Mercurial > repos > xuebing > sharplabtool
view tools/fastq/fastq_combiner.py @ 0:9071e359b9a3
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author | xuebing |
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date | Fri, 09 Mar 2012 19:37:19 -0500 |
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#Dan Blankenberg import sys, os, shutil from galaxy_utils.sequence.fastq import fastqWriter, fastqSequencingRead, fastqCombiner, fastqFakeFastaScoreReader from galaxy_utils.sequence.fasta import fastaReader, fastaNamedReader def main(): #Read command line arguments fasta_filename = sys.argv[1] fasta_type = sys.argv[2] or 'fasta' #should always be fasta or csfasta? what if txt? qual_filename = sys.argv[3] qual_type = sys.argv[4] or 'qualsanger' #qual454 qualsolid output_filename = sys.argv[5] force_quality_encoding = sys.argv[6] if force_quality_encoding == 'None': force_quality_encoding = None format = 'sanger' if fasta_type == 'csfasta' or qual_type == 'qualsolid': format = 'cssanger' elif qual_type == 'qualsolexa': format = 'solexa' elif qual_type == 'qualillumina': format = 'illumina' out = fastqWriter( open( output_filename, 'wb' ), format = format, force_quality_encoding = force_quality_encoding ) if qual_filename == 'None': qual_input = fastqFakeFastaScoreReader( format, quality_encoding = force_quality_encoding ) else: qual_input = fastaNamedReader( open( qual_filename, 'rb' ) ) fastq_combiner = fastqCombiner( format ) i = None skip_count = 0 for i, sequence in enumerate( fastaReader( open( fasta_filename, 'rb' ) ) ): quality = qual_input.get( sequence ) if quality: fastq_read = fastq_combiner.combine( sequence, quality ) out.write( fastq_read ) else: skip_count += 1 out.close() if i is None: print "Your file contains no valid FASTA sequences." else: print qual_input.has_data() print 'Combined %s of %s sequences with quality scores (%.2f%%).' % ( i - skip_count + 1, i + 1, float( i - skip_count + 1 ) / float( i + 1 ) * 100.0 ) if __name__ == "__main__": main()