Hi Stephan,
Would you really sonicate nearly 96 cDNA samples? The whole idea behind using Nextera is that the transposable element fragments the DNA for you. That makes it possible to construct 96 or 384 libraries at a time.

The main problems with running C1 libraries on a HiSeq 4000 would be:

(1) Apparently the 3000/4000 doesn't do so well with with large insert libraries. They can jump the walls of the patterned flowcell?! Not really an issue, I would think as Nextera doesn't tend to make particularly large insert libraries.
Worst case, just do a size select on your library pool prior to clustering.

(2) Illumina sales reps told me that HiSeq 3000/4000 SBS kits come ready to do dual indexing. Nextera 96 and 384-library construction kits use dual indexing. But if the other lanes on the HiSeq flowcell use single indexed libraries, the sequencing core may not want to do the run as a dual indexed one. And the flowcells have 8 lanes.
Whereas the HiSeq 2500 Rapid flowcells only have 2 lanes. So running a dual indexed run on one of them is fine.
Still, I bet running single and dual indexed lanes on the HiSeq 3000/4000 would work. Just run them all as dual and demultiplex off-instrument twice. Once for the dual indexed lanes and once for the single indexed lanes.

Finally, I would recommend your contacting Fluidigm. I'm sure they have experience running their samples on a HiSeq3000/4000

--
Phillip