Job ID = 2007673


sra ファイルのダウンロード中...

Read layout: PAIRED


fastq に変換中...

2019-07-05T07:17:16 fasterq-dump.2.9.6 err: index.c get_nearest_offset() -> too many rounds pos = 24 of 40
2019-07-05T07:17:16 fasterq-dump.2.9.6 err: index.c get_nearest_offset() -> too many rounds pos = 24 of 40
spots read      : 17,719
reads read      : 35,438
reads written   : 35,438
rm: cannot remove ‘[DSE]RR*’: No such file or directory

fastq に変換しました。


bowtie でマッピング中...

Time loading reference: 00:00:00
Time loading forward index: 00:00:00
Time loading mirror index: 00:00:00
Multiseed full-index search: 00:00:00
17719 reads; of these:
  17719 (100.00%) were paired; of these:
    2434 (13.74%) aligned concordantly 0 times
    14215 (80.22%) aligned concordantly exactly 1 time
    1070 (6.04%) aligned concordantly >1 times
    ----
    2434 pairs aligned concordantly 0 times; of these:
      1158 (47.58%) aligned discordantly 1 time
    ----
    1276 pairs aligned 0 times concordantly or discordantly; of these:
      2552 mates make up the pairs; of these:
        2050 (80.33%) aligned 0 times
        300 (11.76%) aligned exactly 1 time
        202 (7.92%) aligned >1 times
94.22% overall alignment rate
Time searching: 00:00:00
Overall time: 00:00:00

マッピングが完了しました。


samtools でBAM に変換中...

[samopen] SAM header is present: 17 sequences.
[bam_rmdup_core] processing reference chrI...
[bam_rmdup_core] processing reference chrII...
[bam_rmdup_core] processing reference chrIII...
[bam_rmdup_core] processing reference chrIV...
[bam_rmdup_core] processing reference chrIX...
[bam_rmdup_core] processing reference chrM...
[bam_rmdup_core] processing reference chrV...
[bam_rmdup_core] processing reference chrVI...
[bam_rmdup_core] processing reference chrVII...
[bam_rmdup_core] processing reference chrVIII...
[bam_rmdup_core] processing reference chrX...
[bam_rmdup_core] processing reference chrXI...
[bam_rmdup_core] processing reference chrXII...
[bam_rmdup_core] processing reference chrXIII...
[bam_rmdup_core] processing reference chrXIV...
[bam_rmdup_core] processing reference chrXV...
[bam_rmdup_core] processing reference chrXVI...
[bam_rmdup_core] 27 / 16305 = 0.0017 in library '	'

BAM に変換しました。


Bed ファイルを作成中...


BedGraph に変換中...

INFO  @ Fri, 05 Jul 2019 16:17:33: 
# Command line: callpeak -t /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.bam -f BAM -g 12100000 -n /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.05 -q 1e-05
# ARGUMENTS LIST:
# name = /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.05
# format = BAM
# ChIP-seq file = ['/home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.bam']
# control file = None
# effective genome size = 1.21e+07
# 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  @ Fri, 05 Jul 2019 16:17:33: #1 read tag files... 
INFO  @ Fri, 05 Jul 2019 16:17:33: #1 read treatment tags... 

BedGraph に変換しました。


BigWig に変換中...

INFO  @ Fri, 05 Jul 2019 16:17:33: #1 tag size is determined as 25 bps 
INFO  @ Fri, 05 Jul 2019 16:17:33: #1 tag size = 25 
INFO  @ Fri, 05 Jul 2019 16:17:33: #1  total tags in treatment: 15259 
INFO  @ Fri, 05 Jul 2019 16:17:33: #1 user defined the maximum tags... 
INFO  @ Fri, 05 Jul 2019 16:17:33: #1 filter out redundant tags at the same location and the same strand by allowing at most 1 tag(s) 
INFO  @ Fri, 05 Jul 2019 16:17:33: #1  tags after filtering in treatment: 15249 
INFO  @ Fri, 05 Jul 2019 16:17:33: #1  Redundant rate of treatment: 0.00 
INFO  @ Fri, 05 Jul 2019 16:17:33: #1 finished! 
INFO  @ Fri, 05 Jul 2019 16:17:33: #2 Build Peak Model... 
INFO  @ Fri, 05 Jul 2019 16:17:33: #2 looking for paired plus/minus strand peaks... 
INFO  @ Fri, 05 Jul 2019 16:17:33: #2 number of paired peaks: 362 
WARNING @ Fri, 05 Jul 2019 16:17:33: Fewer paired peaks (362) than 1000! Model may not be build well! Lower your MFOLD parameter may erase this warning. Now I will use 362 pairs to build model! 
INFO  @ Fri, 05 Jul 2019 16:17:33: start model_add_line... 
INFO  @ Fri, 05 Jul 2019 16:17:33: start X-correlation... 
INFO  @ Fri, 05 Jul 2019 16:17:33: end of X-cor 
INFO  @ Fri, 05 Jul 2019 16:17:33: #2 finished! 
INFO  @ Fri, 05 Jul 2019 16:17:33: #2 predicted fragment length is 302 bps 
INFO  @ Fri, 05 Jul 2019 16:17:33: #2 alternative fragment length(s) may be 61,225,254,270,302 bps 
INFO  @ Fri, 05 Jul 2019 16:17:33: #2.2 Generate R script for model : /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.05_model.r 
INFO  @ Fri, 05 Jul 2019 16:17:33: #3 Call peaks... 
INFO  @ Fri, 05 Jul 2019 16:17:33: #3 Pre-compute pvalue-qvalue table... 
INFO  @ Fri, 05 Jul 2019 16:17:33: #3 Call peaks for each chromosome... 

