fastq' #elif $input.forward.is_of_type('fastq.gz'): #set $ext = 'fastq.gz' #elif $input.forward.is_of_type('fasta.gz'): #set $ext = 'fasta.gz' #elif $input.forward.is_of_type('fasta'): #set $ext = 'fasta' #end if #set $safename_fwd = re.sub('[^\w\-_\.]', '_', $input.forward.element_identifier) ln -fs '$input.forward' $safename_fwd.$ext && #set $safename_rvs = re.sub('[^\w\-_\.]', '_', $input.reverse.element_identifier) ln -fs '$input.reverse' $safename_rvs.$ext && #set $seqsero_input = $safename_fwd+ '.' + $ext + ' ' + $safename_rvs + '.' + $ext #set $seqsero_t_value = '2' #end for #elif $inputs.input_type == 'assembly': #if $inputs.contigs.is_of_type('fasta.gz'): #set $ext = 'fasta.gz' #elif $inputs.contigs.is_of_type('fasta'): #set $ext = 'fasta' #end if #set $safename_seq = re.sub('[^\w\-_\.]', '_', $contigs.element_identifier) ln -fs '$contigs' $safename_seq.$ext && #set $seqsero_input = $safename_seq + '.' + $ext #set $seqsero_t_value = '4' #elif $inputs.input_type == 'single': #if $inputs.single.is_of_type('fastqsanger', 'fastq'): #set $ext = 'fastq' #elif $inputs.single.is_of_type('fastqsanger.gz'): #set $ext = 'fastq.gz' #elif $inputs.single.is_of_type('fastq'): #set $ext = 'fastq' #elif $inputs.single.is_of_type('fastq.gz'): #set $ext = 'fastq.gz' #elif $inputs.single.is_of_type('fasta.gz'): #set $ext = 'fasta.gz' #elif $inputs.single.is_of_type('fasta'): #set $ext = 'fasta' #end if #set $safename_seq = re.sub('[^\w\-_\.]', '_', $single.element_identifier) ln -fs '$single' $safename_seq.$ext && #set $seqsero_input = $safename_seq + '.' + $ext #set $seqsero_t_value = '3' #elif $inputs.input_type == 'nanopore': #if $inputs.nanopore.is_of_type('fastqsanger', 'fastq'): #set $ext = 'fastq' #elif $inputs.nanopore.is_of_type('fastqsanger.gz'): #set $ext = 'fastq.gz' #elif $inputs.nanopore.is_of_type('fastq'): #set $ext = 'fastq' #elif $inputs.nanopore.is_of_type('fastq.gz'): #set $ext = 'fastq.gz' #elif $inputs.nanopore.is_of_type('fasta.gz'): #set $ext = 'fasta.gz' #elif $inputs.nanopore.is_of_type('fasta'): #set $ext = 'fasta' #end if #set $safename_seq = re.sub('[^\w\-_\.]', '_', $nanopore.element_identifier) ln -fs '$nanopore' $safename_seq.$ext && #set $seqsero_input = $safename_seq + '.' + $ext #set $seqsero_t_value = '5' #end if SeqSero2_package.py -m $workflow -t $seqsero_t_value -i $seqsero_input -p \${GALAXY_SLOTS:-4} -d output ]]> </command> <inputs> <conditional name="inputs"> <param name="input_type" type="select" label="Input type" help="Select 'paired end' reads or 'sequence' for genomes/contigs"> <option value="paired">Paired End</option> <option value="collection">Collection</option> <option value="assembly">Contigs</option> <option value="single">Interleaved</option> <option value="nanopore">Nanopore reads</option> </param> <when value="paired"> <param name="R1" type="data" format="fastqsanger,fastqsanger.gz" label="Forward reads (R1)" help="The file of forward reads in FASTQ format"/> <param name="R2" type="data" format="fastqsanger,fastqsanger.gz" label="Reverse reads (R2)" help="The file of reverse reads in FASTQ format"/> </when> <when value="collection"> <param name="input_collection" format="fastqsanger" type="data_collection" collection_type="list:paired" label="Paired collection"/> </when> <when value="single"> <param name="single" type="data" format="fastqsanger,fastqsanger.gz" multiple="false" label="Interleaved" /> </when> <when value="nanopore"> <param name="nanopore" type="data" format="fastqsanger,fastqsanger.gz" multiple="false" label="Nanopore reads" /> </when> <when value="assembly"> <param name="contigs" type="data" format="fasta" multiple="false" label="Contigs/genomes" /> </when> </conditional> <param label="Workflow" type="select" name="workflow"> <option value="a">allele</option> <option value="k" selected="true">k-mer</option> </param> </inputs> <outputs> <data name="results" format="tabular" label="${tool.name} on ${on_string} Results" from_work_dir="output/SeqSero_result.tsv"/> <data name="log" format="txt" label="${tool.name} on ${on_string} Log" from_work_dir="output/SeqSero_log.txt"/> </outputs> <tests> <test> <param name="input_type" value="assembly" /> <param name="contigs" value="CP009102.1.fasta" ftype="fasta" /> <output name="results"> <assert_contents> <has_text text="Salmonella enterica subspecies enterica (subspecies I)" /> <has_text text="Typhimurium" /> </assert_contents> </output> </test> <!-- TODO: Test for fastq files --> </tests> <help><![CDATA[ **Usage: SeqSero2_package.py** -m <string> (which workflow to apply, 'a'(raw reads allele micro-assembly), 'k'(raw reads and genome assembly k-mer), default=a) -t <string> (input data type, '1' for interleaved paired-end reads, '2' for separated paired-end reads, '3' for single reads, '4' for genome assembly, '5' for nanopore reads (fasta/fastq)) -i <file> (/path/to/input/file) -p <int> (number of threads for allele mode, if p >4, only 4 threads will be used for assembly since the amount of extracted reads is small, default=1) -b <string> (algorithms for bwa mapping for allele mode; 'mem' for mem, 'sam' for samse/sampe; default=mem; optional; for now we only optimized for default "mem" mode) -d <string> (output directory name) -c <flag> (if '-c' was flagged, SeqSero2 will only output serotype prediction without the directory containing log files) -n <string> (optional, to specify a sample name in the report output) -s <flag> (if '-s' was flagged, SeqSero2 will not output header in `SeqSero_result.tsv`) --check <flag> (use '--check' flag to check the required dependencies) -v, --version (show program's version number and exit) ----- _`Document`: https://github.com/denglab/SeqSero2 ]]></help> <citations> <citation type="bibtex"> @misc{zhang_yin_jones_zhang_deathrage_dinsmore_fitzgeral_fields_deng_2015, title={Salmonella serotype determination utilizing high-throughput genome sequencing data.}, journal={J Clin Microbiol}, publisher={ASM}, author={Zhang S, Yin Y, Jones MB, Zhang Z, Deatherage Kaiser BL, Dinsmore BA, Fitzgerald C, Fields PI, Deng X.}, year={2015}, month={Max}, url={http://http://jcm.asm.org/content/early/2015/03/05/JCM.00323-15}}, }</citation> <citation type="bibtex"> @misc{cfsan_biostatistics_group_2017, title={CFSAN Biostatistics Group fork of SeqSero2}, url={https://github.com/CFSAN-Biostatistics/SeqSero2.git}}, </citation> </citations> </tool>