Entering edit mode
23 months ago
Tonkatsu
▴
30
I have imported my bam and index files into IGV and want to check the quality of my alignments for a particular gene to ensure the reported rpkm is reasonable. However I am having trouble interpreting what I am seeing from the viewer and what I should be looking for?
Do you understand RPKM well enough to be able to eyeball its accuracy using IGV alignment views?
Please note that RPKM is super outdated and you shouldn't be using it anyway.
Thank you for the reply, I understand the basis of rpkm expression, but I guess I am having trouble with the interface of igv. All I want to do is to discriminate good vs bad quality reads and see if I can more or less be confident in the aligner/ reads observed.
You should be able to set a threshold - IGV will filter out reads that fail that threshold. Read the manual and play around with IGV - that's the best way to learn.
thanks, also just a general question if I am looking at a specific gene that is comprised of 3 exons or 2 protein coding regions, and I find that some of my reads being aligned are very small proportionally to to the entire protein coding region and located only in one of those protein coding regions. Should I consider this a "bad quality" alignment generally speaking? Similarly if the read spans the entirety of one protein coding region, but is largely absent in the other (1/2), how should I classify these alignments?
I'm sure RNAseq experts can answer these questions better - I'm not sure how spliced alignments are counted in quantification operations, where an exon/CDS can be used in multiple transcripts.
Why do you think those reads are bad quality? Do these reads have low pre-alignment QUAL values or low MAPQ values after the "very small" aligned part?