Job ID = 9158425


sra ファイルのダウンロード中...

Completed: 2019632K bytes transferred in 21 seconds
 (763451K bits/sec), in 2 files, 3 directories.

sra ファイルのダウンロードが完了しました。

Read layout: PAIRED


fastq に変換中...

Written 20071109 spots for /home/okishinya/chipatlas/results/dm3/SRX128173/SRR442094.sra
Written 20071109 spots total
Written 20558936 spots for /home/okishinya/chipatlas/results/dm3/SRX128173/SRR443912.sra
Written 20558936 spots total
rm: cannot remove `[DSE]RR*.fastq': そのようなファイルやディレクトリはありません

fastq に変換しました。


bowtie でマッピング中...

Warning: Could not open read file "SRX128173_2.fq" for reading; skipping...
Error: No input read files were valid
(ERR): bowtie2-align exited with value 1

マッピングが完了しました。


samtools でBAM に変換中...

[samopen] no @SQ lines in the header.
[sam_read1] missing header? Abort!
[bam_header_read] EOF marker is absent. The input is probably truncated.
awk: コマンドライン:1: (FILENAME=- FNR=1) 致命的: ゼロによる除算が試みられました
awk: コマンドライン:1: (FILENAME=- FNR=1) 致命的: ゼロによる除算が試みられました
awk: コマンドライン:1: (FILENAME=- FNR=1) 致命的: ゼロによる除算が試みられました

BAM に変換しました。


Bed ファイルを作成中...


BedGraph に変換中...


*****ERROR: Unrecognized parameter: SRX128173.bam *****


Tool:    bedtools genomecov (aka genomeCoverageBed)
Version: v2.17.0
Summary: Compute the coverage of a feature file among a genome.

Usage: bedtools genomecov [OPTIONS] -i <bed/gff/vcf> -g <genome>

Options: 
	-ibam		The input file is in BAM format.
			Note: BAM _must_ be sorted by position

	-d		Report the depth at each genome position (with one-based coordinates).
			Default behavior is to report a histogram.

	-dz		Report the depth at each genome position (with zero-based coordinates).
			Reports only non-zero positions.
			Default behavior is to report a histogram.

	-bg		Report depth in BedGraph format. For details, see:
			genome.ucsc.edu/goldenPath/help/bedgraph.html

	-bga		Report depth in BedGraph format, as above (-bg).
			However with this option, regions with zero 
			coverage are also reported. This allows one to
			quickly extract all regions of a genome with 0 
			coverage by applying: "grep -w 0$" to the output.

	-split		Treat "split" BAM or BED12 entries as distinct BED intervals.
			when computing coverage.
			For BAM files, this uses the CIGAR "N" and "D" operations 
			to infer the blocks for computing coverage.
			For BED12 files, this uses the BlockCount, BlockStarts, and BlockEnds
			fields (i.e., columns 10,11,12).

	-strand		Calculate coverage of intervals from a specific strand.
			With BED files, requires at least 6 columns (strand is column 6). 
			- (STRING): can be + or -

	-5		Calculate coverage of 5" positions (instead of entire interval).

	-3		Calculate coverage of 3" positions (instead of entire interval).

	-max		Combine all positions with a depth >= max into
			a single bin in the histogram. Irrelevant
			for -d and -bedGraph
			- (INTEGER)

	-scale		Scale the coverage by a constant factor.
			Each coverage value is multiplied by this factor before being reported.
			Useful for normalizing coverage by, e.g., reads per million (RPM).
			- Default is 1.0; i.e., unscaled.
			- (FLOAT)

	-trackline	Adds a UCSC/Genome-Browser track line definition in the first line of the output.
			- See here for more details about track line definition:
			      http://genome.ucsc.edu/goldenPath/help/bedgraph.html
			- NOTE: When adding a trackline definition, the output BedGraph can be easily
			      uploaded to the Genome Browser as a custom track,
			      BUT CAN NOT be converted into a BigWig file (w/o removing the first line).

	-trackopts	Writes additional track line definition parameters in the first line.
			- Example:
			   -trackopts 'name="My Track" visibility=2 color=255,30,30'
			   Note the use of single-quotes if you have spaces in your parameters.
			- (TEXT)

Notes: 
	(1) The genome file should tab delimited and structured as follows:
	 <chromName><TAB><chromSize>

	For example, Human (hg19):
	chr1	249250621
	chr2	243199373
	...
	chr18_gl000207_random	4262

	(2) The input BED (-i) file must be grouped by chromosome.
	 A simple "sort -k 1,1 <BED> > <BED>.sorted" will suffice.

	(3) The input BAM (-ibam) file must be sorted by position.
	 A "samtools sort <BAM>" should suffice.

