blat module¶
“In general the coordinates in psl files are “zero based half open.” The first base in a sequence is numbered zero rather than one. When representing a range the end coordinate is not included in the range. Thus the first 100 bases of a sequence are represented as 0-100, and the second 100 bases are represented as 100-200. There is another little unusual feature in the .psl format. It has to do with how coordinates are handled on the negative strand. In the qStart/qEnd fields the coordinates are where it matches from the point of view of the forward strand (even when the match is on the reverse strand). However on the qStarts[] list, the coordinates are reversed.” — http://wiki.bits.vib.be/index.php/Blat
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class
mavis.blat.
Blat
[source]¶ Bases:
object
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static
millibad
(row, is_protein=False, is_mrna=True)[source]¶ this function is used in calculating percent identity direct translation of the perl code # https://genome.ucsc.edu/FAQ/FAQblat.html#blat4
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static
pslx_row_to_pysam
(row, bam_cache, reference_genome)[source]¶ given a ‘row’ from reading a pslx file. converts the row to a BlatAlignedSegment object
Parameters:
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static
score
(row, is_protein=False)[source]¶ direct translation from ucsc guidelines on replicating the web blat score https://genome.ucsc.edu/FAQ/FAQblat.html#blat4
below are lines from the perl code i’ve re-written in python
my $sizeMul = pslIsProtein($blockCount, $strand, $tStart, $tEnd, $tSize, $tStarts, $blockSizes); sizmul = 1 for DNA my $pslScore = $sizeMul * ($matches + ($repMatches >> 1) ) - $sizeMul * $misMatches - $qNumInsert - $tNumIns ert)
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static
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mavis.blat.
process_blat_output
(INPUT_BAM_CACHE, query_id_mapping, reference_genome, aligner_output_file='aligner_out.temp', blat_min_percent_of_max_score=0.8, blat_min_identity=0.7, blat_limit_top_aln=25, is_protein=False, log=<function devnull>, **kwargs)[source]¶ converts the blat output pslx (unheadered file) to bam reads