Entering edit mode
9.4 years ago
silas008
▴
170
Hi
I did a RNAseq to small RNAs (18-30nt). But the last (27-30) bases are with bad quality. Should I to cut that reads or not? I trimmed the last reads to obtain 18-25 reads and analyzed with this approach but I don't know this is correct.
What is your read length? If it is long then you would cut the ends anyway.
Reads = 36nt. Shoul I cut the ends to obtain reads 18-30nt?
Well if your reads are 36nt and 30 bases out of that are bad it will be a challenge to get useful information out regardless what you do.
I think he means base 27 onwards are bad quality. And yes, if they are bad quality you should trim, but if base 26 is good why did you trim it?
I see, I misread that section. There is no problem them ;-)
Sorry. The bad quality scores are about 27 base, not exactly 27. But before 25 base I have very good quality scores.