A Novel Fluorescent Reporter System Identifies Laminin-511/521 as Potent Regulators of Cardiomyocyte Maturation

Author:

Chanthra Nawin,Abe Tomoyuki,Miyamoto Matthew,Sekiguchi Kiyotoshi,Kwon Chulan,Hanazono Yutaka,Uosaki Hideki

Abstract

AbstractPluripotent stem cell-derived cardiomyocytes (PSC-CMs) hold great promise for disease modeling and drug discovery. However, PSC-CMs exhibit immature phenotypes in culture, and the lack of maturity limits their broad applications. While physical and functional analyses are generally used to determine the status of cardiomyocyte maturation, they could be time-consuming and often present challenges in comparing maturation-enhancing strategies. Therefore, there is a demand for a method to assess cardiomyocyte maturation rapidly and reproducibly. In this study, we found that Myomesin-2 (Myom2), encoding M-protein, is upregulated postnatally, and based on this, we targeted TagRFP to the Myom2 locus in mouse embryonic stem cells. Myom2-RFP+ PSC-CMs exhibited more mature phenotypes than RFP- cells in morphology, function and transcriptionally, conductive to sarcomere shortening assays. Using this system, we screened extracellular matrices (ECMs) and identified laminin-511/521 as potent enhancers of cardiomyocyte maturation. Together, we developed and characterized a novel fluorescent reporter system for the assessment of cardiomyocyte maturation and identified potent maturation-enhancing ECMs through this simple and rapid assay. This system is expected to facilitate use of PSC-CMs in a variety of scientific and medical investigations.

Funder

Jichi Medical University

Japan Agency for Medical Research and Development

Japan Society for the Promotion of Science

Novartis Research Grant

Japan Research Promotion Society for Cardiovascular Diseases

Takeda Science Foundation

The Uehara Memorial Foundation

SENSHIN Medical Research Foundation

the Japanese Circulation Society

Publisher

Springer Science and Business Media LLC

Subject

Multidisciplinary

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