De novo metatranscriptome assembly and coral gene expression profile of Montipora capitata with growth anomaly

Monika Frazier; Martin Helmkampf; M Renee Bellinger; Scott M Geib; Misaki Takabayashi

doi:10.1186/s12864-017-4090-y

De novo metatranscriptome assembly and coral gene expression profile of Montipora capitata with growth anomaly

BMC Genomics. 2017 Sep 11;18(1):710. doi: 10.1186/s12864-017-4090-y.

Authors

Monika Frazier¹, Martin Helmkampf¹, M Renee Bellinger¹, Scott M Geib², Misaki Takabayashi^{3

4}

Affiliations

¹ Tropical Conservation Biology and Environmental Science, University of Hawai'i at Hilo, 200 West Kāwili Street, Hilo, HI, 96720, USA.
² United States Department of Agriculture, Agriculture Research Service, Daniel K Inouye U.S. Pacific Basin Agricultural Research Center, 64 Nowelo St, Hilo, HI, 96720, USA.
³ Tropical Conservation Biology and Environmental Science, University of Hawai'i at Hilo, 200 West Kāwili Street, Hilo, HI, 96720, USA. misakita@hawaii.edu.
⁴ Marine Science Department, University of Hawai'i at Hilo, 200 West Kāwili Street, Hilo, HI, 96720, USA. misakita@hawaii.edu.

Abstract

Background: Scleractinian corals are a vital component of coral reef ecosystems, and of significant cultural and economic value worldwide. As anthropogenic and natural stressors are contributing to a global decline of coral reefs, understanding coral health is critical to help preserve these ecosystems. Growth anomaly (GA) is a coral disease that has significant negative impacts on coral biology, yet our understanding of its etiology and pathology is lacking. In this study we used RNA-seq along with de novo metatranscriptome assembly and homology assignment to identify coral genes that are expressed in three distinct coral tissue types: tissue from healthy corals ("healthy"), GA lesion tissue from diseased corals ("GA-affected") and apparently healthy tissue from diseased corals ("GA-unaffected"). We conducted pairwise comparisons of gene expression among these three tissue types to identify genes and pathways that help us to unravel the molecular pathology of this coral disease.

Results: The quality-filtered de novo-assembled metatranscriptome contained 76,063 genes, of which 13,643 were identified as putative coral genes. Overall gene expression profiles of coral genes revealed high similarity between healthy tissue samples, in contrast to high variance among diseased samples. This indicates GA has a variety of genetic effects at the colony level, including on seemingly healthy (GA-unaffected) tissue. A total of 105 unique coral genes were found differentially expressed among tissue types. Pairwise comparisons revealed the greatest number of differentially expressed genes between healthy and GA-affected tissue (93 genes), followed by healthy and GA-unaffected tissue (33 genes), and GA-affected and -unaffected tissue (7 genes). The putative function of these genes suggests GA is associated with changes in the activity of genes involved in developmental processes and activation of the immune system.

Conclusion: This is one of the first transcriptome-level studies to investigate coral GA, and the first metatranscriptome assembly for the M. capitata holobiont. The gene expression data, metatranscriptome assembly and methodology developed through this study represent a significant addition to the molecular information available to further our understanding of this coral disease.

Keywords: Coral disease; Gene expression; Growth anomaly; Metatranscriptome; Montipora capitata; RNA-seq.

MeSH terms

Animals
Anthozoa / genetics*
Anthozoa / growth & development*
Gene Expression Profiling*
Morphogenesis / genetics