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chipseq_analysis
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chipseq_analysis
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3d77cb5b
Commit
3d77cb5b
authored
7 years ago
by
Venkat Malladi
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update the naming of the reads.
parent
d14969c6
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1 changed file
workflow/scripts/map_reads.py
+10
-5
10 additions, 5 deletions
workflow/scripts/map_reads.py
with
10 additions
and
5 deletions
workflow/scripts/map_reads.py
+
10
−
5
View file @
3d77cb5b
...
...
@@ -112,24 +112,27 @@ def align_se(fastq, sai, reference, fastq_basename):
'''
Use BWA to align SE data.
'''
sam_filename
=
"
%s.sam
"
%
(
fastq_basename
)
bam_filename
=
'
%s.bam
'
%
(
fastq_basename
)
steps
=
[
"
bwa samse %s %s %s
"
%
(
reference
,
fastq
[
0
],
sai
[
0
]),
"
samtools view -@%d -Su -
"
%
(
cpu_count
()),
"
samtools sort -@%d -o %s
"
%
(
cpu_count
(),
fastq_bas
ename
)]
%
(
cpu_count
(),
bam_fil
ename
)]
out
,
err
=
utils
.
run_pipe
(
steps
)
if
err
:
logger
.
error
(
"
samse/samtools error: %s
"
%
(
err
))
return
bam_filename
def
align_pe
(
fastq
,
sai
,
reference
,
fastq_basename
):
'''
Use BWA to align PE data.
'''
sam_filename
=
"
%s.sam
"
%
(
fastq_basename
)
badcigar_filename
=
"
%s.badReads
"
%
(
fastq_basename
)
bam_filename
=
'
%s.bam
'
%
(
fastq_basename
)
# Remove read pairs with bad CIGAR strings and sort by position
steps
=
[
...
...
@@ -150,12 +153,14 @@ def align_pe(fastq, sai, reference, fastq_basename):
"
grep -v -F -f %s
"
%
(
badcigar_filename
),
"
samtools view -@%d -Su -
"
%
(
cpu_count
()),
"
samtools sort -@%d -o %s
"
%
(
cpu_count
(),
fastq_bas
ename
)]
%
(
cpu_count
(),
bam_fil
ename
)]
out
,
err
=
utils
.
run_pipe
(
steps
)
if
err
:
logger
.
error
(
"
samtools error: %s
"
%
(
err
))
return
bam_filename
def
main
():
args
=
get_args
()
...
...
@@ -184,18 +189,18 @@ def main():
strip_extensions
(
fastq
[
1
],
STRIP_EXTENSIONS
))
fastq_basename
=
fastq_r1_basename
+
fastq_r2_basename
align_pe
(
fastq
,
sai
,
reference
,
fastq_basename
)
bam_filename
=
align_pe
(
fastq
,
sai
,
reference
,
fastq_basename
)
else
:
fastq_basename
=
os
.
path
.
basename
(
strip_extensions
(
fastq
[
0
],
STRIP_EXTENSIONS
))
align_se
(
fastq
,
sai
,
reference
,
fastq_basename
)
bam_filename
=
align_se
(
fastq
,
sai
,
reference
,
fastq_basename
)
bam_mapstats_filename
=
'
%s.raw.srt.bam.flagstat.qc
'
%
(
fastq_basename
)
with
open
(
bam_mapstats_filename
,
'
w
'
)
as
fh
:
subprocess
.
check_call
(
shlex
.
split
(
"
samtools flagstat %s
"
%
(
bam_
mapstats_
filename
)),
shlex
.
split
(
"
samtools flagstat %s
"
%
(
bam_filename
)),
stdout
=
fh
)
# Remove sai files
...
...
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