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planemo upload for repository https://github.com/bernt-matthias/mb-galaxy-tools/tree/master/tools/maxbin2 commit 8e118a4d24047e2c62912b962e854f789d6ff559-dirty
author | mbernt |
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date | Thu, 28 Jun 2018 08:49:29 -0400 |
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children | 864279a0d64b |
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<tool id="maxbin2" name="MaxBin2" version="2.2.4"> <requirements> <requirement type="package" version="2.2.4">maxbin2</requirement> </requirements> <version_command><![CDATA[run_MaxBin.pl -version | head -n 1]]></version_command> <command detect_errors="exit_code"><![CDATA[ ## generate read or abundance files #if $intype_cond.intype_select == 'rds': #for $r in $intype_cond.reads #if $r echo '$r' >> reads_list && #end if #end for #else if $intype_cond.intype_select == 'abdc': #for $a in $intype_cond.abund #if $a echo '$a' >> abund_list && #end if #end for #end if ## in case of reassembly the IBDA out and err is appended ## to differentiate this a header is added also befor the ## MaxBin2 outputs #if $intype_cond.intype_select == 'rds' and $intype_cond.reassembly != "" echo "==== MaxBin2 stdout ====" && echo "==== MaxBin2 stderr ====" 1>&2 && #end if run_MaxBin.pl -contig '$contig' -out out #if $intype_cond.intype_select == 'rds': -reads_list reads_list $intype_cond.reassembly #else if $intype_cond.intype_select == 'abdc': -abund_list abund_list #end if #if $adv_cond.adv_select == 'yes': -min_contig_length $adv_cond.min_contig_length -max_iteration $adv_cond.max_iteration -prob_threshold $adv_cond.prob_threshold $adv_cond.plotmarker -markerset $adv_cond.markerset #end if -thread \${GALAXY_SLOTS:-1} && tar -xf out.marker_of_each_bin.tar.gz ## redirect the idba out and err file content to stdout and err #if $intype_cond.intype_select == 'rds' and $intype_cond.reassembly != "" && echo "==== IDBA stdout ====" && cat out.idba.out && echo "==== IDBA stderr ====" 1>&2 && cat out.idba.err 1>&2 #end if ]]></command> <inputs> <param argument="-contig" type="data" format="fasta,fasta.gz" label="Contig file"/> <conditional name="intype_cond"> <param name="intype_select" type="select" label="Input type"> <option value="rds" selected="true">Sequencing Reads</option> <option value="abdc">Abundances</option> </param> <when value="rds"> <param name="reads" argument="-read/-read2/..." type="data" format="fasta,fastq" multiple="true" label="Reads file(s)"/> <param argument="--reassembly" type="boolean" truevalue="-reassembly" falsevalue="" checked="false" label="" help="Reassembly option is still highly experimental. To use this function, you need to feed MaxBin interleaved paired-end fastq or fasta file if you were to use this option." /> </when> <when value="abdc"> <param name="abund" argument="-abund/-abund2/..." type="data" format="tabular" multiple="true" label="Abundance file(s)"/> </when> </conditional> <conditional name="adv_cond"> <param name="adv_select" type="select" label="Advanced options"> <option value="yes">Yes</option> <option value="no" selected="true">No</option> </param> <when value="no"/> <when value="yes"> <param argument="-min_contig_length" type="integer" min="0" value="1000" label="minimum contig length" /> <param argument="-max_iteration" type="integer" min="0" value="50" label="Maximum Expectation-Maximization algorithm iteration number" /> <param argument="-prob_threshold" type="float" min="0" max="1.0" value="0.9" label="Probability threshold for EM final classification" /> <param name="plotmarker" type="boolean" truevalue="-plotmarker" falsevalue="" checked="false" label="Generate visualization of the marker gene presence numbers" /> <param argument="-markerset" type="select" label="Marker gene set"> <option value="107" selected="true">107 marker genes present in >95% of bacteria</option> <option value="40">40 marker gene sets that are universal among bacteria and archaea</option> </param> </when> </conditional> </inputs> <outputs> <collection name="bins" type="list" label="${tool.name} on ${on_string} (bins)"> <discover_datasets pattern="out.