Abstract

The goal of this project is to understand the unitary steps of cardiovascular development. The approach combines genetics, molecular biology, and embryology. We have shown that the zebrafish heart and vasculature are amenable to genetic dissection, accessible to embryological manipulation in a transparent embryo, and analogous to the mammalian through the heart tube stage. During the two years of the current grant, we have completed the largest genetic screen for cardiovascular mutations ever undertaken. We have identified 124 recessive lethal mutations which specifically disrupt cardiovascular development. For example, we have mutants which lack endocardium or valves, those which have hearts that are too small or too large, and those constituted of a single chamber. In addition, by single-cell tracer injection, we have discovered the location of a heart field in the blastula and identified cells that give rise to both myocardium and endocardium.
Specific Aim 1 is to complete the complementation analysis of the different mutations and to map the mutations onto our zebrafish genome map. This is the first step towards cloning of the mutant genes.
Specific Aim 2 is to analyze the embryonic heart field and lineage tree of cardiac progenitors. In particular, our evidence suggests that there is a common progenitor cell in the ventral-marginal blastula for myocardium, endocardium, endothelium, and blood and we need to test this hypothesis by defining the sublineages. We have evidence that the heart field of the blastula is spatially determined, at least in part, by the divergent homebox gene tinman, and we will assess this thesis by ectopic overexpression combined with cell tracking.
Specific Aim 3 focuses upon the two mutations we discovered that are of clear-cut interest to the patterning of the vasculature. Each perturbs genesis of a specific stretch of endothelium: (a) cloche abolishes the endocardium (and possibly some head endothelium). Our hypothesis is that it blocks endocardial progenitors during their formation ow migration; (b) gridlock blocks vessel assembly in the region where the two dorsal aortae merge to become a single aorta. Many attributes of this mutant resemble the human disease coarctation of the aorta. Our primary question is whether the defects are in the endothelial cells or in the microenvironment. The mutations provide a resource for the entire community of cardiovascular scientists. They define decisions in vascular development. We hope that they can render more accessible the fashioning of higher order complex organs such as the heart, and can be used to define interacting genes. The identification of the earliest heart field is a first step towards definition of the molecular nature of the earliest cardiac progenitors. The endothelial mutations, in particular, provide the first evidence for discrete regional patterning in endothelial assembly. In medical terms, the mutations provide indices to the key unitary steps of cardiac assembly, ones which may go awry in some of the common congenital and adult heart diseases. Ultimately, these will lead to the cloning of the new genes relevant to fashioning cardiovasculature and which underlie propensities to cardiovascular illness.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
5R01HL049579-06
Application #
2637995
Study Section
Human Embryology and Development Subcommittee 1 (HED)
Project Start
1993-01-01
Project End
1999-12-31
Budget Start
1998-01-01
Budget End
1998-12-31
Support Year
6
Fiscal Year
1998
Total Cost
Indirect Cost

  Institution

Name
Massachusetts General Hospital
Department
Type
DUNS #
City
Boston
State
MA
Country
United States
Zip Code
02199

  Publications

Meder, Benjamin; Katus, Hugo A; Rottbauer, Wolfgang (2008) Right into the heart of microRNA-133a. Genes Dev 22:3227-31
Bendig, Garnet; Grimmler, Matthias; Huttner, Inken G et al. (2006) Integrin-linked kinase, a novel component of the cardiac mechanical stretch sensor, controls contractility in the zebrafish heart. Genes Dev 20:2361-72
Rottbauer, Wolfgang; Wessels, Georgia; Dahme, Tillman et al. (2006) Cardiac myosin light chain-2: a novel essential component of thick-myofilament assembly and contractility of the heart. Circ Res 99:323-31
Mably, John D; Chuang, Lesley P; Serluca, Fabrizio C et al. (2006) santa and valentine pattern concentric growth of cardiac myocardium in the zebrafish. Development 133:3139-46
Rottbauer, Wolfgang; Just, Steffen; Wessels, Georgia et al. (2005) VEGF-PLCgamma1 pathway controls cardiac contractility in the embryonic heart. Genes Dev 19:1624-34
Ebert, A M; Hume, G L; Warren, K S et al. (2005) Calcium extrusion is critical for cardiac morphogenesis and rhythm in embryonic zebrafish hearts. Proc Natl Acad Sci U S A 102:17705-10
Mably, John D; Mohideen, Manzoor Ali P K; Burns, C Geoffrey et al. (2003) heart of glass regulates the concentric growth of the heart in zebrafish. Curr Biol 13:2138-47
Mayer, Alan N; Fishman, Mark C (2003) Nil per os encodes a conserved RNA recognition motif protein required for morphogenesis and cytodifferentiation of digestive organs in zebrafish. Development 130:3917-28
Childs, Sarah; Chen, Jau-Nian; Garrity, Deborah M et al. (2002) Patterning of angiogenesis in the zebrafish embryo. Development 129:973-82
Garrity, Deborah M; Childs, Sarah; Fishman, Mark C (2002) The heartstrings mutation in zebrafish causes heart/fin Tbx5 deficiency syndrome. Development 129:4635-45

Showing the most recent 10 out of 41 publications