Entering edit mode
6.5 years ago
grayapply2009
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300
We recently did RNA-seq for our samples and quantified the expression levels of the 7 transcripts of one gene. We found one of these transcripts are expressed significantly higher (30x) than other transcripts across all of our samples.
Any explanation for this constantly high expression for a single transcript? Why do transcripts of the same gene have different expression levels? Are there any papers about this phenomenon?
Please help me. Thanks.
Another question, we did qPCR to validate the RNAseq results. We found less difference between our "major isoform" and all other isoforms than what we found in RNAseq. Is this just a technical difference or does this have something to do with biology?
Was the RNA-seq sample amplified by PCR before sequencing? You could be seeing 30x increase in the RNA-seq results due to effects from PCR in library prep?
But the ratio should not change, right?
RNAseq: Variant 1 / Variant 2 = 25
qPCR: Variant 1 / Variant 2 = 10
How do you explain this?
Because the exponential nature of PCR, a small original difference in Variant 1 and Variant 2 will be much greater after many cycles of PCR. I believe qPCR will account for this, whereas your RNAseq pipeline may not be accounting for that exponential increase.
Please someone chime in if this is incorrect, but that's how I understand it.
That sounds reasonable, goodez.
It is not a good practice to ask new questions in a thread that is already there. It breaks the flow of conversation of an existing thread. You should have posted this as an independent question.
qPCR generally has poorer sensitivity than RNAseq. Further, you were hopefully checking this on new samples, so you're observing a bit of an expected regression to the mean.