We're currently looking at different assemblers, and I'm in the process of learning about/testing ALLPATHS-LG. At the present we have 14 lanes of illumina data (for a mammalian-sized genome), but don't yet have the fragment (= superread) library. Could I still get a decent assembly by artificially creating the fragment library from a library of Sanger reads?

Thanks!

This would probably work, as long as you have (1) high quality across the whole read (2) enough coverage. For (1) the super-read is constructed by overlapping alignment of 100bp reads from a 180bp fragment, so that the lower quality 3' ends of each read overlap to produce an overall higher quality 180bp read. For (2) I think you could be in trouble, as you won't get the 50x required from a Sanger library, unless you shred your Sanger reads into overlapping 180bp reads to the sufficient depth. In this case it would probably be fine.