Skip to content
New issue

Have a question about this project? Sign up for a free GitHub account to open an issue and contact its maintainers and the community.

Sign up for GitHub

By clicking “Sign up for GitHub”, you agree to our terms of service and privacy statement. We’ll occasionally send you account related emails.

Already on GitHub? Sign in to your account

Jump to bottom

Not an issue but questions #54

Open
FritzPeleke opened this issue Apr 16, 2020 · 2 comments
Open

Not an issue but questions #54

FritzPeleke opened this issue Apr 16, 2020 · 2 comments

Comments

@FritzPeleke
Copy link

Hi I am new to NGS in general and I have a few may be dumb questions.

  • When should I use sickle se and when should I use pe?
    -Is it possible to run sickle like in a for loop so it trims like all my fastq files? If yes how
    -could you please elaborate more on its installation or direct me to a tutorial?
    Thanks :)
@pentalpha
Copy link

SE is for Single End fastq files and PE for Paired End.
A fastq (or just .fq) file is Paired End when, for each sample sequenced, there's a pair of files instead of just one.
Their names will usually be "something.1.fastq and something.2.fastq" or "something.L.fastq and something.R.fastq".

@FritzPeleke
Copy link
Author

Thanks @pentalpha

Sign up for free to join this conversation on GitHub. Already have an account? Sign in to comment
Assignees
No one assigned
Labels
None yet
Projects
None yet
Milestone
No milestone
Development

No branches or pull requests
2 participants
@pentalpha @FritzPeleke