Question

Fastqc, Trimming And Kmers

1

Entering edit mode

10.1 years ago

int11ap1 ▴ 470

Good morning everybody,

I had RNA-seq data from Illumina (paired-ends), which adapters were removed and quality trimming performed successfully using Trimmomatic. After analysing with FastQC, all seems OK. However, there are one thing that worries me: the kmers. Some pictures:

enter image description here

Why is it? Apparently, there are no overrepresented sequences according to FastQC.

fastqc trimming • 4.4k views

ADD COMMENT • link updated 10.1 years ago by jackuser1979 ▴ 890 • written 10.1 years ago by int11ap1 ▴ 470

0

Entering edit mode

Just to note, the images aren't showing up for me in either Chrome of Firefox

ADD REPLY • link 10.1 years ago by Daniel ★ 4.0k

score 0 · Answer 1 · 2014-04-09

0

Entering edit mode

10.1 years ago

jackuser1979 ▴ 890

Have you checked FastQC website?. These examples will give you an idea whats wrong with your sequence:

Overrepresented Kmers: http://www.bioinformatics.babraham.ac.uk/projects/fastqc/Help/3%20Analysis%20Modules/11%20Overrepresented%20Kmers.html

Sequence Length Distribution: http://www.bioinformatics.babraham.ac.uk/projects/fastqc/Help/3%20Analysis%20Modules/8%20Sequence%20Length%20Distribution.html

ADD COMMENT • link 10.1 years ago by jackuser1979 ▴ 890

0

Entering edit mode

That site tells you what is happening and how, but doesn't tell you why or potential scenarios.

ADD REPLY • link 10.1 years ago by Adrian Pelin ★ 2.6k