Tips: 
	One can use the UCSC Genome Browser's MySQL database to extract
	chromosome sizes. For example, H. sapiens:

	mysql --user=genome --host=genome-mysql.cse.ucsc.edu -A -e \
	"select chrom, size from hg19.chromInfo" > hg19.genome


BedGraph に変換しました。


BigWig に変換中...

needLargeMem: trying to allocate 0 bytes (limit: 100000000000)

BigWig に変換しました。

INFO  @ Tue, 27 Jun 2017 16:43:45: 
# Command line: callpeak -t SRX128173.bam -f BAM -g dm -n SRX128173.05 -q 1e-05
# ARGUMENTS LIST:
# name = SRX128173.05
# format = BAM
# ChIP-seq file = ['SRX128173.bam']
# control file = None
# effective genome size = 1.20e+08
# band width = 300
# model fold = [5, 50]
# qvalue cutoff = 1.00e-05
# Larger dataset will be scaled towards smaller dataset.
# Range for calculating regional lambda is: 10000 bps
# Broad region calling is off
# Paired-End mode is off
 
INFO  @ Tue, 27 Jun 2017 16:43:45: #1 read tag files... 
INFO  @ Tue, 27 Jun 2017 16:43:45: #1 read treatment tags... 
INFO  @ Tue, 27 Jun 2017 16:43:45: 
# Command line: callpeak -t SRX128173.bam -f BAM -g dm -n SRX128173.20 -q 1e-20
# ARGUMENTS LIST:
# name = SRX128173.20
# format = BAM
# ChIP-seq file = ['SRX128173.bam']
# control file = None
# effective genome size = 1.20e+08
# band width = 300
# model fold = [5, 50]
# qvalue cutoff = 1.00e-20
# Larger dataset will be scaled towards smaller dataset.
# Range for calculating regional lambda is: 10000 bps
# Broad region calling is off
# Paired-End mode is off
 
INFO  @ Tue, 27 Jun 2017 16:43:45: #1 read tag files... 
INFO  @ Tue, 27 Jun 2017 16:43:45: #1 read treatment tags... 
INFO  @ Tue, 27 Jun 2017 16:43:45: 
# Command line: callpeak -t SRX128173.bam -f BAM -g dm -n SRX128173.10 -q 1e-10
# ARGUMENTS LIST:
# name = SRX128173.10
# format = BAM
# ChIP-seq file = ['SRX128173.bam']
# control file = None
# effective genome size = 1.20e+08
# band width = 300
# model fold = [5, 50]
# qvalue cutoff = 1.00e-10
# Larger dataset will be scaled towards smaller dataset.
# Range for calculating regional lambda is: 10000 bps
# Broad region calling is off
# Paired-End mode is off
 
Exception structINFO  @ Tue, 27 Jun 2017 16:43:45: #1 read tag files... 
.error: 'unpINFO  @ Tue, 27 Jun 2017 16:43:45: #1 read treatment tags... 
ack requires a string argument of length 4' in 'MACS2.IO.Parser.BAMParser.tsize'Exception  ignored
struct.error: 'unpack reException qstruct.uerrori: r'eusn paa cskt rrieINFO  @ Tue, 27 Jun 2017 16:43:45: #1 tag size is determined as 0 bps 
nqgu iaINFO  @ Tue, 27 Jun 2017 16:43:45: #1 tag size = 0 
rrgeusm ean ts torfi nlge nagrtghu m4e'n in t' MoAfC Sl2eINFO  @ Tue, 27 Jun 2017 16:43:45: #1  total tags in treatment: 0 
n.gItOINFO  @ Tue, 27 Jun 2017 16:43:45: #1 user defined the maximum tags... 
.hP a4r's in e'rINFO  @ Tue, 27 Jun 2017 16:43:45: #1 filter out redundant tags at the same location and the same strand by allowing at most 1 tag(s) 
.MBAACMINFO  @ Tue, 27 Jun 2017 16:43:45: #1  tags after filtering in treatment: 0 
PSa2r.sIeOr..Ptasriszeer'. ignored
BTraceback (most recent call last):
A  File "/usr/local/bin/macs2", line 5, in <module>
MP    apkg_resources.run_script('MACS2==2.1.1.20160309', 'macs2')
rs  File "build/bdist.linux-x86_64/egg/pkg_resources.py", line 489, in run_script
er.tsize' ignored
  File "build/bdist.linux-x86_64/egg/pkg_resources.py", line 1214, in run_script
  File "/usr/local/lib/python2.7/site-packages/MACS2-2.1.1.20160309-py2.7-linux-x86_64.egg/EGG-INFO/scripts/macs2", line 617, in <module>
INFO  @ Tue, 27 Jun 2017 16:43:45: #1 tag size is determined as 0 bps 
INFO  @ Tue, 27 Jun 2017 16:43:45: #1 tag size = 0 
INFO  @ Tue, 27 Jun 2017 16:43:45: #1  total tags in treatment: 0 
    INFO  @ Tue, 27 Jun 2017 16:43:45: #1 user defined the maximum tags... 

