Dear all,

I want to download some SRR files, and then convert them to fastq files. For that, I've used the following SRA-toolkit commands:

prefetch SRR3159525
fastq-dump SRR3159525.sra

The download was done successfully, and the size of the resulted fastq file seems correct (~8G).

But when I've checked the content of the fastq file, I found the file was strangely formatted as follows:

 @SRR3159522.1 2_33_78 length=50
 T..................................................G
 +SRR3159522.1 2_33_78 length=50
 !!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!
 @SRR3159522.2 2_36_51 length=50
 T..................................................G
 +SRR3159522.2 2_36_51 length=50
 !!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!
 @SRR3159522.3 2_39_77 length=50
 T30.0..2.0.....2.2..2.0..0......0....1...220.2.3322G
 +SRR3159522.3 2_39_77 length=50
 !(*!%!!(!%!!!!!%!%!!%!&!!%!!!!!!*!!!!&!!!%%*!%!&%'%!
 @SRR3159522.4 2_39_134 length=50
 T01.0..0.1.....2.0..2.2..2......1....1...231.0.3312G
 +SRR3159522.4 2_39_134 length=50
 !1&!(!!&!.!!!!!%!(!!%!%!!)!!!!!!)!!!!%!!!%%(!%!/)%%!
 ...
 ...

As you can see, the sequence of the reads contains integers delimited by T and G?

Thank you for your help in advance

After googling, some biostars posts like (Transforming And Manipulating Color Space Reads) talk about the Color Space representation of the reads generated by some sequencing instruments which operate with color space formats like ABI-SOLID. For such a system the content of the reads are integers representing the colors, then an encoding table can be used to convert the integers to DNA bases.

Please refer to this excellent post which explains the system in more details: Transforming And Manipulating Color Space Reads