annotate ncbi_egapx.xml @ 16:d167f698d5e9 draft

planemo upload for repository https://github.com/richard-burhans/galaxytools/tree/main/tools/ncbi_egapx commit d5c4a9faa18df570d02ce208d301a160d8555f58
author richard-burhans
date Sat, 16 Nov 2024 14:48:29 +0000
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1 <tool id="ncbi_egapx" name="NCBI EGAPx" version="@TOOL_VERSION@+galaxy@VERSION_SUFFIX@" profile="@PROFILE@">
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2 <description>annotates eukaryotic genomes</description>
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3 <macros>
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4 <import>macros.xml</import>
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5 </macros>
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6 <expand macro="edam_ontology"/>
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7 <expand macro="requirements"/>
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8 <command detect_errors="aggressive"><![CDATA[
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9 #if str($cond_input_style.input_style) == "fillform"
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10 #set yamlconfig = $egapx_config
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11 #else
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12 #set yamlconfig = $yamlin
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13 #end if
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14 ## activate the following
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15 ## - nextflow conda environment
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16 ## - EGPAx python virtual environment
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17 source /galaxy/env.bash &&
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18 ## use the augmented container EGAPx config
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19 ln -s /galaxy/egapx/egapx_config &&
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20 ## run EGAPx
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21 python3 /galaxy/egapx/ui/egapx.py '$yamlconfig' -e galaxy -o 'egapx_out'
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22 ]]></command>
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23 <configfiles>
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24 <configfile name="egapx_config"><![CDATA[
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25 #if str($cond_input_style.input_style) == "fillform"
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26 # yaml generated by ncbi_egapx.xml
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27 #if str($cond_input_style.cond_genome_style.genome_style) == "history"
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28 #set genome_value = $cond_input_style.cond_genome_style.genome
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29 #elif str($cond_input_style.cond_genome_style.genome_style) == "indexed"
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30 #set genome_value = $cond_input_style.cond_genome_style.genome.fields.path
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31 #else
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32 #set genome_value = $cond_input_style.cond_genome_style.uri
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33 #end if
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34 genome: $genome_value
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35 taxid: $taxid
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36 #if str($cond_rnaseq_style.rnaseq_style) == "list"
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37 #set $reads_values = $rnaseq.split()
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38 #else
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39 #set $reads_values = $rnaseq
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40 #end if
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41 reads:
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42 #for r in [x.strip() for x in $reads_values]
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43 - $r
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44 #end for
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45 #if str($proteins) != "None"
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46 proteins: $proteins
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47 #end if
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48 #for row in $xtra.strip().split("\n")
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49 $row
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50 #end for
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51 #end if
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52 ]]></configfile>
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53 </configfiles>
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54 <inputs>
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55 <conditional name="cond_input_style">
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56 <param name="input_style" type="select" label="Fill in a tool form or use an existing yaml configuration from the current history?"