(?P<designation>[0-9]+).fasta" format="fasta" visible="false" /> </collection> <data name="summary" format="tabular" label="${tool.name} on ${on_string} (summary)" from_work_dir="out.summary"/> <data name="log" format="txt" label="${tool.name} on ${on_string} (log)" from_work_dir="out.log"/> <data name="abundout" format="tabular" label="${tool.name} on ${on_string} (abundances)" from_work_dir="out.abund1"> <filter>intype_cond['intype_select']=='rds'</filter> </data> <data name="marker" format="tabular" label="${tool.name} on ${on_string} (marker gene presence)" from_work_dir="out.marker"/> <data name="plot" format="pdf" label="${tool.name} on ${on_string} (marker gene presence plot)" from_work_dir="out.marker.pdf"> <filter>adv_cond['adv_select']=='yes' and adv_cond['plotmarker']</filter> </data> <data name="noclass" format="fasta" label="${tool.name} on ${on_string} (unclassified sequences)" from_work_dir="out.noclass"/> <data name="toshort" format="fasta" label="${tool.name} on ${on_string} (to short sequences)" from_work_dir="out.tooshort"/> <collection name="markers" type="list" label="${tool.name} on ${on_string} (markers prediced for bins)"> <discover_datasets pattern="out.(?P<designation>[0-9]+).marker.fasta" format="fasta" visible="false" /> </collection> <!-- additional output in case of reassembly --> <collection name="reassembly_bins" type="list" label="${tool.name} on ${on_string} (reassembly bins)"> <discover_datasets directory="out.reassem" pattern="out.(?P<designation>[0-9]+).fasta" format="fasta" visible="false" /> <filter>intype_cond['intype_select']=='rds' and intype_cond['reassembly']!=""</filter> </collection> <collection name="reassembly_reads" type="list" label="${tool.name} on ${on_string} (reassembly reads)"> <discover_datasets directory="out.reassem" pattern="out.reads.(?P<designation>[0-9]+)" format="fasta" visible="false" /> <filter>intype_cond['intype_select']=='rds' and intype_cond['reassembly']!=""</filter> </collection> <data name="reassembly_noclass" format="fasta" label="${tool.name} on ${on_string} (reassembly unclassified sequences)" from_work_dir="out.reassem/out.reads.noclass"> <filter>intype_cond['intype_select']=='rds' and intype_cond['reassembly']!=""</filter> </data> <data name="reassembly_n50" format="text" label="${tool.name} on ${on_string} (reassembly N50)" from_work_dir="out.reassem/N50.txt"> <filter>intype_cond['intype_select']=='rds' and intype_cond['reassembly']!=""</filter> </data> </outputs> <tests> <test><!-- test w contigs and reads as input --> <param name="contig" value="Bin_Sample3_contigs.fasta" ftype="fasta" /> <conditional name="intype_cond"> <param name="intype_select" value="rds"/> <param name="reads" value="interleavedPE_unmapped_Sample3_total.fasta" ftype="fasta"/> </conditional> <conditional name="adv_cond"> <param name="adv_select" value="no"/> </conditional> <output_collection name="bins" type="list" count="2"> <element name="001" file="1/out.001.fasta" ftype="fasta"/> <element name="002" file="1/out.002.fasta" ftype="fasta"/> </output_collection> <output name="summary" file="1/out.summary" ftype="tabular" /> <output name="log" file="1/out.log" ftype="txt" compare="diff" lines_diff="17" /> <output name="abundout" file="1/out.abund1" ftype="tabular" /> <output name="marker" file="1/out.marker" ftype="tabular" /> <output name="noclass" file="1/out.noclass" ftype="fasta" /> <output name="toshort" file="1/out.tooshort" ftype="fasta" /> <output_collection name="markers" type="list" count="1"> <element name="001" file="1/out.001.marker.fasta" ftype="fasta"/> </output_collection> </test> <test><!--test w contigs and abundances as input + advanced options --> <param name="contig" value="Bin_Sample3_contigs.fasta" ftype="fasta" /> <conditional name="intype_cond"> <param name="intype_select" value="abdc"/> <param name="abund" value="abundances.tsv" ftype="tabular"/> </conditional> <conditional name="adv_cond"> <param name="adv_select" value="yes"/> <param name="min_contig_length" value="500"/> <param name="max_iteration" value="10"/> <param name="prob_threshold" value="0.95"/> <param name="plotmarker" value="-plotmarker"/> <param name="markerset" value="107"/> </conditional> <output_collection name="bins" type="list" count="2"> <element name="001" file="2/out.001.fasta" ftype="fasta"/> <element name="002" file="2/out.002.fasta" ftype="fasta"/> </output_collection> <output name="summary" file="2/out.summary" ftype="tabular" /> <output name="log" file="2/out.log" ftype="txt" compare="diff" lines_diff="17" /> <output name="marker" file="2/out.marker" ftype="tabular" /> <output name="plot" file="2/out.marker.pdf" ftype="pdf" compare="sim_size" /> <output name="noclass" file="2/out.noclass" ftype="fasta" /> <output name="toshort" file="2/out.tooshort" ftype="fasta" /> <output_collection name="markers" type="list" count="1"> <element name="001" file="2/out.001.marker.fasta" ftype="fasta"/> </output_collection> </test> <test><!