Hi everybody,

i'm doing an analysis on 16S PE amplicon sequencing data of soil samples taken from the same soil in two different seasons. I want to measure and test for differences in alpha diversity using 3 samples per season.

My problem is that i have one of these samples (i'm gonna call it A) already with lower number of reads, than also the reverse (R2) reads of this sample are low quality!! ... so when i use trimmomatic the number of total reads of A is already reduced (around 48% of only R1 surviving reads). after all of this i have around 17k of sequences for R1A and R2A while around 100k for R1 and R2 in the other samples.

Wouldn't it be better if i just remove R2A prior to trimmomatic so i'll reatin more information?

do you think reviewer will be ok with this? (treating different samples in different ways)

Michele

First of all, if you still have the samples and the funding, I recommend you to re-sequencing them again, if you have enough time.

However, in this case, I assume your sample is 16s, then it should be bacteria. You may use only R1 as long you have the phenotype result, for example increment of pH due to nitrite amount to prove your soil sample contains nitrite-synthesis bacteria. Then, all reads should be treated similar as your worst case.

Hope it helps!