Hey I figured it out myself:

The following commands works:
samtools view -b -f 67,131,179,115 old.bam > new.bam

I am sorry for not giving this enough try before posting. I will not delete the post as it may help someone stupid like me in future.

Hey I thought I found the solution but I was wrong

Hi,

I am using the following samtool view command to output the information about properly placed mate pairs (solid) in the output bam file.

samtools view -b -f 67,131,179,115 old.bam > new.bam

-f 67 and -f 115 correspond to first read in the mate pairs that are properly placed on forward strand and reverse strand respectively.

-f 131 and -f 179 correspond to second read in the mate pairs that are properly placed on forward strand and reverse strand respectively.

Somehow in the new.bam file I am only getting reads with -f 115 and -f 67 flags (first read in the mate pair). The reads for -f 131 and -f 179 flags are totally missing (second read in the mate pair). When I run samtool flagstat I get something like:

71398431 + 0 read1
0 + 0 read2

Can someone help me with this ? I need both first and second reads of the mate-pair in the output file.

Thanks.