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planemo upload for repository https://github.com/galaxyproject/tools-iuc/tree/master/tools/DIMet commit b74312f0a6cb28e204f8633453e493fa0b2c89d8
author | iuc |
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date | Tue, 21 May 2024 13:45:48 +0000 |
parents | 1df18470e3d0 |
children | db1e58e44a5c |
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<tool id="dimet_@EXECUTABLE@" name="dimet @TOOL_LABEL@" version="@TOOL_VERSION@+galaxy@VERSION_SUFFIX@" profile="20.05"> <description> Figures of metabolites total abundance as barplots (by DIMet) </description> <macros> <token name="@TOOL_LABEL@">abundance plot</token> <token name="@EXECUTABLE@">abundance_plot</token> <import>macros.xml</import> </macros> <expand macro="requirements"/> <command detect_errors="exit_code"><![CDATA[ @INIT_CONFIG@ @INIT_ABUNDANCE_PLOT@ @INIT_ABUNDANCE_PLOT_CONDITIONS@ @INIT_TIMEPOINTS@ @INIT_ENRICHMENT_METABOLITES@ HYDRA_FULL_ERROR=1 python -m dimet -cp '$__new_file_path__/config' '++hydra.run.dir=abundance_plot' '++figure_path=figures' '++table_path=tables' '++analysis={ metabolites:${metabolites}, dataset:{ _target_:dimet.data.DatasetConfig, name: "Galaxy DIMet run" }, method:{ _target_: dimet.method.AbundancePlotConfig, label: abundance_plot, name: "Generate abundance plots", barcolor: '${output_options.bar_color}', axisx: ${axisx}, axisx_labeltilt: '${output_options.axisx_labeltilt}', height_each_subfig: '${output_options.height_each_subfig}', palette:${output_options.palette}, as_grid:${output_options.as_grid}, x_text_modify_as:null, do_stripplot:${output_options.do_stripplot}, figure_format:${output_options.figure_format} }, label: abundance_plot, width_each_subfig: '${output_options.width_each_subfig}' }' '++analysis.dataset.label=' '++analysis.timepoints=${timepoints}' '++analysis.dataset.subfolder=' '++analysis.dataset.conditions=${conditions}' #if $metadata_path: '++analysis.dataset.metadata=metadata' #end if #if $abundance_file: '++analysis.dataset.abundances=abundance' #end if @REMOVE_CONFIG@ ]]></command> <inputs> <expand macro="input_parameters_abundance"/> <expand macro="plot_abundance_factor_list"/> <expand macro="timepoint"/> <expand macro="compartments_abundance"/> <expand macro="abundance_metabolites_list"/> <section name="output_options" title="Output options"> <expand macro="palette"/> <param name="figure_format" type="select" value="pdf" display="radio" label="Select output figure format" help="Please enter at max 1 format"> <option value="pdf">Pdf</option> <option value="svg">Svg</option> </param> <param name="bar_color" type="select" value="timepoint" display="radio" label="Select output figure barcolor" help="Please enter at max 1 format"> <option value="timepoint">timepoint</option> <option value="condition">condition</option> </param> <param name="axisx_labeltilt" type="integer" min="0" max="180" value="70" label="X axis label tilt" help="Default value is 70."/> <param name="width_each_subfig" type="float" min="1.0" max="15.0" value="3.0" label="width of subfig plots" help="Default value is 3."/> <param name="height_each_subfig" type="float" min="1.0" max="15.0" value="5.5" label="height of subfig plots" help="Default value is 5.5"/> <param name="as_grid" type="boolean" value="false" label="plot as grid" help="Default value is false."/> <param name="do_stripplot" type="boolean" value="false" label="add strip plot on abundance bar" help="Default value is false."/> </section> </inputs> <outputs> <collection name="report" type="list"> <discover_datasets pattern="__designation_and_ext__" directory="figures"/> </collection> </outputs> <tests> <test> <param name="abundance_file" ftype="tabular" value="AbundanceCorrected.csv"/> <param name="metadata_path" ftype="tabular" value="example1_metadata.csv"/> <repeat name="plot_abundance_factor_list"> <param name="condition" value="sgLDHA"/> </repeat> <param name="timepoint" value='T0,T24'/> <param name="compartments" value='endo'/> <param name="metabolites_list" value="Fru1P"/> <section name="output_options"> <param name="axisx_labeltilt" value="70"/> <param name="bar_color" value="timepoint"/> <param name="axisx" value="condition"/> <param name="palette" value="pastel"/> <param name="width_each_subfig" value="3.0"/> <param name="height_each_subfig" value="5.5"/> <param name="as_grid" value="false"/> <param name="do_stripplot" value="false"/> <param name="figure_format" value="svg"/> </section> <output_collection name="report" type="list" count="2"> <element file="bars_endo_Fru1P-total_abundance.svg" name="bars_endo_Fru1P-total_abundance" ftype="svg" compare="sim_size" delta="100"/> <element file="legend.svg" name="legend" ftype="svg" compare="sim_size" delta="100"/> </output_collection> </test> </tests> <help><![CDATA[ This module is part of DIMet: Differential analysis of Isotope-labeled targeted Metabolomics data (https://pypi.org/project/DIMet/). DIMet total abundances plot performs comparative bars for visualization of the total abundances of each metabolite across the different