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57 help="Use the tool form to select inputs from the history, or use a pre-prepared yaml file.">
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58 <option value="fillform" selected="True">Provide configuration details for conversion into a configuration yaml</option>
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59 <option value="history">Use a pre-prepared yaml egapx configuration</option>
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60 </param>
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61 <when value="fillform">
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62 <conditional name="cond_genome_style">
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63 <param name="genome_style" type="select" label="Reference genome source for mapping supplied RNA-seq reads"
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64 help="Select a built in, history or remote URI for the reference genome FASTA">
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65 <option value="history" selected="True">Use a genome FASTA file from the current history</option>
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66 <option value="indexed">Use a Galaxy server built-in genome</option>
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67 <option value="uri">Provide a remote web link URI ("https://...") pointing at the required genome reference FASTA file</option>
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68 </param>
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69 <when value="history">
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70 <param name="genome" type="data" format="fasta" label="Select the reference genome FASTA from the current history"/>
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71 </when>
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72 <when value="indexed">
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73 <param name="genome" type="select" label="Select a built in reference genome or custom genome"
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74 help="If not listed, add a custom genome or use a reference genome from the history">
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75 <options from_data_table="all_fasta">
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76 <validator message="No genomes are available " type="no_options"/>
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77 </options>
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78 </param>
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79 </when>
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80 <when value="uri">
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81 <param name="uri" type="text" label="URI pointing to the reference genome FASTA file"/>
9
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82 </when>
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83 </conditional>
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84
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85 <param name="taxid" type="text" label="NCBI Taxon ID" help="Used to identify the HMM model files needed">
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86 <validator type="regex" message="Numeric">^[0-9]+$</validator>
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87 </param>
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88
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89 <conditional name="cond_rnaseq_style">
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90 <param name="rnaseq_style" type="select" label="RNA sequence data source"
9
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91 help="Select RNAseq input data from history or input a list of SRA identifiers or remote URI">
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92 <option value="history" selected="True">Select one or more RNA-seq fastq datasets from the current history</option>
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93 <option value="list">Type in a list of SRA identifiers and/or remote RNA-seq FASTA URI</option>
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94 </param>
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95 <when value="history">
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96 <param name="rnaseq" type="data" format="fastqsanger,fastqsanger.gz" multiple="true" label="Select multiple RNA-seq fastqsanger inputs from the current history"
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97 help="All selected rna-seq fastqsanger will be added to the yaml for egapx configuration"/>
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98 </when>
9
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99 <when value="list">
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100 <param name="rnaseq" type="text" area="true" label="List all required individual RNA-seq URI or SRA identifiers, separated by spaces or newlines"
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101 help="Either a working URI for a RNA-seq FASTA, or a bare SRA identifier will work - can be mixed">
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102 <validator type="empty_field"/>
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103 </param>
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104 </when>
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105 </conditional>
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106 <param name="proteins" type="data" format="fasta,fasta.gz" optional="true" label="Select a protein set"/>
9
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107 <param name="xtra" type="text" area="true" label="Additional yaml to append to the egapx.yaml configuration"
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108 help="Not normally needed but useful for testing additional configuration elements">
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109 <sanitizer invalid_char="">
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110 <valid initial="string.printable"/>
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111 </sanitizer>
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112 </param>
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113 </when>
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114 <when value="history">
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115 <param name="yamlin" type="data" format="yaml" label="egapx configuration yaml file to pass to Nextflow"/>
3
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116 </when>
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117 </conditional>
0
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118 </inputs>
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119 <outputs>
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120 <data name="output" format="gff" label="EGAPx annotation for ${on_string}" from_work_dir="egapx_out/accept.gff"/>
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121 <collection name="nextflow_stats" type="list" label="EGAPx nextflow stats for ${on_string}">
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122 <data name="nf_log" format="txt" label="Nextflow execution log" from_work_dir="egapx_out/nextflow.log"/>
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123 <data name="nf_report" format="html" label="Nextflow execution report" from_work_dir="egapx_out/run.report.html"/>
