GoodDay Guys!

It seldom happens to me that samtools sort leaves the temporary files behind.

samtools sort : This command will also create temporary filesout.prefix.%d.bam as needed when the entire alignment data cannot fit into memory (as controlled via the -m option)

Ex. file.001.bam file.002.bam .......... file.00X.bam

A normal course is these split up files are merged later on to a single BAM file and deleted. I ran samtools sort on a sam file (22G) and it generated an output of 2.9G

samtools view -bSh file.sam | samtools sort - file.sam.sorted

But, now I am not sure if the samtools sort finished normally or not (because of these files left behind). How can I confirm that, rather than just running it again.

I think it's not right to just concatenate all the temporary files, (which I did) outputted a BAM file of 6.7G. There is the discrepancy.

Thanks

There have been a few errors related to samtools sort not propagating an error return value properly. One of these was fixed in PR #467, but I vaguely recall others.

In general, you would need to echo "${PIPESTATUS[0]} ${PIPESTATUS[1]}" to check the return status, but that assumes that it's returning a proper return value. The other method would be to "samtools view -c foo.bam" and see if the counts of entries jive. If the merged file is truncated then you can be certain that the temp files are not and can "samtools merge" them.

I'd say samtools sort didn't complete, since temp files are not deleted. Try to index the sorted file, if the sorted file is not complete samtools index will complain. You could also count the number of reads in the sorted file and check that this count matches the read count in the input sam.

Does the final file contains the same read count as the initial non-sorted file ? You can check that (samtools view in.bam | wc -l or samtools idxstats if the file is indexed). Both files (non-sorted and sorted) should have the same size.

Also, I would check if the header of the sorted file indicates (Should be like @HD VN:1.3 SO:coordinate)

You could try samtools idxstats bamfile.bam to count the number of reads in the bam file :

echo $(($(samtools idxstats bafile.bam | cut -f 3| tr "\n" "+" | xargs -I{} echo {} 0) ))

Then
wc -l samfile.sam
to count the number of lines in the sam file which is the number of reads mapped + the header.

PS : from my experience, samtools always merge its intermediary files. Isn't there an error report somewhere in your terminal log ?