I think I found the corresponding read (same spot) in another file. Sorry for the post.

dumping paired-end reads from .sra files

Dear All,
I am sharing an experience how to dump .sra file into fastq files. Always pass flag to fastq-dump command. It will save forward and reverse reads in separate files. If the .sra file contains only the single end read only one fastq file will be generated.
Thanks

query

kindly someone pls help me as to will the --split3 flag in fastq dump will surely generate a R1 and R2 file... as to I am not quite sure that my data is single ended or paired. when i converted using this flag and used for bowtie the result was as follows:
102886046 reads; of these:
102886046 (100.00%) were paired; of these:
95447806 (92.77%) aligned concordantly 0 times
3451944 (3.36%) aligned concordantly exactly 1 time
3986296 (3.87%) aligned concordantly >1 times
----
95447806 pairs aligned concordantly 0 times; of these:
30023949 (31.46%) aligned discordantly 1 time
----
65423857 pairs aligned 0 times concordantly or discordantly; of these:
130847714 mates make up the pairs; of these:
57243419 (43.75%) aligned 0 times
46040125 (35.19%) aligned exactly 1 time
27564170 (21.07%) aligned >1 times
72.18% overall alignment rate



I think this is not a good result for a paired seq.!!!


kindly help.