BigWig に変換しました。

INFO  @ Fri, 05 Jul 2019 16:17:33: #4 Write output xls file... /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.05_peaks.xls 
INFO  @ Fri, 05 Jul 2019 16:17:33: #4 Write peak in narrowPeak format file... /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.05_peaks.narrowPeak 
INFO  @ Fri, 05 Jul 2019 16:17:33: #4 Write summits bed file... /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.05_summits.bed 
INFO  @ Fri, 05 Jul 2019 16:17:33: Done! 
pass1 - making usageList (0 chroms): 411 millis
needLargeMem: trying to allocate 0 bytes (limit: 17179869184)
INFO  @ Fri, 05 Jul 2019 16:17:34: 
# Command line: callpeak -t /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.bam -f BAM -g 12100000 -n /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.10 -q 1e-10
# ARGUMENTS LIST:
# name = /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.10
# format = BAM
# ChIP-seq file = ['/home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.bam']
# control file = None
# effective genome size = 1.21e+07
# 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
 
INFO  @ Fri, 05 Jul 2019 16:17:34: #1 read tag files... 
INFO  @ Fri, 05 Jul 2019 16:17:34: #1 read treatment tags... 
INFO  @ Fri, 05 Jul 2019 16:17:34: #1 tag size is determined as 25 bps 
INFO  @ Fri, 05 Jul 2019 16:17:34: #1 tag size = 25 
INFO  @ Fri, 05 Jul 2019 16:17:34: #1  total tags in treatment: 15259 
INFO  @ Fri, 05 Jul 2019 16:17:34: #1 user defined the maximum tags... 
INFO  @ Fri, 05 Jul 2019 16:17:34: #1 filter out redundant tags at the same location and the same strand by allowing at most 1 tag(s) 
INFO  @ Fri, 05 Jul 2019 16:17:34: #1  tags after filtering in treatment: 15249 
INFO  @ Fri, 05 Jul 2019 16:17:34: #1  Redundant rate of treatment: 0.00 
INFO  @ Fri, 05 Jul 2019 16:17:34: #1 finished! 
INFO  @ Fri, 05 Jul 2019 16:17:34: #2 Build Peak Model... 
INFO  @ Fri, 05 Jul 2019 16:17:34: #2 looking for paired plus/minus strand peaks... 
INFO  @ Fri, 05 Jul 2019 16:17:34: #2 number of paired peaks: 362 
WARNING @ Fri, 05 Jul 2019 16:17:34: Fewer paired peaks (362) than 1000! Model may not be build well! Lower your MFOLD parameter may erase this warning. Now I will use 362 pairs to build model! 
INFO  @ Fri, 05 Jul 2019 16:17:34: start model_add_line... 
INFO  @ Fri, 05 Jul 2019 16:17:34: start X-correlation... 
INFO  @ Fri, 05 Jul 2019 16:17:34: end of X-cor 
INFO  @ Fri, 05 Jul 2019 16:17:34: #2 finished! 
INFO  @ Fri, 05 Jul 2019 16:17:34: #2 predicted fragment length is 302 bps 
INFO  @ Fri, 05 Jul 2019 16:17:34: #2 alternative fragment length(s) may be 61,225,254,270,302 bps 
INFO  @ Fri, 05 Jul 2019 16:17:34: #2.2 Generate R script for model : /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.10_model.r 
INFO  @ Fri, 05 Jul 2019 16:17:34: #3 Call peaks... 
INFO  @ Fri, 05 Jul 2019 16:17:34: #3 Pre-compute pvalue-qvalue table... 
INFO  @ Fri, 05 Jul 2019 16:17:34: #3 Call peaks for each chromosome... 
INFO  @ Fri, 05 Jul 2019 16:17:34: #4 Write output xls file... /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.10_peaks.xls 
INFO  @ Fri, 05 Jul 2019 16:17:34: #4 Write peak in narrowPeak format file... /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.10_peaks.narrowPeak 