-- test w contigs and reads as input + reassembly--> <param name="contig" value="Bin_Sample3_contigs.fasta" ftype="fasta" /> <conditional name="intype_cond"> <param name="intype_select" value="rds"/> <param name="reads" value="interleavedPE_unmapped_Sample3_total.fasta" ftype="fasta"/> <param name="reassembly" value="-reassembly"/> </conditional> <conditional name="adv_cond"> <param name="adv_select" value="no"/> </conditional> <output_collection name="bins" type="list" count="2"> <element name="001" file="3/out.001.fasta" ftype="fasta"/> <element name="002" file="3/out.002.fasta" ftype="fasta"/> </output_collection> <output name="summary" file="3/out.summary" ftype="tabular" /> <output name="log" file="3/out.log" ftype="txt" compare="diff" lines_diff="17" /> <output name="abundout" file="3/out.abund1" ftype="tabular" /> <output name="marker" file="3/out.marker" ftype="tabular" /> <output name="noclass" file="3/out.noclass" ftype="fasta" /> <output name="toshort" file="3/out.tooshort" ftype="fasta" /> <output_collection name="markers" type="list" count="1"> <element name="001" file="3/out.001.marker.fasta" ftype="fasta"/> </output_collection> <output_collection name="reassembly_bins" type="list" count="2"> <element name="001" file="3/out.reassem/out.001.fasta" ftype="fasta"/> <element name="002" file="3/out.reassem/out.002.fasta" ftype="fasta"/> </output_collection> <output_collection name="reassembly_reads" type="list" count="2"> <element name="001" file="3/out.reassem/out.reads.001" ftype="fasta"/> <element name="002" file="3/out.reassem/out.reads.002" ftype="fasta"/> </output_collection> <output name="reassembly_noclass" file="3/out.reassem/out.reads.noclass" ftype="fasta" /> <output name="reassembly_n50" file="3/out.reassem/N50.txt" ftype="text" /> </test> </tests> <help><![CDATA[ MaxBin is a software that clusters metagenomic contigs into different bins, each consists (hopefully) of contigs from one species. MaxBin uses the nucleotide composition information and contig abundance information to do achieve binning through an Expectation-Maximization algorithm. **Input**: MaxBin need the contigs and contig abundance information. The contig abundance information can be provided in two ways: the user can choose to provide - the abundance file or - the sequencing reads in fasta format (and MaxBin will use Bowtie2 to map the sequencing reads against the contigs and generate the abundance information) The abundance information can be provided as tabular file: For example, assume I have three contigs named A0001, A0002, and A0003, then my abundance file will look like A0001 30.89 A0002 20.02 A0003 78.93 Reads/Abundundance files can be given in multiple files. By default MaxBin will look for 107 marker genes present in >95% of bacteria. Alternatively you can also choose 40 marker gene sets that are universal among bacteria and archaea (Wu et al., PLoS ONE 2013). This option may be better suited for environment dominated by archaea; however it tend to split genomes into more bins. You can choose between different marker gene sets and see which one works better. **Outputs** - bins: binned sequences - summary: a summary file describing which contigs are being classified into which bin. - log: a log file recording the core steps of MaxBin algorithm - abundances (only if reads are used as input): a summary file describing which contigs are being classified into which bin - marker: marker gene presence numbers for each bin. This table is ready to be plotted by R or other 3rd-party software. - marker plot (anly present if selected in the advanced options): visualization of the marker gene presence numbers using R. Will only appear if -plotmarker is specified. - unclassified sequences: this file stores all sequences that pass the minimum length threshold but are not classified successfully. - to short sequences: this file stores all sequences that do not meet the minimum length threshold. - markers prediced for bins: these data sets store all markers predicted from the individual bins. **Reassembly** This is an experimental feature of MaxBin. It calls for each read bin IDBA_UD with the pre_correction parameter. Of course this IDBA_UD call can be done also with the corresponding Galaxy tool ]]></help> <citations> <citation type="doi">10.1093/bioinformatics/btv638</citation> <citation type="bibtex"> @misc{renameTODO, author = {LastTODO, FirstTODO}, year = {TODO}, title = {TODO}, url = {https://downloads.jbei.org/data/microbial_communities/MaxBin/MaxBin.html}, }</citation> </citations> </tool>