Hi Petter,

I'm still pretty new to this all, so if anyone spots a wrong statement below, please feel free to point it out.

As for question 1, I think this is an inherent property of the -g (RABT) option, which tiles reference transcripts with faux reads wether the transcript is expressed in your sample or not (see http://cufflinks.cbcb.umd.edu/howitworks#hrga ). If you take your output through Cuffcompare, the "-R" option should remove any reference *.gtf transcript not expressed.

As for question 2, I don't think this is a trivial one and pretty much an own topic of research. The best ways (from a biological point of view) in my opinion would be to see if a) the transcript expression / (structure) is reproducible between replicates; and b) if the transcript is still detected when using higher mapping stringency (mismatch allowance, multimapper limit), i.e. "playing around" with the input parameters of the Mapper and Assembler. The first point of course raises your invoice considerable .

Hi

Thanks for the reply. I've realised that the output annotation is a bit unprecise, or I don't understand the labelling. Transcripts with 0 coverage and 0 in all positions except the highFPKM are labelled OK for example.

Anyhow, I have 48 samples and I've decided to filterout anything that is not present in at least two samples. After that I'll see what I have left.

/Petter