INFO  @ Fri, 05 Jul 2019 16:17:34: #4 Write summits bed file... /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.10_summits.bed 
INFO  @ Fri, 05 Jul 2019 16:17:34: Done! 
CompletedMACS2peakCalling
INFO  @ Fri, 05 Jul 2019 16:17:35: 
# Command line: callpeak -t /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.bam -f BAM -g 12100000 -n /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.20 -q 1e-20
# ARGUMENTS LIST:
# name = /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.20
# format = BAM
# ChIP-seq file = ['/home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.bam']
# control file = None
# effective genome size = 1.21e+07
# 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  @ Fri, 05 Jul 2019 16:17:35: #1 read tag files... 
INFO  @ Fri, 05 Jul 2019 16:17:35: #1 read treatment tags... 
pass1 - making usageList (0 chroms): 425 millis
needLargeMem: trying to allocate 0 bytes (limit: 17179869184)
INFO  @ Fri, 05 Jul 2019 16:17:35: #1 tag size is determined as 25 bps 
INFO  @ Fri, 05 Jul 2019 16:17:35: #1 tag size = 25 
INFO  @ Fri, 05 Jul 2019 16:17:35: #1  total tags in treatment: 15259 
INFO  @ Fri, 05 Jul 2019 16:17:35: #1 user defined the maximum tags... 
INFO  @ Fri, 05 Jul 2019 16:17:35: #1 filter out redundant tags at the same location and the same strand by allowing at most 1 tag(s) 
INFO  @ Fri, 05 Jul 2019 16:17:35: #1  tags after filtering in treatment: 15249 
INFO  @ Fri, 05 Jul 2019 16:17:35: #1  Redundant rate of treatment: 0.00 
INFO  @ Fri, 05 Jul 2019 16:17:35: #1 finished! 
INFO  @ Fri, 05 Jul 2019 16:17:35: #2 Build Peak Model... 
INFO  @ Fri, 05 Jul 2019 16:17:35: #2 looking for paired plus/minus strand peaks... 
INFO  @ Fri, 05 Jul 2019 16:17:35: #2 number of paired peaks: 362 
WARNING @ Fri, 05 Jul 2019 16:17:35: Fewer paired peaks (362) than 1000! Model may not be build well! Lower your MFOLD parameter may erase this warning. Now I will use 362 pairs to build model! 
INFO  @ Fri, 05 Jul 2019 16:17:35: start model_add_line... 
INFO  @ Fri, 05 Jul 2019 16:17:35: start X-correlation... 
INFO  @ Fri, 05 Jul 2019 16:17:35: end of X-cor 
INFO  @ Fri, 05 Jul 2019 16:17:35: #2 finished! 
INFO  @ Fri, 05 Jul 2019 16:17:35: #2 predicted fragment length is 302 bps 
INFO  @ Fri, 05 Jul 2019 16:17:35: #2 alternative fragment length(s) may be 61,225,254,270,302 bps 
INFO  @ Fri, 05 Jul 2019 16:17:35: #2.2 Generate R script for model : /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.20_model.r 
INFO  @ Fri, 05 Jul 2019 16:17:35: #3 Call peaks... 
INFO  @ Fri, 05 Jul 2019 16:17:35: #3 Pre-compute pvalue-qvalue table... 
CompletedMACS2peakCalling
INFO  @ Fri, 05 Jul 2019 16:17:35: #3 Call peaks for each chromosome... 
INFO  @ Fri, 05 Jul 2019 16:17:35: #4 Write output xls file... /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.20_peaks.xls 
INFO  @ Fri, 05 Jul 2019 16:17:35: #4 Write peak in narrowPeak format file... /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.20_peaks.narrowPeak 
INFO  @ Fri, 05 Jul 2019 16:17:35: #4 Write summits bed file... /home/okishinya/chipatlas/results/sacCer3/ERX433650/ERX433650.20_summits.bed 
INFO  @ Fri, 05 Jul 2019 16:17:35: Done! 
pass1 - making usageList (0 chroms): 1 millis
needLargeMem: trying to allocate 0 bytes (limit: 17179869184)
CompletedMACS2peakCalling