Our lab has again questioned if single end sequencing does indeed sequence both strands of the original fragment, the Illumina videos do make this somewhat confusing. Can we confirm that the below diagram is indeed what happens?

In the Illumina video it only shows one strand binding the flow cell and beginning the process of clustering, but I assume both strands bind and then begin the process, but showing both strands would have made the video confusing.

My lab needs to sequence up to 250bp in one direction with an iseq (300 max cycles) and capture the sequence of both the forward and reverse strands (looking for base errors in each strand).

If you do single-end sequencing then only one end of the library fragment is going to be be sampled. If you have the exact DNA fragment (but now flipped 180 in a separate library fragment) then the other strand in that fragment will be sequenced.

While both p7/p5 bind at the end of the initial clustering p5 are washed away leaving only the p7 end bound strands. http://nextgen.mgh.harvard.edu/IlluminaChemistry.html should help clarify this. Also https://kscbioinformatics.wordpress.com/2017/02/13/illumina-sequencing-for-dummies-samples-are-sequenced/

My lab needs to sequence up to 250bp in one direction with an iseq (300 max cycles) and capture the sequence of both the forward and reverse strands (looking for base errors in each strand).

If you need sequence from both strands then you should do paired-end sequencing. Use a MiSeq if iseq only does 300 cycles max. Please remember that library fragments have a distribution of insert sizes. Not every fragment is going to be of the same size.