diff tools/fastq/fastq_paired_unpaired.py @ 0:72e9fcaec61f

Migrated tool version 0.0.4 from old tool shed archive to new tool shed repository
author peterjc
date Tue, 07 Jun 2011 17:21:17 -0400
parents
children 7ed81e36fc1c
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--- /dev/null	Thu Jan 01 00:00:00 1970 +0000
+++ b/tools/fastq/fastq_paired_unpaired.py	Tue Jun 07 17:21:17 2011 -0400
@@ -0,0 +1,212 @@
+#!/usr/bin/env python
+"""Divides a FASTQ into paired and single (orphan reads) as separate files.
+
+The input file should be a valid FASTQ file which has been sorted so that
+any partner forward+reverse reads are consecutive. The output files all
+preserve this sort order. Pairing are recognised based on standard name
+suffices. See below or run the tool with no arguments for more details.
+
+Note that the FASTQ variant is unimportant (Sanger, Solexa, Illumina, or even
+Color Space should all work equally well).
+
+This script is copyright 2010 by Peter Cock, SCRI, UK. All rights reserved.
+See accompanying text file for licence details (MIT/BSD style).
+
+This is version 0.0.4 of the script.
+"""
+import os
+import sys
+import re
+from galaxy_utils.sequence.fastq import fastqReader, fastqWriter
+
+def stop_err(msg, err=1):
+   sys.stderr.write(msg.rstrip() + "\n")
+   sys.exit(err)
+
+msg = """Expect either 3 or 4 arguments, all FASTQ filenames.
+
+If you want two output files, use four arguments:
+ - FASTQ variant (e.g. sanger, solexa, illumina or cssanger)
+ - Sorted input FASTQ filename,
+ - Output paired FASTQ filename (forward then reverse interleaved),
+ - Output singles FASTQ filename (orphan reads)
+
+If you want three output files, use five arguments:
+ - FASTQ variant (e.g. sanger, solexa, illumina or cssanger)
+ - Sorted input FASTQ filename,
+ - Output forward paired FASTQ filename,
+ - Output reverse paired FASTQ filename,
+ - Output singles FASTQ filename (orphan reads)
+
+The input file should be a valid FASTQ file which has been sorted so that
+any partner forward+reverse reads are consecutive. The output files all
+preserve this sort order.
+
+Any reads where the forward/reverse naming suffix used is not recognised
+are treated as orphan reads. The tool supports the /1 and /2 convention
+used by Illumina, the .f and .r convention, and the Sanger convention
+(see http://staden.sourceforge.net/manual/pregap4_unix_50.html for details).
+
+Note that this does support multiple forward and reverse reads per template
+(which is quite common with Sanger sequencing), e.g. this which is sorted
+alphabetically:
+
+WTSI_1055_4p17.p1kapIBF
+WTSI_1055_4p17.p1kpIBF
+WTSI_1055_4p17.q1kapIBR
+WTSI_1055_4p17.q1kpIBR
+
+or this where the reads already come in pairs:
+
+WTSI_1055_4p17.p1kapIBF
+WTSI_1055_4p17.q1kapIBR
+WTSI_1055_4p17.p1kpIBF
+WTSI_1055_4p17.q1kpIBR
+
+both become:
+
+WTSI_1055_4p17.p1kapIBF paired with WTSI_1055_4p17.q1kapIBR
+WTSI_1055_4p17.p1kpIBF paired with WTSI_1055_4p17.q1kpIBR
+"""
+
+if len(sys.argv) == 5:
+    format, input_fastq, pairs_fastq, singles_fastq = sys.argv[1:]
+elif len(sys.argv) == 6:
+    pairs_fastq = None
+    format, input_fastq, pairs_f_fastq, pairs_r_fastq, singles_fastq = sys.argv[1:]
+else:
+    stop_err(msg)
+
+format = format.replace("fastq", "").lower()
+if not format:
+    format="sanger" #safe default
+elif format not in ["sanger","solexa","illumina","cssanger"]:
+    stop_err("Unrecognised format %s" % format)
+
+def f_match(name):
+   if name.endswith("/1") or name.endswith(".f"):
+      return True
+
+#Cope with three widely used suffix naming convensions,
+#Illumina: /1 or /2
+#Forward/revered: .f or .r
+#Sanger, e.g. .p1k and .q1k
+#See http://staden.sourceforge.net/manual/pregap4_unix_50.html
+re_f = re.compile(r"(/1|\.f|\.[sfp]\d\w*)$")
+re_r = re.compile(r"(/2|\.r|\.[rq]\d\w*)$")
+
+#assert re_f.match("demo/1")
+assert re_f.search("demo.f")
+assert re_f.search("demo.s1")
+assert re_f.search("demo.f1k")
+assert re_f.search("demo.p1")
+assert re_f.search("demo.p1k")