  File "/usr/local/lib/python2.7/site-packages/MACS2-2.1.1.20160309-py2.7-linux-x86_64.egg/EGG-INFO/scripts/macs2", line 57, in main
INFO  @ Tue, 27 Jun 2017 16:43:45: #1 tag size is determined as 0 bps 
INFO  @ Tue, 27 Jun 2017 16:43:45: #1 filter out redundant tags at the same location and the same strand by allowing at most 1 tag(s) 
    
  File "build/bdist.linux-x86_64/egg/MACS2/callpeak_cmd.py", line 112, in run
INFO  @ Tue, 27 Jun 2017 16:43:45: #1 tag size = 0 
INFO  @ Tue, 27 Jun 2017 16:43:45: #1  tags after filtering in treatment: 0 
ZeroDivisionError: Traceback (most recent call last):
INFO  @ Tue, 27 Jun 2017 16:43:45: #1  total tags in treatment: 0 
  File "/usr/local/bin/macs2", line 5, in <module>
float division by zero    
pkg_resources.run_script('MACS2==2.1.1.20160309', 'macs2')
INFO  @ Tue, 27 Jun 2017 16:43:45: #1 user defined the maximum tags... 
  File "build/bdist.linux-x86_64/egg/pkg_resources.py", line 489, in run_script
INFO  @ Tue, 27 Jun 2017 16:43:45: #1 filter out redundant tags at the same location and the same strand by allowing at most 1 tag(s) 
  File "build/bdist.linux-x86_64/egg/pkg_resources.py", line 1214, in run_script
  File "/usr/local/lib/python2.7/site-packages/MACS2-2.1.1.20160309-py2.7-linux-x86_64.egg/EGG-INFO/scripts/macs2", line 617, in <module>
INFO  @ Tue, 27 Jun 2017 16:43:45: #1  tags after filtering in treatment: 0 
Traceback (most recent call last):
  File "/usr/local/bin/macs2", line 5, in <module>
    pkg_resources.run_script('MACS2==2.1.1.20160309', 'macs2')
  File "build/bdist.linux-x86_64/egg/pkg_resources.py", line 489, in run_script
  File "build/bdist.linux-x86_64/egg/pkg_resources.py", line 1214, in run_script
  File "/usr/local/lib/python2.7/site-packages/MACS2-2.1.1.20160309-py2.7-linux-x86_64.egg/EGG-INFO/scripts/macs2", line 617, in <module>
    
  File "/usr/local/lib/python2.7/site-packages/MACS2-2.1.1.20160309-py2.7-linux-x86_64.egg/EGG-INFO/scripts/macs2", line 57, in main
    
  File "build/bdist.linux-x86_64/egg/MACS2/callpeak_cmd.py", line 112, in run
ZeroDivisionError: float division by zero
    
  File "/usr/local/lib/python2.7/site-packages/MACS2-2.1.1.20160309-py2.7-linux-x86_64.egg/EGG-INFO/scripts/macs2", line 57, in main
    
  File "build/bdist.linux-x86_64/egg/MACS2/callpeak_cmd.py", line 112, in run
ZeroDivisionError: float division by zero
cat: SRX128173.05_peaks.narrowPeak: そのようなファイルやディレクトリはありません
cat: SRX128173.20_peaks.narrowPeak: そのようなファイルやディレクトリはありません
cat: SRX128173.10_peaks.narrowPeak: そのようなファイルやディレクトリはありません
pass1 - making usageList (0 chroms): 1 millis
needLargeMem: trying to allocate 0 bytes (limit: 17179869184)
pass1 - making usageList (0 chroms): 1 millis
pass1 - making usageList (0 chroms): 1 millis
needLargeMem: trying to allocate 0 bytes (limit: 17179869184)
needLargeMem: trying to allocate 0 bytes (limit: 17179869184)
rm: cannot remove `SRX128173.20_model.r': そのようなファイルやディレクトリはありません
rm: cannot remove `SRX128173.20_*.xls': そのようなファイルやディレクトリはありません
rm: cannot remove `SRX128173.20_peaks.narrowPeak': そのようなファイルやディレクトリはありません
rm: cannot remove `SRX128173.05_model.r': そのようなファイルやディレクトリはありません
CompletedMACS2peakCalling
rm: cannot remove `SRX128173.05_*.xls': そのようなファイルやディレクトリはありません
rm: cannot remove `SRX128173.10_model.r'rm: cannot remove `SRX128173.05_peaks.narrowPeak': そのようなファイルやディレクトリはありません
: そのようなファイルやディレクトリはありません
rm: cannot remove `SRX128173.10_*.xls': そのようなファイルやディレクトリはありません
CompletedMACS2peakCalling
rm: cannot remove `SRX128173.10_peaks.narrowPeak': そのようなファイルやディレクトリはありません
CompletedMACS2peakCalling