A larval zebrafish model of cardiac physiological recovery following cardiac arrest and myocardial hypoxic damage

Author:

Burggren Warren12ORCID,Abramova Regina12,Bautista Naim M.12ORCID,Fritsche Danielson Regina3ORCID,Dubansky Ben12ORCID,Gupta Avi12,Hansson Kenny4ORCID,Iyer Neha12ORCID,Jagadeeswaran Pudur12ORCID,Jennbacken Karin4ORCID,Rydén-Markinhutha Katarina4,Patel Vishal12,Raman Revathi12ORCID,Trivedi Hersh12,Vazquez Roman Karem12ORCID,Williams Steven12,Wang Qing-Dong4ORCID

Affiliation:

1. Developmental Integrative Biology Research Group 1 , Department of Biological Sciences , , Denton, TX 76205 , USA

2. University of North Texas 1 , Department of Biological Sciences , , Denton, TX 76205 , USA

3. SVP and head of Research and Early Development, Cardiovascular, Renal and Metabolism (CVRM), BioPharmaceuticals R&D 2 , AstraZeneca, Gothenburg 431 50 , Sweden

4. Bioscience Cardiovascular, Research and Early Development, Cardiovascular, Renal and Metabolism (CVRM), BioPharmaceuticals R&D 3 , AstraZeneca, Gothenburg 431 50 , Sweden

Abstract

ABSTRACT Contemporary cardiac injury models in zebrafish larvae include cryoinjury, laser ablation, pharmacological treatment and cardiac dysfunction mutations. Although effective in damaging cardiomyocytes, these models lack the important element of myocardial hypoxia, which induces critical molecular cascades within cardiac muscle. We have developed a novel, tractable, high throughput in vivo model of hypoxia-induced cardiac damage that can subsequently be used in screening cardioactive drugs and testing recovery therapies. Our potentially more realistic model for studying cardiac arrest and recovery involves larval zebrafish (Danio rerio) acutely exposed to severe hypoxia (PO2=5-7 mmHg). Such exposure induces loss of mobility quickly followed by cardiac arrest occurring within 120 min in 5 days post fertilization (dpf) and within 40 min at 10 dpf. Approximately 90% of 5 dpf larvae survive acute hypoxic exposure, but survival fell to 30% by 10 dpf. Upon return to air-saturated water, only a subset of larvae resumed heartbeat, occurring within 4 min (5 dpf) and 6-8 min (8-10 dpf). Heart rate, stroke volume and cardiac output in control larvae before hypoxic exposure were 188±5 bpm, 0.20±0.001 nL and 35.5±2.2 nL/min (n=35), respectively. After briefly falling to zero upon severe hypoxic exposure, heart rate returned to control values by 24 h of recovery. However, reflecting the severe cardiac damage induced by the hypoxic episode, stroke volume and cardiac output remained depressed by ∼50% from control values at 24 h of recovery, and full restoration of cardiac function ultimately required 72 h post-cardiac arrest. Immunohistological staining showed co-localization of Troponin C (identifying cardiomyocytes) and Capase-3 (identifying cellular apoptosis). As an alternative to models employing mechanical or pharmacological damage to the developing myocardium, the highly reproducible cardiac effects of acute hypoxia-induced cardiac arrest in the larval zebrafish represent an alternative, potentially more realistic model that mimics the cellular and molecular consequences of an infarction for studying cardiac tissue hypoxia injury and recovery of function.

Funder

AstraZeneca

University of North Texas

Publisher

The Company of Biologists

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