BBMAP paired-end alignment problem

Mark · 03-01-2018, 06:45 PM

Hi All

I'm having a problem with aligning Illumina PE reads with BBMap version 35.92.

Execution of

Code:

bbmap.sh overwrite=t ref=Z.fasta in=R1_001_val_1.100.fq in2=R2_001_val_2.100.fq minid=0.25 mappedonly=true out=out.sam  outu=unaligned_reads.fa maxindel=100000

yields out.sam which contains only alignments of read1 even though the log info seems to suggest read2 reads were also aligned

Code:

Pairing data:           pct reads       num reads       pct bases          num bases

mated pairs:            100.0000%             100       107.4763%              59558
bad pairs:                0.0000%               0         0.0000%                  0
insert size avg:          412.82


Read 1 data:            pct reads       num reads       pct bases          num bases

mapped:                 100.0000%             100       100.0000%              29779
unambiguous:            100.0000%             100       100.0000%              29779
ambiguous:                0.0000%               0         0.0000%                  0
low-Q discards:           0.0000%               0         0.0000%                  0

perfect best site:        0.0000%               0         0.0000%                  0
semiperfect site:        35.0000%              35        35.1758%              10475
rescued:                  0.0000%               0

Match Rate:                   NA               NA        88.8176%              26449
Error Rate:              65.0000%              65         4.4763%               1333
Sub Rate:                65.0000%              65         0.3627%                108
Del Rate:                 0.0000%               0         0.0000%                  0
Ins Rate:                49.0000%              49         4.1136%               1225
N Rate:                 100.0000%             100         6.7061%               1997


Read 2 data:            pct reads       num reads       pct bases          num bases

mapped:                 100.0000%             100       100.0000%              25636
unambiguous:            100.0000%             100       100.0000%              25636
ambiguous:                0.0000%               0         0.0000%                  0
low-Q discards:           0.0000%               0         0.0000%                  0

perfect best site:        0.0000%               0         0.0000%                  0
semiperfect site:        26.0000%              26        25.3745%               6505
rescued:                  2.0000%               2

Match Rate:                   NA               NA        86.8232%              22258
Error Rate:              74.0000%              74         4.9852%               1278
Sub Rate:                74.0000%              74         0.8894%                228
Del Rate:                 0.0000%               0         0.0000%                  0
Ins Rate:                42.0000%              42         4.0958%               1050
N Rate:                 100.0000%             100         8.1916%               2100

As a test I then tried

Code:

bbmap.sh overwrite=t ref=Z.fasta in=R2_001_val_2.100.fq minid=0.25 mappedonly=true out=out.sam  outu=unaligned_reads.fa maxindel=100000

Here read2 reads were aligned.

Any ideas what is wrong with the first command line for the paired-end reads?

Thanks

Mark

GenoMax · 03-02-2018, 09:30 AM

Cross-posted and answered on Biostars:https://www.biostars.org/p/301541/

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03-02-2018, 09:30 AM	#2
GenoMax Senior Member Location: East Coast USA Join Date: Feb 2008 Posts: 7,082	Cross-posted and answered on Biostars:https://www.biostars.org/p/301541/