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**srasdk** · 07-06-2011, 09:33 PM

All of the mentioned runs are fragments - single read

**ndeshpan** · 07-06-2011, 10:06 PM

hi,

I have downloaded a file from SRA and used fastq-dump..

However when I check my output .fastq file I see this

head -10 SRR036210.fastq
@SRR036210.1 VAB_S0040_20080711_Legend_quad_2_NK_Act_462_9_144 length=25
T2030201230313112312001111
+SRR036210.1 VAB_S0040_20080711_Legend_quad_2_NK_Act_462_9_144 length=25
!"""""""""""""""""""""""""
@SRR036210.2 VAB_S0040_20080711_Legend_quad_2_NK_Act_462_9_198 length=25
T2030201230313112312001111
+SRR036210.2 VAB_S0040_20080711_Legend_quad_2_NK_Act_462_9_198 length=25
!"""""""""""""""""""""""""
@SRR036210.3 VAB_S0040_20080711_Legend_quad_2_NK_Act_462_9_1360 length=25
T2030201230313112312001111

Any suggestions?

cheers,

Nandan

**simonandrews** · 07-06-2011, 11:12 PM

That's a colorspace fastq file. From the bit you posted it looks OK, but you'll need to use colorspace aware tools to do anything with it.

**srasdk** · 07-06-2011, 11:30 PM

fastq-dump defaults to colorspace for SOLiD technology.
You can use '-B' option to force translation into basespace if you wish - the only downside - all bases after miscalled color '.' will become 'N'

**harlock0083** · 07-07-2011, 05:41 AM

Originally posted by srasdk View Post

All of the mentioned runs are fragments - single read

Thank you for the reply.

**ndeshpan** · 07-08-2011, 07:04 PM

Thanks everyone

**afkoeppel** · 07-12-2011, 07:10 AM

I'm having the same basic problem as the original poster in this thread.
I downloaded the file: SRR063783.sra, and ran fastq-dump on it.

It's supposed to be paired-end data, but I'm only getting a single file: SRR063783.fastq

In this file it looks as though each pair of forward and reverse reads has been combined into a single sequence. Is there a way to split them up again?

**Benjamin Vincent** · 07-20-2011, 08:27 AM

Try fastq-dump -SL

**afkoeppel** · 07-20-2011, 10:30 AM

Originally posted by Benjamin Vincent View Post

Try fastq-dump -SL

This did the trick. Thank you very much.

**hithesh** · 12-01-2015, 10:34 PM

To Convert SRA to Fastq

use this command

open SRA toolkit kit path

open bin folder

fastq-dump.exe pathfile\filename outputfilename

**Tlexander** · 10-31-2016, 08:37 AM

fastq-dump --split-files --gzip ./SRR1232309.sra

**yasbo** · 09-19-2018, 11:03 PM

Hi,
Been using fasterq-dump.2 to download and save fastq files.
How can I download the fastq files using fasterq-dump and still keep original read names with details about each read as seen on ncbi website?

site: https://www.ncbi.nlm.nih.gov/sra

**fraurelie** · 10-18-2018, 01:13 AM

Converting SRA files into Fastq

Hi I am new to bioinformatics I did some courses online and loved it which doesn't mean I find it easy! On the contrary and I really admire you guys who can get around it!

First step, I want to get SRR7962225 as fastq format.

I downloaded the data sra_data.fastq.gz and the SRA toolkit but it refuses to convert it using fastq-dump however I get something like

2·43222Õ3Ô3T0TÈIÍK/É°540ä ÿÿ,ŒÁ......etc

using Notepad.

Any suggestions?

**ddb** · 10-18-2018, 03:19 AM

Some more details about the commands you have run would be helpful. If the file has a .gz extension then it needs to be unzipped first. I may be wrong but it sounds like you are on a windows os so try 7zip to decompress. Depending on your objective you might be limited on the analyses you can perform on windows os.

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