Hi All!

I am analyzing scRNAseq data. Unfortunately, I have the same sample split in multiple flowcells (2) and multiple lanes (2). I have read that there is no problem merging the fastqs files from different lanes. I am wondering if I can then merge the merged fastq (by lanes) by flowcells.

Thank you!

If it's the exact same library, cat it together, no matter how many lanes or flowcells it is distributed on.