Investigating microbial size classes associated with the transmission of stony coral tissue loss disease (SCTLD)

James S. Evans; Valerie J. Paul; Blake Ushijima; Kelly A. Pitts; Christina A. Kellogg

doi:10.7717/peerj.15836

PeerJ (Aug 2023)

Investigating microbial size classes associated with the transmission of stony coral tissue loss disease (SCTLD)

James S. Evans,
Valerie J. Paul,
Blake Ushijima,
Kelly A. Pitts,
Christina A. Kellogg

Affiliations

James S. Evans: St. Petersburg Coastal and Marine Science Center, U.S. Geological Survey, St. Petersburg, Florida, United States of America
Valerie J. Paul: Smithsonian Marine Station, Ft. Pierce, Florida, United States of America
Blake Ushijima: Smithsonian Marine Station, Ft. Pierce, Florida, United States of America
Kelly A. Pitts: Smithsonian Marine Station, Ft. Pierce, Florida, United States of America
Christina A. Kellogg: St. Petersburg Coastal and Marine Science Center, U.S. Geological Survey, St. Petersburg, Florida, United States of America

DOI: https://doi.org/10.7717/peerj.15836
Journal volume & issue: Vol. 11
p. e15836

Abstract

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Effective treatment and prevention of any disease necessitates knowledge of the causative agent, yet the causative agents of most coral diseases remain unknown, in part due to the difficulty of distinguishing the pathogenic microbe(s) among the complex microbial backdrop of coral hosts. Stony coral tissue loss disease (SCTLD) is a particularly destructive disease of unknown etiology, capable of transmitting through the water column and killing entire colonies within a matter of weeks. Here we used a previously described method to (i) isolate diseased and apparently healthy coral colonies within individual mesocosms containing filtered seawater with low microbial background levels; (ii) incubate for several days to enrich the water with coral-shed microbes; (iii) use tangential-flow filtration to concentrate the microbial community in the mesocosm water; and then (iv) filter the resulting concentrate through a sequential series of different pore-sized filters. To investigate the size class of microorganism(s) associated with SCTLD transmission, we used 0.8 µm pore size filters to capture microeukaryotes and expelled zooxanthellae, 0.22 µm pore size filters to capture bacteria and large viruses, and 0.025 µm pore size filters to capture smaller viruses. In an attempt to further refine which size fraction(s) contained the transmissible element of SCTLD, we then applied these filters to healthy “receiver” coral fragments and monitored them for the onset of SCTLD signs over three separate experimental runs. However, several factors outside of our control confounded the transmission results, rendering them inconclusive. As the bulk of prior studies of SCTLD in coral tissues have primarily investigated the associated bacterial community, we chose to characterize the prokaryotic community associated with all mesocosm 0.22 µm pore size filters using Illumina sequencing of the V4 region of the 16S rRNA gene. We identified overlaps with prior SCTLD studies, including the presence of numerous previously identified SCTLD bioindicators within our mesocosms. The identification in our mesocosms of specific bacterial amplicon sequence variants that also appear across prior studies spanning different collection years, geographic regions, source material, and coral species, suggests that bacteria may play some role in the disease.

Published in PeerJ

ISSN: 2167-8359 (Online)
Publisher: PeerJ Inc.
Country of publisher: United States
LCC subjects: Medicine; Science: Biology (General)
Website: https://peerj.com/

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