Not yet, but probably soon. We have a group that is doing a type of IP that yields ssDNA. We have not had our Illumina a year yet, so we are pretty much sticking with the TruSeq kits from Illumina where possible. But we did have success modifying the TruSeq RNA prep protocol to use RiboZero ribo-depleted RNA. We "cut" this RNA into the step immediately following the normal polyA binding step.

So, I was wanting to try a similar trick with this ssDNA. That is, cut it in after the first strand of cDNA synthesis. This may prove to be more difficult. Many of the steps in TruSeq are tightly coupled to increase the speed of the protocol.

Next along those lines would be to replace the nucleotide mix used in second strand synthesis with a dUTP-instead-of-dTTP dNTP mix. That way, after adapter ligation, a uracil-N-glycosylase step could be added to produce strand-specific libraries.

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Phillip