I have encountered a public dataset where they have generated scRNAseq using the 10x Chromium with both 3’ and 5’ chemistries. Since I am used to work with 3' and I do not know anybody who has worked with 5' to ask them, I wonder if I have to take special attention with the 5' data or if I have to do something different as I usually do.
I have tried to search for information... but I did not find anything about the processing (if there are differences).
I have read that the difference between them is the technique and aim of use.
In 3’ scRNA-Sequencing, poly(A)+ mRNAs are reverse transcribed using a polydT primer. This polydT sequence is located directly adjacent to the barcodes required for the identification of unique cells and for sequencing.
In 5’ scRNA-Sequencing, poly(A)+ mRNAs are reverse transcribed using a polydT primer. However, in contrast to 3’ scRNA-Sequencing, the sequencing barcodes are not adjacent to the polydT primer, but they are located at the 5' end of the transcripts. Moreover, I read that the major advantage and use of the 5′ is to combine gene expression profiling with the identification of the full V(D)J fragment (a and b chain of TCR, heavy and light chain of Igs and BCR in B-cells) in the same cells.
... but regarding the processing (if some particular steps need to be taken into account), I didn't find anything.
Does anybody can help me, please?
Any feedback will be well received.
Thanks in advance
Thanks very much for your feedback! I will take all those things in consideration once I start the analysis!
Just out of curiosity, do you usually check all those things between sc/snRNAseq too? (overlap of cell types, housekeeping genes...)
sc/snRNASeq tends to have differences in things like mitochondrial genes etc, which you can account for using tools like SCTransform but in general I just keep it in the back of my mind that there's likely a difference and I look the clustering results to see if there's likely an effect.
Noted! Thanks very much for your help!