conditions present in your data and all/selected time points. All (or selected) metabolites are processed automatically. The figures in .pdf format are of publication quality, and as they are vectorial images you can open them and customize aesthetics with a professional image software such as Inkscape, Adobe Illustrator, Sketch, CorelDRAW, etc. **Input data files** For running DIMet @EXECUTABLE@ you need the following .csv files : - The total **abundances** file, and - The metadata file, a unique file with the description of the samples. This file is compulsory (see section **Metadata File Information**). The total abundances file must be organized as a matrix: - The first column must contain Metabolite IDs that are unique (not repeated) within the file. - The rest of the columns correspond to the samples - The rows correspond to the metabolites - The values must be tab separated, with the first row containing the sample/column labels. Example - Metabolites **abundances**: =============== ================== ================== ================== ================== ================== ================== ID **MCF001089_TD01** **MCF001089_TD02** **MCF001089_TD03** **MCF001089_TD04** **MCF001089_TD05** **MCF001089_TD06** =============== ================== ================== ================== ================== ================== ================== 2_3-PG 8698823.9926 10718737.7217 10724373.9 8536484.5 22060650 28898956 2-OHGLu 36924336 424336 92060650 45165 84951950 965165051 Glc6P 2310 2142 2683 1683 012532068 1252172 Gly3P 399298 991656565 525195 6365231 89451625 4952651963 IsoCit 0 0 0 84915613 856236 954651610 =============== ================== ================== ================== ================== ================== ================== **Metadata File Information** Provide a tab-separated file that has the names of the samples in the first column and one header row. Column names must be exactly in this order: name_to_plot condition timepoint timenum compartment original_name Example **Metadata File**: ==================== =============== ============= ============ ================ ================= **name_to_plot** **condition** **timepoint** **timenum** **compartment** **original_name** -------------------- --------------- ------------- ------------ ---------------- ----------------- Control_cell_T0-1 Control T0 0 cell MCF001089_TD01 Control_cell_T0-2 Control T0 0 cell MCF001089_TD02 Control_cell_T0-3 Control T0 0 cell MCF001089_TD03 Tumoral_cell_T0-1 Tumoral T0 0 cell MCF001089_TD04 Tumoral_cell_T0-2 Tumoral T0 0 cell MCF001089_TD05 Tumoral_cell_T0-3 Tumoral T0 0 cell MCF001089_TD06 Tumoral_cell_T24-1 Tumoral T24 24 cell MCF001089_TD07 Tumoral_cell_T24-2 Tumoral T24 24 cell MCF001089_TD08 Tumoral_cell_T24-3 Tumoral T24 24 cell MCF001090_TD01 Control_med_T24-1 Control T24 24 med MCF001090_TD02 Control_med_T24-2 Control T24 24 med MCF001090_TD03 Tumoral_med_T24-1 Tumoral T24 24 med MCF001090_TD04 Tumoral_med_T24-2 Tumoral T24 24 med MCF001090_TD05 Control_med_T0-1 Control T0 0 med MCF001090_TD06 Tumoral_med_T0-1 Tumoral T0 0 med MCF001090_TD07 Tumoral_med_T0-2 Tumoral T0 0 med MCF001090_TD08 ==================== =============== ============= ============ ================ ================= The column **original_name** must have the names of the samples as given in your data. The column **name_to_plot** must have the names as you want them to be (or set identical to original_name if you prefer). To set names that are meaningful is a better choice, as we will take them to display the results. The column **timenum** must contain only the numeric part of the timepoint, for example 2,0, 10, 100 (this means, without letters ("T", "t", "s", "h" etc) nor any other symbol). Make sure these time numbers are in the same units (but do not write the units here!). The column **compartment** is an abbreviation, coined by you, for the compartments. This will be used for the results' files names: the longer the compartments names are, the longer the output files' names! Please pick short and clear abbreviations to fill this column. **Running the analysis** You can precise how you want your analysis to be executed, with the parameters: - **conditions** : the conditions present in your data, exactly in the ORDER you want them to appear both in the x axis and in the legend. - **timepoints** : the selected (you can select all) time points, that will be shown in the x axis. - **width_each_subfig** : the desired width (in inches) for the the individual metabolites' figures There exist hints on use that will guide you, next to the parameters. The output consists of bar-plot figures, one by each metabolite, and one legend .pdf file, common to all the produced figures. **Available data for testing** You can test our tool with the data from our manuscript https://zenodo.org/record/10579862 (the pertinent files for you are located in the subfolders inside the data folder). You can also use the minimal data examples from https://zenodo.org/record/10579891 ]]> </help> <expand macro="citations"/> </tool>