Our local sequencing centers will generally us 454 data as the raw SFF file, plus the reads as FASTA with QUAL files (redundant if you can cope with the SFF file), plus a folder with all the output from running it through Newbler to give a draft assembly (redundant if you have the resources to run Newbler or other tools yourself). For example, the file 454ReadStatus.txt tells you which reads were used in contigs, were singletons, or were discarded.

Some sequencing centers will also generate some basic graphs, for example looking at the read lengths or contig lengths as a very simple way to gauge the overall quality/volume of output.

If you plan to do your own assembly or other analysis, I would ask for the raw SFF file.

Could somebody explain in detail about 'Singleton' reads and how they can be identified in the 'all reads' file. Also how useful it is to filter the singletons?

Hi maubp,

i have sff files from 454 and want to use CLC for de novo assembly and further analysis, I wana ask that what's the difference if I map my contigs to reference or do BLAST??????
what you could recommend the settings for de novo assembly?????????
waiting for reply

What's that got to do with this thread (Extracting contig info and singletons) AAWT?

Maybe you should start a new thread with more details about your problem.