Entering edit mode
2.1 years ago
Aiswarya
▴
10
Hai,
I am running fastQC on small RNAseq datasets, the per-base sequence content is peculiar (they are not parallel but all squiggly). I thought it might be because of my dataset and ran fastqc on another small RNAseq data but it looks the same. Any idea why this is happening??
This is what it looks like:
take known small RNA sequences, turn them into a fastq file
now run fastqc on that file. I bet the plot will be squiggly as well
The small rna has a function, and the fragments start in the same position. the bases are not supposed to be random by position.
That makes perfect sense. And as you said the fastq for known small RNA seq (attached is fastqc for a list of piRNAs from piRNA
bank) looks all squiggly.
(Offtopic - I wonder why there are no 'G's)
probably T is missing because you have RNA with uracil (U) instead
fear not you can fix it with another tool called
seqkit, not to be confused withseqtk:-)uh!! A reminder to remember the basics.
Thank you :)