+assert re_f.search("demo.p1lk")
+assert re_r.search("demo/2")
+assert re_r.search("demo.r")
+assert re_r.search("demo.q1")
+assert re_r.search("demo.q1lk")
+assert not re_r.search("demo/1")
+assert not re_r.search("demo.f")
+assert not re_r.search("demo.p")
+assert not re_f.search("demo/2")
+assert not re_f.search("demo.r")
+assert not re_f.search("demo.q")
+
+count, forward, reverse, neither, pairs, singles = 0, 0, 0, 0, 0, 0
+in_handle = open(input_fastq)
+if pairs_fastq:
+    pairs_f_writer = fastqWriter(open(pairs_fastq, "w"), format)
+    pairs_r_writer = pairs_f_writer
+else:
+    pairs_f_writer = fastqWriter(open(pairs_f_fastq, "w"), format)
+    pairs_r_writer = fastqWriter(open(pairs_r_fastq, "w"), format)
+singles_writer = fastqWriter(open(singles_fastq, "w"), format)
+last_template, buffered_reads = None, []
+
+for record in fastqReader(in_handle, format):
+    count += 1
+    name = record.identifier.split(None,1)[0]
+    assert name[0]=="@", record.identifier #Quirk of the Galaxy parser
+    suffix = re_f.search(name)
+    if suffix:
+        #============
+        #Forward read
+        #============
+        template = name[:suffix.start()]
+        #print name, "forward", template
+        forward += 1
+        if last_template == template:
+            buffered_reads.append(record)
+        else:
+            #Any old buffered reads are orphans
+            for old in buffered_reads:
+                singles_writer.write(old)
+                singles += 1
+            #Save this read in buffer
+            buffered_reads = [record]
+            last_template = template  
+    else:
+        suffix = re_r.search(name)
+        if suffix:
+            #============
+            #Reverse read
+            #============
+            template = name[:suffix.start()]
+            #print name, "reverse", template
+            reverse += 1
+            if last_template == template and buffered_reads:
+                #We have a pair!
+                #If there are multiple buffered forward reads, want to pick
+                #the first one (although we could try and do something more
+                #clever looking at the suffix to match them up...)
+                old = buffered_reads.pop(0)
+                pairs_f_writer.write(old)
+                pairs_r_writer.write(record)
+                pairs += 2
+            else:
+                #As this is a reverse read, this and any buffered read(s) are
+                #all orphans
+                for old in buffered_reads:
+                    singles_writer.write(old)
+                    singles += 1
+                buffered_reads = []
+                singles_writer.write(record)
+                singles += 1
+                last_template = None
+        else:
+            #===========================
+            #Neither forward nor reverse
+            #===========================
+            singles_writer.write(record)
+            singles += 1
+            neither += 1
+            for old in buffered_reads:
+                singles_writer.write(old)
+                singles += 1
+            buffered_reads = []
+            last_template = None
+if last_template:
+    #Left over singles...
+    for old in buffered_reads:
+        singles_writer.write(old)
+        singles += 1
+in_handle.close
+singles_writer.close()
+if pairs_fastq:
+    pairs_f_writer.close()
+    assert pairs_r_writer.file.closed
+else:
+    pairs_f_writer.close()
+    pairs_r_writer.close()
+
+if neither:
+    print "%i reads (%i forward, %i reverse, %i neither), %i in pairs, %i as singles" \
+           % (count, forward, reverse, neither, pairs, singles)
+else:
+    print "%i reads (%i forward, %i reverse), %i in pairs, %i as singles" \
+           % (count, forward, reverse, pairs, singles)
+
+assert count == pairs + singles == forward + reverse + neither, \
+       "%i vs %i+%i=%i vs %i+%i=%i" \
+       % (count,pairs,singles,pairs+singles,forward,reverse,neither,forward+reverse+neither)