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planemo upload for repository https://github.com/ebi-gene-expression-group/container-galaxy-sc-tertiary/tree/develop/tools/tertiary-analysis/scanpy commit d52bedbcef249117567014584058429525883ef7-dirty
author ebi-gxa
date Wed, 19 Feb 2020 11:48:21 -0500
parents 9e42d8795385
children 3636ec97f3af
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<?xml version="1.0" encoding="utf-8"?>
<tool id="scanpy_normalise_data" name="Scanpy NormaliseData" version="@TOOL_VERSION@+galaxy8" profile="@PROFILE@">
  <description>to make all cells having the same total expression</description>
  <macros>
    <import>scanpy_macros2.xml</import>
  </macros>
  <expand macro="requirements"/>
  <command detect_errors="exit_code"><![CDATA[
ln -s '${input_obj_file}' input.h5 &&
PYTHONIOENCODING=utf-8 scanpy-normalise-data
    --normalize-to ${scale_factor}
    --fraction ${fraction}
    --save-raw ${save_raw}
    ${log_transform}
    @INPUT_OPTS@
    @OUTPUT_OPTS@
    @EXPORT_MTX_OPTS@
]]></command>

  <inputs>
    <expand macro="input_object_params"/>
    <expand macro="output_object_params"/>
    <param name="scale_factor" argument="--normalize-to" type="float" value="1e4" min="0"
           label="Target number to normalise to" help="Aimed counts per cell after normalisation."/>
    <param name="fraction" argument="--fraction" type="float" value="1" min="0" max="1"
           label="Exclude top expressed genes until the remaining account for no greater than specified fraction of total counts"
           help="Only non-excluded genes will sum up the target number."/>
    <param name="log_transform" argument="--no-log-transform" type="boolean" truevalue="" falsevalue="--no-log-transform" checked="True"
           label="Apply log transform?" help="If enabled, will apply a log transformation following normalisation."/>
    <param name="save_raw" argument="--save-raw" type="boolean" truevalue="yes" falsevalue="no" checked="true"
           label="Save normalised data in `.raw`" help="The saved normalised data are log1p transformed."/>
    <expand macro="export_mtx_params"/>
  </inputs>

  <outputs>
    <expand macro="output_data_obj" description="Normalised data"/>
    <expand macro="export_mtx_outputs"/>
  </outputs>

  <tests>
    <test>
      <param name="input_obj_file" value="filter_genes.h5"/>
      <param name="input_format" value="anndata"/>
      <param name="output_format" value="anndata"/>
      <param name="scale_factor" value="1e4"/>
      <param name="save_raw" value="false"/>
      <output name="output_h5" file="normalise_data.h5" ftype="h5" compare="sim_size"/>
    </test>
  </tests>

  <help><![CDATA[
=============================================================
Normalise total counts per cell (`scanpy.pp.normalize_total`)
=============================================================

Normalise each cell by total counts over all genes (excluding top expressed
genes if so required), so that every cell has the same total count after
normalisation.

Similar functions are used, for example, by Seurat, Cell Ranger or SPRING.

@HELP@

@VERSION_HISTORY@
]]></help>
  <expand macro="citations"/>
</tool>