I have H3K4me3 and H3K27me3 datasets (replicates) from mouse ESCs. I generated a list of

1. active promoters (K4me3+ K27me3-)
2. bivalent promoters (K4me3+ K27me3+)
3. nonActive promoters (K4me3- K27me3-)

I am working with protein coding Ensembl annotations, where unique TSS are included and I made a promoter set of it. I also have expression profiling from mouse ESCs and appended the isoform level expression values (using Tuxedo-Cufflinks/Cuffdiff) to the above promoter sets. What I see is a bit of discrepancy and would like your inputs.

64% of my promoters in the active list (according to histone marks) have significant H3K4me3 peak on them but are not expressed according to expression dataset. So, my questions are:

1. How Cufflinks/Cuffdiff calculates and how well it performs at isoform level calculations (considering lot of overlapping transcripts with nearby TSS from same or different genes). For example, 7 protein coding transcripts of gene Lypla1, 3 are expressed but 4 is not.

chr1    4806788    4808788    Lypla1    ENSMUST00000134384    +    1.7341
chr1    4806823    4808823    Lypla1    ENSMUST00000027036    +    66.4909
chr1    4806830    4808830    Lypla1    ENSMUST00000150971    +    0.6529 #this one
chr1    4806896    4808896    Lypla1    ENSMUST00000119612    +    18.9053
chr1    4806898    4808898    Lypla1    ENSMUST00000137887    +    3.5388
chr1    4806911    4808911    Lypla1    ENSMUST00000115529    +    15.4683
chr1    4807237    4809237    Lypla1    ENSMUST00000131119    +    3.6185

2. According to this screenshot, if loaded the Ensembl transcript id (highlighted in red). This id according to expression data has a value of <1 FPKM (definitely not expressed) but there is a K4me3 sig. peak here. So, again how well are these isoform level calculations. For sure with normal ChIP protocols we cannot differentiate that his K4me3 peak is because of which trancsript but combining with expression profiling, we can depending upon how robust and credible the values are.

Thanks for your time

This doesn't seem unusual to me.

From your data, isoform ENSMUST00000150971 was not expressed in your sample because the reads that were sequenced did not favour the presence of that transcript. Reads might have "fit" in ENSMUST00000150971 - they might have even fit nicely - but those reads where much better explained by the high abundance of the transcript ENSMUST00000027036, and so thats why it has the much higher FPKM (or whatever your expression units are).

Furthermore, be warned about making intersections between ChIP data and RNA data. There is a misconception in some areas of Epigenetics that you can compare RNA data from the transcriptome directly to DNA data (ChIP-Seq/WGBS/DNAse) from the Genome like they are the same thing. They are not at all the same thing. They don't even occupy in the same space in the cell. Intersections of one with the other will only cause pain, for exactly the reason shown here. There is no reason to even believe that high ChIP signal == high RNA expression, or anything like that. It does not even stand that ChIP signal should overlap with RNA expression when both are mapped to the genome.

Perhaps you would be better off looking at a total RNA count for the whole gene, then comparing to the ChIP signal at the promotor of that gene?