Mercurial > repos > iuc > ruvseq
diff ruvseq.xml @ 4:3a083c78896e draft default tip
planemo upload for repository https://github.com/galaxyproject/tools-iuc/tree/master/tools/ruvseq commit 30117fce22f3771c9c0c13e70c3ad14b694de6e2
| author | iuc |
|---|---|
| date | Fri, 21 Apr 2023 14:09:17 +0000 |
| parents | d1f7fa5bb3cb |
| children |
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--- a/ruvseq.xml Fri Jul 23 22:37:45 2021 +0000 +++ b/ruvseq.xml Fri Apr 21 14:09:17 2023 +0000 @@ -1,8 +1,12 @@ <tool id="ruvseq" name="Remove Unwanted Variation" version="@TOOL_VERSION@+galaxy@WRAPPER_VERSION@"> <description>from RNA-seq data</description> + <xrefs> + <xref type="bio.tools">ruvseq</xref> + <xref type="bioconductor">ruvseq</xref> + </xrefs> <macros> <token name="@TOOL_VERSION@">1.26.0</token> - <token name="@WRAPPER_VERSION@">0</token> + <token name="@WRAPPER_VERSION@">1</token> </macros> <requirements> <requirement type="package" version="@TOOL_VERSION@">bioconductor-ruvseq</requirement> @@ -60,6 +64,10 @@ --tx2gene mapping.txt #end if #end if + +#if $ruv_ncounts == 1: + --ruv_ncounts +#end if ]]></command> <configfiles> <configfile name="sampleTable"> @@ -117,10 +125,17 @@ <param name="pdf" type="boolean" truevalue="1" falsevalue="0" checked="true" label="Visualising the analysis results" help="output an additional PDF files" /> + <param name="ruv_ncounts" type="boolean" truevalue="1" falsevalue="0" checked="false" + label="Output RUVSeq normalized count tables" + help="If this option is set to Yes, the tool will generate RUVseq normalized count files. Default: No" /> </inputs> <outputs> <collection name="unwanted_variation" type="list" label="RUVSeq covariate files on ${on_string}"> - <discover_datasets pattern="(?P<designation>.+)\.tabular" format="tabular" directory="." visible="false"/> + <discover_datasets pattern="uv_(?P<designation>.+)\.tabular" format="tabular" directory="." visible="false"/> + </collection> + <collection name="ruv_normcounts" type="list" label="RUVSeq normalized counts on ${on_string}"> + <filter>ruv_ncounts == True</filter> + <discover_datasets pattern="ruv_(?P<designation>.+)\.tabular" format="tabular" directory="." visible="false"/> </collection> <data format="pdf" name="plots" label="RUVSeq diagonstic plots on ${on_string}"> <filter>pdf == True</filter> @@ -232,6 +247,73 @@ </element> </output_collection> </test> + <!--Ensure Normalized counts files are generated --> + <test> + <repeat name="rep_factorLevel"> + <param name="factorLevel" value="Treated"/> + <param name="countsFile" value="GSM461179_treat_single.counts,GSM461180_treat_paired.counts,GSM461181_treat_paired.counts"/> + </repeat> + <repeat name="rep_factorLevel"> + <param name="factorLevel" value="Untreated"/> + <param name="countsFile" value="GSM461176_untreat_single.counts,GSM461177_untreat_paired.counts,GSM461178_untreat_paired.counts,GSM461182_untreat_single.counts"/> + </repeat> + <param name="pdf" value="true"/> + <param name="ruv_ncounts" value="true"/> + <output name="plots" file="ruvseq_diag.pdf" ftype="pdf" compare="sim_size"/> + <output_collection name="ruv_normcounts" type="list"> + <element name="norm_counts_control_method_k1"> + <assert_contents> + <has_text_matching expression="geneID\tGSM461179_treat_single.counts\tGSM461180_treat_paired.counts\t.+"/> + </assert_contents> + </element> + <element name="norm_counts_replicate_method_k1"> + <assert_contents> + <has_text_matching expression="geneID\tGSM461179_treat_single.counts\tGSM461180_treat_paired.counts\t.+"/> + </assert_contents> + </element> + <element name="norm_counts_residual_method_k1"> + <assert_contents> + <has_text_matching expression="geneID\tGSM461179_treat_single.counts\tGSM461180_treat_paired.counts\t.+"/> + </assert_contents> + </element> + </output_collection> + </test> + <!--Ensure Normalized counts are generated with sailfish files --> + <test> + <repeat name="rep_factorLevel"> + <param name="factorLevel" value="Treated"/> + <param name="countsFile" value="sailfish/sailfish_quant.sf1.tab,sailfish/sailfish_quant.sf2.tab,sailfish/sailfish_quant.sf3.tab"/> + </repeat> + <repeat name="rep_factorLevel"> + <param name="factorLevel" value="Untreated"/> + <param name="countsFile" value="sailfish/sailfish_quant.sf4.tab,sailfish/sailfish_quant.sf5.tab,sailfish/sailfish_quant.sf6.tab"/> + </repeat> + <param name="pdf" value="true"/> + <param name="tximport_selector" value="tximport"/> + <param name="txtype" value="sailfish"/> + <param name="mapping_format_selector" value="tabular"/> + <param name="tabular_file" value="tx2gene.tab"/> + <param name="min_mean_count" value="0"/> + <param name="ruv_ncounts" value="true"/> + <output name="plots" file="ruvseq_diag_sailfish.pdf" ftype="pdf" compare="sim_size"/> + <output_collection name="ruv_normcounts" type="list"> + <element name="norm_counts_control_method_k1"> + <assert_contents> + <has_text_matching expression="geneID\tsailfish_quant.sf1.tab\tsailfish_quant.sf2.tab\t.+"/> + </assert_contents> + </element> + <element name="norm_counts_replicate_method_k1"> + <assert_contents> + <has_text_matching expression="geneID\tsailfish_quant.sf1.tab\tsailfish_quant.sf2.tab\t.+"/> + </assert_contents> + </element> + <element name="norm_counts_residual_method_k1"> + <assert_contents> + <has_text_matching expression="geneID\tsailfish_quant.sf1.tab\tsailfish_quant.sf2.tab\t.+"/> + </assert_contents> + </element> + </output_collection> + </test> </tests> <help><![CDATA[ .. class:: infomark @@ -306,6 +388,9 @@ RUVSeq_ generates a tabular file for each method and each k of variation as well as a summary PDF. +RUVSeq can also generate RUVSeq normalized count tables. However, *these counts should be used only for exploration. It is important that subsequent DE analysis be done on the original counts, as removing the unwanted factors from the counts can also remove part of a factor of interest*. + + .. _RUVSeq: http://master.bioconductor.org/packages/release/bioc/html/RUVSeq.html .. _tximport: https://bioconductor.org/packages/devel/bioc/vignettes/tximport/inst/doc/tximport.html ]]></help>