AbstractsBiology & Animal Science

Transcriptome analysis of the New Zealand sea urchin Kina (Evechinus Chloroticus)

by Gareth Gillard

Institution: University of Otago
Year: 0
Keywords: Transcriptome Assembly; RNA-Seq; Differential Gene Expression Analysis; Sea Urchin; Kina; Evechinus Chloroticus; Molecular Phylogenetics
Record ID: 1298038
Full text PDF: http://hdl.handle.net/10523/4885


Sea urchins are studied as model organisms for developmental and systems biology, and the sequencing of one species’ genome revealed many avenues for further studies. Sea urchins’ highly expanded innate immune system is a valuable resource for antimicrobials. Furthermore, the gonads of male and female sea urchins, referred to as the roe, are a highly valued food product internationally, with the largest demand from Asian countries such as Japan. The price of roe is greatly influenced by sensory qualities such as colour, texture and flavour, and research has focused on increasing roe quality to give it higher value. Evechinus chloroticus (Kina) is a sea urchin species that is indigenous to New Zealand. It is the type member of the Evechinus genus based on its morphological characteristics. Previous research has focused on identifying physical factors affecting the commercial roe quality of E. chloroticus, including protein and metabolite analysis, but there is almost no genetic information available for this species. E. chloroticus is the only species in its genus and has yet to be subjected to molecular phylogenetic analysis. This study aimed to increase the amount of genetic data available for the E. chloroticus species through transcriptome assembly and analysis, which would aid current and future research on E. chloroticus. In this study, a de novo transcriptome assembly of Illumina sequencing data was carried out. A total of 123 million 100 base length paired-end reads were generated using RNA-Seq libraries from a range of E. chloroticus tissues from two individuals obtained from Fiordland, New Zealand. The assembly resulted in a set of 75,002 transcripts with an accepted read coverage and length, of which 24,655 transcripts could be functionally annotated using protein similarity. Transcripts were further annotated with Gene Ontology, KEGG Orthology and InterPro terms. The first molecular phylogenetic analysis of E. chloroticus to other species of its family was done using multiple genes. When sequences for the mitochondrial NADH dehydrogenase genes were compared, E. chloroticus remained outside of a family level clade, which indicated E. chloroticus is indeed a genetically distinct genus within its family. A differential gene expression analysis was carried out using the new reference transcriptome data. RNA-Seq libraries were generated from the roe of individual E. chloroticus females that showed a distinct grade of roe colour (light, medium or dark) and the expression of genes between different coloured roe was analysed. The results showed most gene expression in the roe remains consistent regardless of the roe colour, with a small proportion of genes shown to have differential expression. Differentially expressed genes could now be investigated to understand the role of genes whose expression correlates with colour. This study has produced a large set of E. chloroticus transcripts (and predicted proteins) along with functional annotations, vastly increasing the amount of genomic data available…