17 Oct
2012
17 Oct
'12
8:16 a.m.
On Tue, Oct 16, 2012 at 8:22 PM, Fang,Xiefan <xiefanfang@ufl.edu> wrote:
Dear Galaxy users,
Does anyone know how to merge several FASTQ groomer files by using Galaxy? If not, is there any other program that can achieve this? The size of one FASTQ groomer file is around 1GB. Thank you!
The Galaxy tool "Concatenate datasets tail-to-head" under "Text Manipulation" should work. I'm assuming you just need a simple concatenation of individual FASTQ files, not a more complex merge dealing with duplicates or sorting. Peter