Seqanswers Leaderboard Ad

**Richard Finney** · 05-02-2011, 10:27 AM

use -S parameter

Usage: samtools view [options] <in.bam>|<in.sam> [region1 [...]]

Options: -b output BAM
-h print header for the SAM output
-H print header only (no alignments)
-S input is SAM
-u uncompressed BAM output (force -b)
-1 fast compression (force -b)
-x output FLAG in HEX (samtools-C specific)
-X output FLAG in string (samtools-C specific)
-c print only the count of matching records
-L FILE output alignments overlapping the input BED FILE [null]
-t FILE list of reference names and lengths (force -S) [null]
-T FILE reference sequence file (force -S) [null]
-o FILE output file name [stdout]
-R FILE list of read groups to be outputted [null]
-f INT required flag, 0 for unset [0]
-F INT filtering flag, 0 for unset [0]
-q INT minimum mapping quality [0]
-l STR only output reads in library STR [null]
-r STR only output reads in read group STR [null]
-? longer help

**emilyjia2000** · 05-02-2011, 11:08 AM

Hi Richard,

I do want to convert SAM to BAM, it output error when I used "samtools view -b in.sam -o out.bam". I checked the header of SAM file, it comes with @PG. I don't know how to deal with it?

Thanks

**kmcarr** · 05-03-2011, 05:24 AM

Originally posted by emilyjia2000 View Post

Hi Richard,

I do want to convert SAM to BAM, it output error when I used "samtools view -b in.sam -o out.bam". I checked the header of SAM file, it comes with @PG. I don't know how to deal with it?

Thanks

Emily,

As Richard said you need to us the -S option (in addition to your other options) to tell samtools view that the INPUT is in SAM format. By default samtools view expects a BAM file as input but you are giving it a SAM file, that's what is causing an error.

**SDBP** · 06-14-2011, 08:00 AM

I am dealing with the same kind of SAM files - header @PG.
I tried -S option, it didn't work.
First I saw the segmentation fault. When I fixed that and ran

samtools view -bt my.fa.fai my.sam > my.bam - It showed the following

[sam_read1] reference 'chr3.fa' is recognized as '*'.
[sam_read1] reference 'chr1.fa' is recognized as '*'.
[sam_read1] reference 'chr19.fa' is recognized as '*'.
[sam_read1] reference 'chr3.fa' is recognized as '*'.

Then I did a sed s/.fa// on the input file before doing export2sam.pl and ran export2sam.pl, it throws the following errors:

ERROR: Unexpected number of fields in export record on line 285 of read1 export file. Found 21 fields but expected 22.
...erroneous export record:
ABC-GA2 1 4 1 3 1347 0 1 TTTCNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNN_BBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBB QC

Any insight will be helpful.
Any other SAM to BAM tools known for sam files with @PG ?????

**Richard Finney** · 06-14-2011, 08:25 AM

What is the full command you are using for export2sam.pl ?
Beware that the input is supposed to be a "GERALD" type of file (also know as "illumina export file").

**SDBP** · 06-14-2011, 09:11 AM

perl export2sam.pl --read1=my_export.txt > my_export.sam

**Richard Finney** · 06-14-2011, 09:13 AM

What version of samtools?

**SDBP** · 06-14-2011, 11:31 AM

samtools-0.1.16

**Richard Finney** · 06-14-2011, 11:38 AM

The perl code is ...

if(scalar(@t) < EXPORT_SIZE) {
my $msg="\nERROR: Unexpected number of fields in export record on line $line_no of read$read_no export file. Found " . scalar(@t) . " fields but expected " . EXPORT_SIZE . ".\n";
$msg.="\t...erroneous export record:\n" . $line . "\n\n";
die($msg);

EXPORT_SIZE is 22 ( EXPORT_SIZE => 22 )

It's complaining that line 285 has only 21 fields.

What are on lines 284 and 285 ?

**SDBP** · 06-14-2011, 11:58 AM

Line 284:

ABC-DE2 1 4 1 3 119 0 1 GAGTNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNN BBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBB QC N

Line 285:
ABC-DE2 1 4 1 3 1347 0 1 TTTCNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNN fa_BBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBB QC N

I see that there is the extra 'fa' in line 285.....
can I try deleting it?
will deleting it work?

**SDBP** · 06-14-2011, 12:10 PM

Sorry, the above was from the file where I did not remove the .fa

Below is from the file which I am working on:

ABC-DE2 1 4 1 3 1347 0 1 TTTCNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNN_BBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBB QC

**SDBP** · 06-14-2011, 12:19 PM

On another line I see :

ABC-DE2 1 4 1 3 1978 0 1 CAATNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNN _]_BBBBBBBBBBBBBBBBBBBBBBBBBBBBBBBB QC

This way I will have to go through the whole file?

**Richard Finney** · 06-14-2011, 12:21 PM

Hmmmm.

You might be messing up with the sed command:

sed s/.fa//

that's saying change "anychar+f+a" to nothing.

"f" and "a" appear to be legitimate GERALD (or whatever, "export") quality value, so they'll get unintentionally changed to null , as well as the intended strings likes "chr1.fa" --> "chr1"

Glance at the input file for legitimate quality values (the field after the sequence field)

In sed language , putting a backslash before dot (i.e. \. ) means "period" to distinguish from the sole dot (i.e. .) which means "any character".

Topics	Statistics	Last Post
Evaluating Genome Sequencing for ECMO Patients in the NICU by seqadmin Started by seqadmin, 12-17-2024, 10:28 AM	0 responses 23 views 0 likes	Last Post by seqadmin 12-17-2024, 10:28 AM
New Genetic Toolkit Refines Studies on Gene Function and Disease by seqadmin Started by seqadmin, 12-13-2024, 08:24 AM	0 responses 42 views 0 likes	Last Post by seqadmin 12-13-2024, 08:24 AM
Study Links Brain Mechanism to Emotional Responses in Animals and Humans by seqadmin Started by seqadmin, 12-12-2024, 07:41 AM	0 responses 28 views 0 likes	Last Post by seqadmin 12-12-2024, 07:41 AM
Study Identifies Ribosomal RNA Fingerprints as Early Cancer Biomarkers by seqadmin Started by seqadmin, 12-11-2024, 07:45 AM	0 responses 42 views 0 likes	Last Post by seqadmin 12-11-2024, 07:45 AM

Seqanswers Leaderboard Ad

Announcement

.SAM to .BAM with SAM file header @PG

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Comment

Latest Articles

ad_right_rmr

News