The UO_Cmon_1.0 assembly was submitted by University of Otago on November 2019. The assembly is on scaffold level, consisting of 11,985 contigs assembled into 2,996 scaffolds. The N50 size is the length such that 50% of the assembled genome lies in blocks of the N50 size or longer. The N50 length for the contigs is 331,397 while the scaffold N50 is 4,457,533.
The gene annotation process was carried out using a combination of protein-to-genome alignments, annotation mapping from a suitable reference species and RNA-seq alignments (where RNA-seq data with appropriate meta data were publicly available). For each candidate gene region, a selection process was applied to choose the most appropriate set of transcripts based on evolutionary distance, experimental evidence for the source data and quality of the alignments.Small ncRNAs were obtained using a combination of BLAST and Infernal/RNAfold. Pseudogenes were calculated by looking at genes with a large percentage of non-biological introns (introns of <10bp), where the gene was covered in repeats, or where the gene was single exon and evidence of a functional multi-exon paralog was found elsewhere in the genome. lincRNAs were generated via RNA-seq data where no evidence of protein homology or protein domains could be found in the transcript.
In accordance with the Fort Lauderdale Agreement, please check the publication status of the genome/assembly before publishing any genome-wide analyses using these data.
General information about this species can be found in Wikipedia.
|Assembly||UO_Cmon_1.0, INSDC Assembly GCA_009650515.1, Nov 2019|
|Golden Path Length||1,056,558,033|
|Annotation method||Full genebuild|
|Genebuild started||Feb 2020|
|Genebuild released||May 2020|
|Genebuild last updated/patched||Feb 2020|
|Non coding genes||1,358|
|Small non coding genes||361|
|Long non coding genes||994|
|Misc non coding genes||3|
|Genscan gene predictions||44,434|