by
lmh » Wed Aug 05, 2009 12:49 pm
tcay54, aren't they spoilsports. You could get your own back by getting a very large dictionary and looking out the weirdest words you can find...
DonHilton, there's some interesting work by Rick Dunn (maybe you know it, sorry if yes!) (W. Dunn, W=Warwick) on the situation you describe, with regard to metabolomics and large studies. Their approach is to make up a QC sample ideally by mixing all other samples, and run it once in every 5 runs throughout every batch they analyse. I don't believe they use any replication on the individual samples between, but can't swear to this.
The idea is that the mixed QC sample should give the same answer every time for all 500 peaks of interest that you have. You can find the relative standard deviation for each of the 500 peaks, and reject any peak that is deemed unacceptable. Dunn's lot use a 30% RSD cut-off on the grounds that biological variability of the sort of things they're looking at is of the order of 30%, and they don't want a situation where analytical variability is greater than biological/treatment variability.
They've also extended their use of QC samples to allow matching up of different batches run at different times, but that's another story.
