Mercurial > repos > bgruening > flye
diff flye.xml @ 2:156e0da5b917 draft
planemo upload for repository https://github.com/bgruening/galaxytools/tree/master/tools/flye commit a926a92aed3e22b14fb88af204c8450987c59743
| author | bgruening |
|---|---|
| date | Thu, 29 Nov 2018 04:34:34 -0500 |
| parents | cd256484eb1a |
| children | 1ce9b1d72ec3 |
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--- a/flye.xml Fri Sep 28 19:18:54 2018 -0400 +++ b/flye.xml Thu Nov 29 04:34:34 2018 -0500 @@ -1,4 +1,4 @@ -<tool id="flye" name="Assembly" version="2.3.5"> +<tool id="flye" name="Assembly" version="2.3.7"> <description>of long and error-prone reads</description> <macros> <import>macros.xml</import> @@ -25,7 +25,7 @@ flye $mode #for $counter, $input in enumerate($inputs): - ./input_${counter}.${input.ext} + ./input_${counter}.$ext #end for -o out_dir @@ -61,30 +61,30 @@ </outputs> <tests> <test> - <param name="inputs" ftype="fasta" value="E.coli_PacBio_40x_first_200_reads.fasta"/> + <param name="inputs" ftype="fasta" value="nanopore.fasta"/> <param name="mode" value="--pacbio-raw"/> - <param name="g" value="1m"/> - <output name="contigs" file="result1_contigs.fasta" ftype="fasta"/> - <output name="scaffolds" file="result1_scaffolds.fasta" ftype="fasta"/> - <output name="assembly_info" file="result1_assembly_info.txt" ftype="tabular"/> + <param name="g" value="10000"/> + <output name="contigs" file="result1_contigs.fasta" ftype="fasta" compare="sim_size"/> + <output name="scaffolds" file="result1_scaffolds.fasta" ftype="fasta" compare="sim_size"/> + <output name="assembly_info" file="result1_assembly_info.txt" ftype="tabular" compare="sim_size"/> <output name="assembly_graph" file="result1_assembly_graph.dot" ftype="graph_dot" compare="sim_size"/> </test> <test> - <param name="inputs" ftype="fasta" value="Loman_E.coli_MAP006-1_2D_50x_first_500_reads.fasta"/> + <param name="inputs" ftype="fasta" value="nanopore.fasta"/> <param name="mode" value="--nano-raw"/> - <param name="g" value="100000"/> - <output name="contigs" file="result2_contigs.fasta" ftype="fasta"/> - <output name="scaffolds" file="result2_scaffolds.fasta" ftype="fasta"/> - <output name="assembly_info" file="result2_assembly_info.txt" ftype="tabular"/> + <param name="g" value="10000"/> + <output name="contigs" file="result2_contigs.fasta" ftype="fasta" compare="sim_size"/> + <output name="scaffolds" file="result2_scaffolds.fasta" ftype="fasta" compare="sim_size"/> + <output name="assembly_info" file="result2_assembly_info.txt" ftype="tabular" compare="sim_size"/> <output name="assembly_graph" file="result2_assembly_graph.dot" ftype="graph_dot" compare="sim_size"/> </test> <test> - <param name="inputs" ftype="fasta" value="E.coli_PacBio_40x_first_200_reads.fasta"/> + <param name="inputs" ftype="fasta" value="nanopore.fasta"/> <param name="mode" value="--pacbio-raw"/> - <param name="g" value="1.1m"/> + <param name="g" value="10000"/> <param name="i" value="2"/> - <output name="contigs" file="result3_contigs.fasta" ftype="fasta"/> - <output name="scaffolds" file="result3_scaffolds.fasta" ftype="fasta"/> + <output name="contigs" file="result3_contigs.fasta" ftype="fasta" compare="sim_size"/> + <output name="scaffolds" file="result3_scaffolds.fasta" ftype="fasta" compare="sim_size"/> </test> </tests> <help><![CDATA[