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124 <data name="nf_trace" format="tabular" label="Nextflow trace file" from_work_dir="egapx_out/run.trace.txt"/>
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125 <data name="nf_timeline" format="html" label="Nextflow execution timeline" from_work_dir="egapx_out/run.timeline.html"/>
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126 <data name="nf_params" format="yaml" label="Nextflow run parameters" from_work_dir="egapx_out/run_params.yaml"/>
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127 </collection>
0
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128 </outputs>
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129 <tests>
9
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130 <test expect_test_failure="true">
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131 <param name="input_style" value="fillform"/>
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132 <param name="taxid" value="6954"/>
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133 <param name="genome_style" value="uri"/>
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134 <param name="uri" value="https://ftp.ncbi.nlm.nih.gov/genomes/all/GCF/020/809/275/GCF_020809275.1_ASM2080927v1/GCF_020809275.1_ASM2080927v1_genomic.fna.gz"/>
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135 <param name="rnaseq_style" value="list"/>
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136 <param name="rnaseq" value="https://ftp.ncbi.nlm.nih.gov/genomes/TOOLS/EGAP/sample_data/Dermatophagoides_farinae_small/SRR8506572.1 https://ftp.ncbi.nlm.nih.gov/genomes/TOOLS/EGAP/sample_data/Dermatophagoides_farinae_small/SRR8506572.2 https://ftp.ncbi.nlm.nih.gov/genomes/TOOLS/EGAP/sample_data/Dermatophagoides_farinae_small/SRR9005248.1 https://ftp.ncbi.nlm.nih.gov/genomes/TOOLS/EGAP/sample_data/Dermatophagoides_farinae_small/SRR9005248.2"/>
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137 <param name="xtra" value="hmm: https://ftp.ncbi.nlm.nih.gov/genomes/TOOLS/EGAP/gnomon/hmm_parameters/6956.params&#10;tasks:&#10; star_wnode:&#10; star_wnode: -cpus-per-worker 4"/>
9
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138 <output name="output"><assert_contents><has_size min="1"/></assert_contents></output>
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139 <output_collection name="nextflow_stats" type="list">
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140 <element name="nf_log"><assert_contents><has_size min="1"/></assert_contents></element>
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141 <element name="nf_report"><assert_contents><has_size min="1"/></assert_contents></element>
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142 <element name="nf_trace"><assert_contents><has_size min="1"/></assert_contents></element>
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143 <element name="nf_timeline"><assert_contents><has_size min="1"/></assert_contents></element>
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144 <element name="nf_params"><assert_contents><has_size min="1"/></assert_contents></element>
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145 </output_collection>
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146 </test>
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147 <test expect_test_failure="true">
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148 <param name="input_style" value="history"/>
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149 <param name="yamlin" value="input.yaml"/>
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150 <output name="output"><assert_contents><has_size min="1"/></assert_contents></output>
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151 <output_collection name="nextflow_stats" type="list">
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152 <element name="nf_log"><assert_contents><has_size min="1"/></assert_contents></element>
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153 <element name="nf_report"><assert_contents><has_size min="1"/></assert_contents></element>
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154 <element name="nf_trace"><assert_contents><has_size min="1"/></assert_contents></element>
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155 <element name="nf_timeline"><assert_contents><has_size min="1"/></assert_contents></element>
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156 <element name="nf_params"><assert_contents><has_size min="1"/></assert_contents></element>
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157 </output_collection>
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158 </test>
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159 </tests>
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160 <help><![CDATA[
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161 Galaxy tool wrapping the Eukaryotic Genome Annotation Pipeline (EGAPx)
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162 =================================================================================================
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163
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164 .. class:: warningmark
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165
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166 **Proof of concept: a hack to run a NF workflow inside a specialised Galaxy tool wrapper**
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167
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168 EGAPx is a big, complicated Nextflow workflow, challenging and costly to re-implement **properly**, requiring dozens of new tools and replicating a lot of
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169 complicated *groovy* workflow logic.
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170
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171 It is also very new and in rapid development. Investing developer effort and keeping updated as EGAPx changes rapidly may be *inefficient of developer resources*.
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173 This wrapper is designed to allow measuring how *inefficient* it is in terms of computing resource utilisation, in comparison to the developer effort
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174 required to convert Nextflow DDL into tools and WF logic. Balancing these competing requirements is a fundamental Galaxy challenge.
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175
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176
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177 EGAPx requires very substantial resources to run with real data. *132GB and 32 cores* are the minimum requirement; *256GB and 64 cores* are recommended.
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179 A special minimal example that can be run in 6GB with 4 cores is provided as a yaml configuration and is used for the tool test.
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180
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181 In this implementation, the user must supply a yaml configuration file as initial proof of concept.
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182 History inputs and even a yaml editor might be provided in future.
