De novo transcriptome sequencing of the Octopus vulgaris hemocytes using Illumina RNA-Seq technology: response to the infection by the gastrointestinal parasite Aggregata octopiana

Sheila Castellanos-Martínez; David Arteta; Susana Catarino; Camino Gestal

doi:10.1371/journal.pone.0107873

De novo transcriptome sequencing of the Octopus vulgaris hemocytes using Illumina RNA-Seq technology: response to the infection by the gastrointestinal parasite Aggregata octopiana

PLoS One. 2014 Oct 16;9(10):e107873. doi: 10.1371/journal.pone.0107873. eCollection 2014.

Authors

Sheila Castellanos-Martínez¹, David Arteta², Susana Catarino², Camino Gestal¹

Affiliations

¹ Departamento de Biotecnología y Acuicultura. Instituto de Investigaciones Marinas, Consejo Superior de Investigaciones Científicas, Vigo, Spain.
² PROGENIKA Biopharma. A Grifols Company. Parque tecnológico de Bizkaia. Derio, Bizkaia, Spain.

Abstract

Background: Octopus vulgaris is a highly valuable species of great commercial interest and excellent candidate for aquaculture diversification; however, the octopus' well-being is impaired by pathogens, of which the gastrointestinal coccidian parasite Aggregata octopiana is one of the most important. The knowledge of the molecular mechanisms of the immune response in cephalopods, especially in octopus is scarce. The transcriptome of the hemocytes of O. vulgaris was de novo sequenced using the high-throughput paired-end Illumina technology to identify genes involved in immune defense and to understand the molecular basis of octopus tolerance/resistance to coccidiosis.

Results: A bi-directional mRNA library was constructed from hemocytes of two groups of octopus according to the infection by A. octopiana, sick octopus, suffering coccidiosis, and healthy octopus, and reads were de novo assembled together. The differential expression of transcripts was analysed using the general assembly as a reference for mapping the reads from each condition. After sequencing, a total of 75,571,280 high quality reads were obtained from the sick octopus group and 74,731,646 from the healthy group. The general transcriptome of the O. vulgaris hemocytes was assembled in 254,506 contigs. A total of 48,225 contigs were successfully identified, and 538 transcripts exhibited differential expression between groups of infection. The general transcriptome revealed genes involved in pathways like NF-kB, TLR and Complement. Differential expression of TLR-2, PGRP, C1q and PRDX genes due to infection was validated using RT-qPCR. In sick octopuses, only TLR-2 was up-regulated in hemocytes, but all of them were up-regulated in caecum and gills.

Conclusion: The transcriptome reported here de novo establishes the first molecular clues to understand how the octopus immune system works and interacts with a highly pathogenic coccidian. The data provided here will contribute to identification of biomarkers for octopus resistance against pathogens, which could improve octopus farming in the near future.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Apicomplexa / physiology*
Gastrointestinal Tract / parasitology*
Gene Expression Profiling*
Gene Ontology
Hemocytes / metabolism*
Immunity, Cellular / genetics
Molecular Sequence Annotation
Octopodiformes / cytology
Octopodiformes / genetics*
Octopodiformes / immunology
Octopodiformes / parasitology
Protozoan Infections / genetics*
Protozoan Infections / immunology
Protozoan Infections / pathology
Sequence Analysis, RNA*
Signal Transduction / genetics

Grants and funding

This work has been funded by Xunta de Galicia (10PXIB402116PR). SCM wishes to acknowledge additional funding from CONACyT (Mexico). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.