Generating an imagingbased approach for enhanced structural and functional analysis of zebrafish cardiovascular systems
Date
2018Metadata
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Cardiovascular diseases (CVDs) have latterly become one of the leading cause of death and impairment
worldwide. According to the World Health Organization (WHO), data estimation in 2008 were about
17.3, 7.3 and 6.2 million death cases for CVDs, heart attacks, and strokes, respectively [1]. Congenital
heart defects (CHDs) are important forms of CVDs affecting about 1% of the population. According to
Dr. Ahmad Sallehuddin (Consultant and Chief of Pediatric Cardiac Surgery at HMC), CHD incidence in
Qatar is about 6-8 in every 1,000 births and about 100 new patients with CHDs require surgery every year
[4]. Both genetic and environmental factors were shown to contribute to CVDs. Human genetic studies
are not sufficient alone to explain the genetic basis of CVDs due to disease heterogeneity, inconsistent
penetrance, and predominantly a delayed onset of symptoms. Therefore, animal models are necessary
to investigate and distinguish novel genes that contribute to the pathology of CVDs and also to unravel
environmental factors that play role [5]. More recently, the Danio rerio (Zebrafish) has emerged to become
an intriguing vertebral model in medical science research. This model has several advantages, such as an
almost entirely sequenced genome that is highly preserved with humans: approximately 70% of the human
genes are estimated to have orthologue genes in the zebrafish genome [2,8]. The features of the zebrafish
over mammals as a vertebral model include its simplicity of genetic manipulation, a large quantity of
offspring, and their external and fast development [5,8]. Transparency of zebrafish embryos provide
precise observation of the heart beats, heart chambers and circulating blood in vivo via light microscopy
[5]. Additionally, passive diffusion is sufficient for oxygen delivery during early stages of zebrafish embryos development because they are independent of circulatory system [7]. Therefore, embryos
having intensive cardiac faults survive early development, which enables investigation of mutations
whereas mammalian models are not appropriate. There are many genetic cardiovascular models for
zebrafish that allow researchers to investigate cardiovascular diseases. Novel techniques are needed
for these models to assess comprehensive and quantitative phenotyping of mutant hearts and blood
vessels. These analyses involve determination of the cardiac atrial and ventricular shortening fractions,
examination of the blood flow velocities and recording of the electrocardiograms. In addition to genetic
studies, cardiotoxicity investigations for drugs or teratogens necessitate heart function and morphology
assessment. For the current study, the aim is to adapt previously established experimental and image
analysis techniques to zebrafish studies, which will enhance structural and functional analysis of the
zebrafish cardiovascular systems in biomedical research Methodology: This project involves generation
of two main protocols, which are for structural and functional analysis of zebrafish embryos. Both these
analyses are required to be performed to assess the severity of induced heart defects in zebrafish
embryos. For the structural analysis, we will perfuse zebrafish (3 -5 days post fertilization (dpf)) hearts
with microfilm, a CT- dense agent. Once it polymerises, a cast is generated for heart lumen. The embryos
are then fixed with paraformaldehyde and scanned via micro-CT. This procedure provides 3D images for
the cardiovascular systems of the animals enabling measurement of the volumes of the heart chambers.
This technique enables us to measure the effect of induced heart mutations on the heart morphology
during the embryonic growth of the animal. We have previously used this technique for visualization
of cardiac chambers for embryonic chicken successfully [3,10]. The approach is adapted for zebrafish
studies in the current work. For the functional analysis, image sequences of the beating ventricles and
the red blood cell (RBC) movements of the zebrafish larvae (3 -5 dpf) are recorded at a camera speed of
70 fps and above. This imaging is done by taking videos using Micromanager Program that is connected
to a stereomicroscope. To take image sequences, zebrafish larvae are placed on its lateral side, in which
the right side will be on top. A variety of measurements and calculations are performed using Image J
Program to assess heart functions. The parameters that are calculated include myocardial wall velocities
for assessment of severity of induced heart muscle defects, and measurement of RBC blood flow
velocities for assessment of rhythmic beating defects of the heart. Other parameters are fractional area
change, fractional shortening, heart rate, stroke volume, cardiac output and ejection fraction [9]. Stroke
volume, is the blood volume that is ejected from the heart in each beat, cardiac output, is the amount
of circulating blood across the heart in each minute, and ejection fraction, is the measurement of blood
that is ejected from the ventricle with each beat. This will provide more precise and accurate evaluation
on the heart function for genetically mutated animals to be compared with the normal ones. Several
zebrafish mutants display phenotypic features resembling human cardiac diseases. These mutants
whose molecular damages have been determined like mutations in regulatory myosin light chain, titin,
cardiac troponin T, essential myosin light chain, and beta-myosin heavy chain, have been linked with
cardiomyopathy in humans [6]. Therefore, reduced contractility, myocardial wall velocities, and cardiac
output can be studied as a sign of having cardiomyopathy. Accordingly, opening ways to apply drugs
for morphological and structural evaluation of the heart. In conclusion, in this study, we are developing
imaging-based techniques for accurate structural and functional analysis of the zebrafish hearts through
adapting previously established methods on another animal systems. Once we establish our approach,
analysis methods will be readily available for other Zebrafish researchers.
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