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183
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184 The NF workflow to tool model tested here may be applicable to other NF workflows that take a single configuration yaml.
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185
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186 .. class:: warningmark
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187
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188 The computational resource cost of typing the wrong SRA identifiers into a tool form is potentially enormous with this tool!
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189
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190
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191 Sample yaml configurations
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192 ===========================
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193
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194 YAML sample configurations can be uploaded into your Galaxy history from the `EGAPx github repository <https://github.com/ncbi/egapx/tree/main/examples/>`_.
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195 The simplest possible example is shown below - can be cut/paste into a history dataset in the upload tool.
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196
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197
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198 *./examples/input_D_farinae_small.yaml* is shown below and can be cut and pasted into the upload form to create a yaml file.
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199 RNA-seq data is provided as URI to the reads FASTA files.
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201 input_D_farinae_small.yaml
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203 ::
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204
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205 genome: https://ftp.ncbi.nlm.nih.gov/genomes/all/GCF/020/809/275/GCF_020809275.1_ASM2080927v1/GCF_020809275.1_ASM2080927v1_genomic.fna.gz
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206 taxid: 6954
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207 reads:
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208 - https://ftp.ncbi.nlm.nih.gov/genomes/TOOLS/EGAP/sample_data/Dermatophagoides_farinae_small/SRR8506572.1
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209 - https://ftp.ncbi.nlm.nih.gov/genomes/TOOLS/EGAP/sample_data/Dermatophagoides_farinae_small/SRR8506572.2
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210 - https://ftp.ncbi.nlm.nih.gov/genomes/TOOLS/EGAP/sample_data/Dermatophagoides_farinae_small/SRR9005248.1
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211 - https://ftp.ncbi.nlm.nih.gov/genomes/TOOLS/EGAP/sample_data/Dermatophagoides_farinae_small/SRR9005248.2
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214 input_Gavia_stellata.yaml
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216 ::
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218 genome: https://ftp.ncbi.nlm.nih.gov/genomes/all/GCF/030/936/135/GCF_030936135.1_bGavSte3.hap2/GCF_030936135.1_bGavSte3.hap2_genomic.fna.gz
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219 reads: txid37040[Organism] AND biomol_transcript[properties] NOT SRS024887[Accession]
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220 taxid: 37040
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222 input_C_longicornis.yaml
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224 ::
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226 genome: https://ftp.ncbi.nlm.nih.gov/genomes/all/GCF/029//603/195/GCF_029603195.1_ASM2960319v2/GCF_029603195.1_ASM2960319v2_genomic.fna.gz
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227 reads: txid2530218[Organism] AND biomol_transcript[properties] NOT SRS024887[Accession]
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228 taxid: 2530218
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230 Purpose
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231 ========
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233 **This is not intended for production**
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234
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235 Just a proof of concept.
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236 It is possibly too inefficient to be useful although it may turn out not to be a problem if run on a dedicated workstation.
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237 At least the efficiency can now be more easily estimated.
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239 This tool is not recommended for public deployment because of the resource demands.
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240
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241 EGAPx Overview
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242 ===============
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243
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244 .. image:: $PATH_TO_IMAGES/Pipeline_sm_ncRNA_CAGE_80pct.png
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245
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246 **Warning:**
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247 The current version is an alpha release with limited features and organism scope to collect initial feedback on execution. Outputs are not yet complete and not intended for production use. Please open a GitHub [Issue](https://github.com/ncbi/egapx/issues) if you encounter any problems with EGAPx. You can also write to cgr@nlm.nih.gov to give us your feedback or if you have any questions.
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248
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249 EGAPx is the publicly accessible version of the updated NCBI [Eukaryotic Genome Annotation Pipeline](https://www.ncbi.nlm.nih.gov/genome/annotation_euk/process/).
