Hi Gavin, generally speaking that's true assuming sufficient depth of coverage. Your aligner needs to be produce high quality gapped alignments when dealing with Ion Torrent or 454 data, which is why people tend to use aligners like TMAP, Newbler gsMapper, Novoalign, SSAHA2 or BWA-SW for these datasets.

This is a good treatment from EdgeBio of this specific problem comparing Ion Torrent and Illumina variant calling: http://www.edgebio.com/blog/?p=442

Generally speaking you can filter your SNPs by increasing thresholds on metrics such as variant frequency and proximity to homopolymers to gain a "trusted" set of variants. This means you are trading sensitivity for specificity.

Thanks a lot for the input Nick - it's a great help.

Nick, can I just follow this up?

Between MiSeq and Ion Torrent - which do you see having the greater clinical application (generally)?

Also, more specifically are the homopolymers likely to be an issue in such applications?

Cheers in advance.