Development of Tg(UAS:SEC-Hsa.ANXA5-YFP,myl7:RFP); Casper( roy-/-,nacre-/-) Transparent Transgenic In Vivo Zebrafish Model to Study the Cardiomyocyte Function

Surendra K Rajpurohit; Aaron Gopal; May Ye Mon; Nikhil G Patel; Vishal Arora

doi:10.3390/cells10081963

Development of Tg(UAS:SEC-Hsa.ANXA5-YFP,myl7:RFP); Casper( roy^-/-,nacre^-/-) Transparent Transgenic In Vivo Zebrafish Model to Study the Cardiomyocyte Function

Cells. 2021 Aug 2;10(8):1963. doi: 10.3390/cells10081963.

Authors

Surendra K Rajpurohit¹, Aaron Gopal², May Ye Mon¹, Nikhil G Patel³, Vishal Arora²

Affiliations

¹ Georgia Cancer Center, Medical College of Georgia, Augusta University, Augusta, GA 30912, USA.
² Department of Medicine, Division of Cardiology, Medical College of Georgia, Augusta University, Augusta, GA 30912, USA.
³ Department of Pathology, Medical College of Georgia, Augusta University, Augusta, GA 30912, USA.

Abstract

The zebrafish provided an excellent platform to study the genetic and molecular approach of cellular phenotype-based cardiac research. We designed a novel protocol to develop the transparent transgenic zebrafish model to study annexin-5 activity in the cardiovascular function by generating homozygous transparent skin Casper(roy^-/-,nacre^-/-); myl7:RFP; annexin-5:YFP transgenic zebrafish. The skin pigmentation background of any vertebrate model organism is a major obstruction for in vivo confocal imaging to study the transgenic cellular phenotype-based study. By developing Casper(roy^-/-,nacre^-/-); myl7; annexin-5 transparent transgenic zebrafish strain, we established time-lapse in vivo confocal microscopy to study cellular phenotype/pathologies of cardiomyocytes over time to quantify changes in cardiomyocyte morphology and function over time, comparing control and cardiac injury and cardio-oncology. Casper contributes to the study by integrating a transparent characteristic in adult zebrafish that allows for simpler transparent visualization and observation. The Casper(roy^-/-,nacre^-/-) transgenic progenies developed through cross-breeding with the transgenic strain of Tg(UAS:SEC-Hsa.ANXA5-YFP,myl7:RFP). Confocal and fluorescent microscopy were being used to obtain accurate, precise imaging and to determine fluorescent protein being activated. This study protocol was conducted under two sections; 1.1: Generation of homozygous Tg(UAS:SEC-Hsa.ANXA5-YFP,myl7:RFP); Casper(roy^-/-,nacre^-/-) zebrafish (generation F01-F06) and 1.2: Screening and sorting the transparent transgenic progeny and in vivo imaging to validate cardiac morphology through in vivo confocal imaging. We coined the newly developed strain as Tg(UAS:SEC-Hsa.ANXA5-YFP,myl7:RFP); Casper(roy^-/-,nacre^-/-)^gmc1. Thus, the newly developed strain maintains transparency of the skin throughout the entire life of zebrafish and is capable of application of a non-invasive in vivo imaging process. These novel results provide an in vivo whole organism-based platform to design high-throughput screening and establish a new horizon for drug discovery in cardiac cell death and cardio-oncology therapeutics and treatment.

Keywords: annexin-5; cardiomyocyte; cellular phenotype; fluorescent screening; in vivo confocal imaging; transgenic strain; transparent skin mutant-Casper(roy−/−,nacre−/−); zebrafish.

Publication types

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

MeSH terms

Animals
Animals, Genetically Modified / genetics*
Annexin A5 / genetics
Annexin A5 / metabolism
Luminescent Proteins / genetics
Luminescent Proteins / metabolism
Microphthalmia-Associated Transcription Factor / deficiency
Microphthalmia-Associated Transcription Factor / genetics
Microscopy, Confocal
Models, Animal
Myocytes, Cardiac / metabolism*
Skin Pigmentation
Zebrafish / genetics*
Zebrafish Proteins / deficiency
Zebrafish Proteins / genetics*
Zebrafish Proteins / metabolism

Substances

Annexin A5
Luminescent Proteins
Microphthalmia-Associated Transcription Factor
Zebrafish Proteins
mitfa protein, zebrafish

Grants and funding

CURS Grant/Medical College of Georgia, Augusta University