We had this issue when trying to sequence 10x libraries alongside 150/100 PE samples on our HiSeq 4000. I spoke to Illumina and they weren't able to give me a clear answer, but basically said that after the intensity drop after the first 28 cycles the focus point drifts. It refocuses during the indexing cycles but then moves back to focus point for R1 (which is now out of focus) for R2 without refocusing. I think the bottom surface focuses better because it's a fixed distance from there to the stage, but the top surface is a little more variable.

This is how I understood it from my conversation, but at this point Illumina didn't really have much knowledge of the issue - if you access to support they may have more and clearer information now.

I have heard through the grapevine that 10x Genomics will be switiching to dual index for all their kits down the road. The new Visium kit has 10bp dual index, and the ATACseq kit already uses dual index that is clunky.

This actually makes a sense. Yeah we tried to talk to people at Illumina and 10x and none of them could really tell us whats going on or how to fix this issue except for not sequencing dual indexed. Thanks for your explanation!