Transcriptomic response to elevated water temperatures in adult migrating Yukon River Chinook salmon (Oncorhynchus tshawytscha)

Author:

Bowen Lizabeth1,von Biela Vanessa R2,McCormick Stephen D34,Regish Amy M3,Waters Shannon C1,Durbin-Johnson Blythe5,Britton Monica5,Settles Matthew L5,Donnelly Daniel S2,Laske Sarah M2,Carey Michael P2,Brown Randy J6,Zimmerman Christian E2

Affiliation:

1. U.S. Geological Survey, Western Ecological Research Center, One Shields Avenue, Davis, CA, 95616, USA

2. U.S. Geological Survey, Alaska Science Center, 4210 University Drive, Anchorage, AK, 99508, USA

3. U.S. Geological Survey, Leetown Science Center, Conte Anadromous Fish Research Laboratory, 1 Migratory Way, Turner Falls, Massachusetts, 01376, USA

4. Department of Biology, University of Massachusetts, Amherst, MA, 01003, USA

5. University of California, Genome Center and Bioinformatics Core Facility, One Shields Avenue, Davis, CA, 95616, USA

6. U.S. Fish and Wildlife Service, 101 12th Avenue, Room 110, Fairbanks, AK, 99701, USA

Abstract

ABSTRACT Chinook salmon (Oncorhynchus tshawytscha) declines are widespread and may be attributed, at least in part, to warming river temperatures. Water temperatures in the Yukon River and tributaries often exceed 18°C, a threshold commonly associated with heat stress and elevated mortality in Pacific salmon. Untangling the complex web of direct and indirect physiological effects of heat stress on salmon is difficult in a natural setting with innumerable system challenges but is necessary to increase our understanding of both lethal and sublethal impacts of heat stress on populations. The goal of this study was to characterize the cellular stress response in multiple Chinook salmon tissues after acute elevated temperature challenges. We conducted a controlled 4-hour temperature exposure (control, 18°C and 21°C) experiment on the bank of the Yukon River followed by gene expression (GE) profiling using a 3′-Tag-RNA-Seq protocol. The full transcriptome was analysed for 22 Chinook salmon in muscle, gill and liver tissue. Both the 21°C and 18°C treatments induced greater activity in genes associated with protein folding (e.g. HSP70, HSP90 mRNA) processes in all tissues. Global GE patterns indicate that transcriptomic responses to heat stress were highly tissue-specific, underscoring the importance of analyzing multiple tissues for determination of physiological effect. Primary superclusters (i.e. groupings of loosely related terms) of altered biological processes were identified in each tissue type, including regulation of DNA damage response (gill), regulation by host of viral transcription (liver) and regulation of the force of heart contraction (muscle) in the 21°C treatment. This study provides insight into mechanisms potentially affecting adult Chinook salmon as they encounter warm water during their spawning migration in the Yukon River and suggests that both basic and more specialized cellular functions may be disrupted.

Funder

NIH Shared Instrumentation

U.S. Geological Survey Ecosystems Mission Area and the Arctic-Yukon-Kuskokwim Sustainable Salmon Initiative

Publisher

Oxford University Press (OUP)

Subject

Management, Monitoring, Policy and Law,Nature and Landscape Conservation,Ecological Modelling,Physiology

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