Around half should be "forward" and half should be "reverse". Each molecule should generate one read of insert, not two.

Reference

Dear Brian, thank you for your answer.

Are you aware about any possible reference where I can find more detailed information about the process of producing forward and reverse reads, and how this can be treated in the context of the downstream analysis.

Many thanks

All normal high-throughput DNA sequencing produces 50% of reads forward and 50% reverse; so, downstream analysis tools are designed to cope with that, typically by treating the strand as unimportant. There are some notable exceptions, such as strand-specific RNA-seq.

In some cases, like when calling variations after alignment, requiring the variation to have been seen both on a plus and minus mapped read can be used as a heuristic to reduce false positives, but for the most part, the strand is ignored.

PacBio is a little different because the molecules can be read multiple times, alternating between plus and minus. Probably, the strand of the read of insert is the strand of the first complete read-through, but it doesn't really matter, and of course the software has no way of knowing which strand is which since it depends on the reference.

As for references for reading further... hmmm, maybe someone else will suggest one?

For a single molecule (SMRT Bell) sequencing can start anywhere, therefore for a single consensus (read of insert) the chances of being forward or reverse are 50/50. http://www.ncbi.nlm.nih.gov/pmc/articles/PMC2926623/

Thank you very much