Dear all,

I'm busy with an RNA-seq analysis of case and control samples and got some differentially expressed coding genes and long non-coding RNA (lncRNA) by edgeR. I would like to do an integrative lncRNA-mRNA analysis; the library size of cases is small (about 2 million raw counts) compared to controls (about 60 million raw counts), so I filtered the genes with CPM value of less than 5 during the edgeR analysis. Given that the lncRNAs usually have the low expression value, I'm concerned about the CPM threshold as some lncRNA may miss during the analysis. Could you please share your idea about the analysis?

Thanks a lot

The fact is indeed that lncRNAs are lowly expressed, apart from notable exceptions (MALAT1, XIST, TSIX, etc) under certain conditions. Are you more worried about the difference in library size? Neither of us can see your data and try out different filters. However, you could start with CPM > 1 as a minimum cut-off, and take it from there.

It is likely, in my opinion, that many known lncRNAs are merely reflective of 'transcriptional noise' —being expressed as a result of the expression of nearby protein coding genes, for example— and, for all intents and purposes, may have no function other than to occupy volume in the nucleus and cytoplasm, where they will be digested. They are still expressed, though, and using a cut-off of 1 will at least ensure that these are included in your analysis, for better or for worse.

If your approach is ultimately about correlation, then the large library size differences may not have as large an effect as you think (because correlation metrics will be independent of it). Again, though, we cannot see the data - I would be checking histograms, box-and-whisker plots, summary statistics, etc.

Kevin