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author | florianbegusch |
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date | Thu, 03 Sep 2020 10:51:34 +0000 |
parents | a0a8d77a991c |
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<?xml version="1.0" ?> <tool id="qiime_deblur_denoise-other" name="qiime deblur denoise-other" version="2020.8"> <description>Deblur sequences using a user-specified positive filter.</description> <requirements> <requirement type="package" version="2020.8">qiime2</requirement> </requirements> <command><![CDATA[ qiime deblur denoise-other --i-demultiplexed-seqs=$idemultiplexedseqs --i-reference-seqs=$ireferenceseqs --p-trim-length=$ptrimlength --p-left-trim-len=$plefttrimlen #if $psamplestats: --p-sample-stats #end if --p-mean-error=$pmeanerror --p-indel-prob=$pindelprob --p-indel-max=$pindelmax --p-min-reads=$pminreads --p-min-size=$pminsize --p-jobs-to-start=$pjobstostart #if $pnohashedfeatureids: --p-no-hashed-feature-ids #end if --o-table=otable --o-representative-sequences=orepresentativesequences --o-stats=ostats #if str($examples) != 'None': --examples=$examples #end if ; cp ostats.qza $ostats ]]></command> <inputs> <param format="qza,no_unzip.zip" label="--i-demultiplexed-seqs: ARTIFACT SampleData[SequencesWithQuality | PairedEndSequencesWithQuality | JoinedSequencesWithQuality] The demultiplexed sequences to be denoised. [required]" name="idemultiplexedseqs" optional="False" type="data" /> <param format="qza,no_unzip.zip" label="--i-reference-seqs: ARTIFACT FeatureData[Sequence] Positive filtering database. Keep all sequences aligning to these sequences. [required]" name="ireferenceseqs" optional="False" type="data" /> <param label="--p-trim-length: INTEGER Sequence trim length, specify -1 to disable trimming. [required]" name="ptrimlength" optional="False" type="text" /> <param label="--p-left-trim-len: INTEGER Range(0, None) Sequence trimming from the 5\' end. A value of 0 will disable this trim. [default: 0]" min="0" name="plefttrimlen" optional="True" type="integer" value="0" /> <param label="--p-sample-stats: --p-sample-stats: / --p-no-sample-stats If true, gather stats per sample. [default: False]" name="psamplestats" selected="False" type="boolean" /> <param label="--p-mean-error: NUMBER The mean per nucleotide error, used for original sequence estimate. [default: 0.005]" name="pmeanerror" optional="True" type="float" value="0.005" /> <param label="--p-indel-prob: NUMBER Insertion/deletion (indel) probability (same for N indels). [default: 0.01]" name="pindelprob" optional="True" type="float" value="0.01" /> <param label="--p-indel-max: INTEGER Maximum number of insertion/deletions. [default: 3]" name="pindelmax" optional="True" type="integer" value="3" /> <param label="--p-min-reads: INTEGER Retain only features appearing at least min-reads times across all samples in the resulting feature table. [default: 10]" name="pminreads" optional="True" type="integer" value="10" /> <param label="--p-min-size: INTEGER In each sample, discard all features with an abundance less than min-size. [default: 2]" name="pminsize" optional="True" type="integer" value="2" /> <param label="--p-no-hashed-feature-ids: Do not if true, hash the feature IDs. [default: True]" name="pnohashedfeatureids" selected="False" type="boolean" /> <param label="--examples: Show usage examples and exit." name="examples" optional="False" type="data" /> </inputs> <outputs> <data format="qza" label="${tool.name} on ${on_string}: table.qza" name="otable" /> <data format="qza" label="${tool.name} on ${on_string}: representativesequences.qza" name="orepresentativesequences" /> <data format="qza" label="${tool.name} on ${on_string}: stats.qza" name="ostats" /> </outputs> <help><![CDATA[ Deblur sequences using a user-specified positive filter. ############################################################### Perform sequence quality control for Illumina data using the Deblur workflow, including positive alignment-based filtering. Only forward reads are supported at this time. This mode of execution is particularly useful when operating on non-16S data. For example, to apply Deblur to 18S data, you would want to specify a reference composed of 18S sequences in order to filter out sequences which do not appear to be 18S. The assessment is performed by local alignment using SortMeRNA with a permissive e-value threshold. Parameters ---------- demultiplexed_seqs : SampleData[SequencesWithQuality | PairedEndSequencesWithQuality | JoinedSequencesWithQuality] The demultiplexed sequences to be denoised. reference_seqs : FeatureData[Sequence] Positive filtering database. Keep all sequences aligning to these sequences. trim_length : Int Sequence trim length, specify -1 to disable trimming. left_trim_len : Int % Range(0, None), optional Sequence trimming from the 5' end. A value of 0 will disable this trim. sample_stats : Bool, optional If true, gather stats per sample. mean_error : Float, optional The mean per nucleotide error, used for original sequence estimate. indel_prob : Float, optional Insertion/deletion (indel) probability (same for N indels). indel_max : Int, optional Maximum number of insertion/deletions. min_reads : Int, optional Retain only features appearing at least min_reads times across all samples in the resulting feature table. min_size : Int, optional In each sample, discard all features with an abundance less than min_size. jobs_to_start : Int, optional Number of jobs to start (if to run in parallel). hashed_feature_ids : Bool, optional If true, hash the feature IDs. Returns ------- table : FeatureTable[Frequency] The resulting denoised feature table. representative_sequences : FeatureData[Sequence] The resulting feature sequences. stats : DeblurStats Per-sample stats if requested. ]]></help> <macros> <import>qiime_citation.xml</import> </macros> <expand macro="qiime_citation"/> </tool>