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250
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251 EGAPx takes an assembly FASTA file, a taxid of the organism, and RNA-seq data. Based on the taxid, EGAPx will pick protein sets and HMM models. The pipeline runs `miniprot` to align protein sequences, and `STAR` to align RNA-seq to the assembly. Protein alignments and RNA-seq read alignments are then passed to `Gnomon` for gene prediction. In the first step of `Gnomon`, the short alignments are chained together into putative gene models.
0
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252 In the second step, these predictions are further supplemented by *ab-initio* predictions based on HMM models. The final annotation for the input assembly is produced as a `gff` file.
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253
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254 **Security Notice:**
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255
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256 EGAPx has dependencies in and outside of its execution path that include several thousand files from the [NCBI C++ toolkit](https://www.ncbi.nlm.nih.gov/toolkit), and more than a million total lines of code. Static Application Security Testing has shown a small number of verified buffer overrun security vulnerabilities. Users should consult with their organizational security team on risk and if there is concern, consider mitigating options like running via VM or cloud instance.
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257
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258
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259 *To specify an array of NCBI SRA datasets in yaml*
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260
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261 ::
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262
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263 reads:
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264 - SRR8506572
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265 - SRR9005248
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266
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267
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268 *To specify an SRA entrez query*
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270 ::
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272 reads: 'txid6954[Organism] AND biomol_transcript[properties] NOT SRS024887[Accession] AND (SRR8506572[Accession] OR SRR9005248[Accession] )'
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273
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274
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275 **Note:** Both the above examples will have more RNA-seq data than the `input_D_farinae_small.yaml` example. To make sure the entrez query does not produce a large number of SRA runs, please run it first at the [NCBI SRA page](https://www.ncbi.nlm.nih.gov/sra). If there are too many SRA runs, then select a few of them and list it in the input yaml.
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276
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277 Output
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278 =======
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279
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280 EGAPx output will appear as a collection in the user history. The main annotation file is called *accept.gff*.
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282 ::
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284 accept.gff
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285 annot_builder_output
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286 nextflow.log
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287 run.report.html
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288 run.timeline.html
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289 run.trace.txt
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290 run_params.yaml
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291
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293 The *nextflow.log* is the log file that captures all the process information and their work directories. ``run_params.yaml`` has all the parameters that were used in the EGAPx run. More information about the process time and resources can be found in the other run* files.
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294
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295 ## Intermediate files
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297 In the log, each line denotes the process that completed in the workflow. The first column (_e.g._ `[96/621c4b]`) is the subdirectory where the intermediate output files and logs are found for the process in the same line, _i.e._, `egapx:miniprot:run_miniprot`. To see the intermediate files for that process, you can go to the work directory path that you had supplied and traverse to the subdirectory `96/621c4b`:
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299 ::
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301 $ aws s3 ls s3://temp_datapath/D_farinae/96/
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302 PRE 06834b76c8d7ceb8c97d2ccf75cda4/
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303 PRE 621c4ba4e6e87a4d869c696fe50034/
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304 $ aws s3 ls s3://temp_datapath/D_farinae/96/621c4ba4e6e87a4d869c696fe50034/
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305 PRE output/
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306 2024-03-27 11:19:18 0
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307 2024-03-27 11:19:28 6 .command.begin
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308 2024-03-27 11:20:24 762 .command.err
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309 2024-03-27 11:20:26 762 .command.log
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310 2024-03-27 11:20:23 0 .command.out
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311 2024-03-27 11:19:18 13103 .command.run
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312 2024-03-27 11:19:18 129 .command.sh
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313 2024-03-27 11:20:24 276 .command.trace
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314 2024-03-27 11:20:25 1 .exitcode
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315 $ aws s3 ls s3://temp_datapath/D_farinae/96/621c4ba4e6e87a4d869c696fe50034/output/
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316 2024-03-27 11:20:24 17127134 aligns.paf
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317 ]]></help>
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318 <expand macro="citations"/>
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319 <expand macro="creators"/>
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320 </tool>