I searched at UCSC Genome Browser's website, but couldn't find relevant information.
The hg19 version of the canonical transcripts (knownCanonical) has 32K entries whereas hg38 version (GENCODE based) has 66K entries.
What accounts for this 2x difference?
Hello,
We have an FAQ page that covers this topic (http://genome.ucsc.edu/FAQ/FAQgenes.html#singledownload). As posted by ATpoint, it boils down to different datasets and different approaches.
hg19 knownCanonical was last updated in 2013 and built primarily from RefSeq and GenBank sequences and a few other sources. One isoform was identified from each gene (as defined by UCSC IDs) which was typically the longest isoform.
For hg38, knownCanonical was last built on the GENCODE v36 models earlier this year. In this case one canonical isoform was chosen per ENSEMBL gene ID. The hierarchy for which was chosen is described in the FAQ page.
So while the tables have the same name, they originate from different data and different designations of a gene.
A more recent and 'standardized' approach is to use NCBI's RefSeq Select transcripts (https://www.ncbi.nlm.nih.gov/refseq/refseq_select/). These are NCBI's pick of a single representative transcript for every protein-coding gene. if you compare these numbers across hg19 and hg38, you'll see they are very similar:
#Assembly #tableName #count
hg19 ncbiRefSeqSelect 21461
hg38 ncbiRefSeqSelect 21763
Sometime in the near future the MANE project (https://www.ncbi.nlm.nih.gov/refseq/refseq_select/#MANE) will release a list of canonical transcripts for hg38 that are standardized between RefSeq and GENCODE.
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Sometime in the near future the MANE project (https://www.ncbi.nlm.nih.gov/refseq/refseq_select/#MANE) will release a list of canonical transcripts for hg38 that are standardized between RefSeq and GENCODE.
These data are available now. See: https://www.ncbi.nlm.nih.gov/refseq/MANE/ for more details, and, this section for data access.
That's a good point. I'll update that now.
We also host a track (https://genome.ucsc.edu/cgi-bin/hgTrackUi?db=hg38&c=chr1&g=mane) which is .92 but will be updated to the latest .95 next week. I don't know the exact number, but .95 covers 90-95% of genes (it's slightly less than version number).
They are not specifically standardized, that's really what MANE is set to accomplish. Currently NCBI (RefSeq) and EBI (GENCODE) have a large amount of overlap with regards to their gene models as you would expect since their goal is the same. However, there are some differences.
knownGene for hg19 closely matches RefSeq but may have some major differences from GENCODE since it has not been updated in a long time, I have not looked at this closely.
knownGene for hg38 matches GENCODE, and the exon coordinates should be similar to RefSeq, but certainly not standard or the same. For one, the GENCODE comprehensive list has 232K items vs RefSeq's 173k.
So in short I'd expect most genes for hg38 would have equivalent exon coordinates (especially well annotated and researched genes), but not all.
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version 2.3.6
A: which annotation I should for RNA-seq? Ensembl, UCSC or refseq?
You are not only comparing two different genome builds here but also two different consortia (RefSeq vs GENCODE). Ensembl uses GENCODE, see linked answer.
Also: https://bmcgenomics.biomedcentral.com/articles/10.1186/1471-2164-16-S8-S2
Or simply search for Gencode vs RefSeq on the web, there are many posts addressing this.
Yes, it's RefSeq vs. GENCODE. But still it amazes me that there's 2x difference in canonical transcripts.
A canonical transcript is linked to a gene (maybe not strictly, but if we consider a cluster a gene that's what it translates to). So does that mean that when we use hg19/RefSeq based canonical transcripts, we are missing half of expressed regions?