Abstract

The lens has for some time served as a simple model in which to study the processes of cellular proliferation, migration and differentiation that constitute many aspects of development. Despite a large body of data describing lens development, the molecular mechanism by which this structure forms remains largely a matter of conjecture, in part because there have been few attempts to directly address questions of mechanism using in vivo systems. It is our long term aim to determine the role of fibroblast growth factor (FGF) and insulin-like growth factor type I (IUF- I) in lens development. Previous in vitro experiments have implicated these growth factors in lens development and we have chosen to develop in vivo systems that will allow us to determine if this is the case.
Our specific aims i nclude: (1 and 2) determining whether FGF is required for the differentiation of lens fiber cells and/or the proliferation of lens epithelial cells. (3 and 4) determining whether IGF-I is required for the differentiation of lens fiber cells and/or the proliferation of lens epithelial cells. (5) determining the earliest discernible time in lens development that each of these growth factors is required. (6) determining whether migration of lens epithelial cells is dependent on FGF and/or IGF- I. (7) determining whether FGF and IGF-I act in concert in a synergistic manner to stimulate lens development. Our general approach to these questions is to block growth factor signal transduction in transgenic mice using dominant negative forms of the FGF and IGF-I receptors. This approach has proven fruitful in the past for answering questions about growth factor requirements during development. A key element of the proposed experiments is our ability to direct expression of a transgene to different populations of lens cells. By using the appropriate transgene (or combination of transgenes), we will have the ability to direct expression of a dominant negative growth factor receptor to those lens cells that are either proliferating or differentiating. This experimental system is made possible by the natural expression region of alphaA-crystallin in rodents. The anterior expression boundary of alphaA- crystallin corresponds precisely to the boundary between proliferating and differentiating cells in the lens. Thus, the alphaA-crystallin promoter can be used to express transgenes in differentiating cells directly or indirectly to restrict transgene expression to proliferating cells. This experimental system will give us a unique opportunity to determine whether FGF and/or IGF-I are required for lens cell proliferation of differentiation. Abnormal modifications of the lens are a frequent cause of impaired vision. A complete knowledge of the way in which the lens forms will almost certainly have an impact on our understanding of the way in which its structure is disrupted.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Research Project (R01)
Project #
5R01EY011234-05
Application #
6138197
Study Section
Visual Sciences A Study Section (VISA)
Program Officer
Liberman, Ellen S
Project Start
1996-01-26
Project End
2000-12-31
Budget Start
2000-01-01
Budget End
2000-12-31
Support Year
5
Fiscal Year
2000
Total Cost
$251,401
Indirect Cost

  Institution

Name
New York University
Department
Anatomy/Cell Biology
Type
Schools of Medicine
DUNS #
City
New York
State
NY
Country
United States
Zip Code
10016

  Publications

Cailhier, Jean Francois; Sawatzky, Deborah A; Kipari, Tiina et al. (2006) Resident pleural macrophages are key orchestrators of neutrophil recruitment in pleural inflammation. Am J Respir Crit Care Med 173:540-7
Gotoh, N; Ito, M; Yamamoto, S et al. (2004) Tyrosine phosphorylation sites on FRS2alpha responsible for Shp2 recruitment are critical for induction of lens and retina. Proc Natl Acad Sci U S A 101:17144-9
Lang, Richard A (2004) Pathways regulating lens induction in the mouse. Int J Dev Biol 48:783-91
Faber, Sonya C; Robinson, Michael L; Makarenkova, Helen P et al. (2002) Bmp signaling is required for development of primary lens fiber cells. Development 129:3727-37
Lobov, Ivan B; Brooks, Peter C; Lang, Richard A (2002) Angiopoietin-2 displays VEGF-dependent modulation of capillary structure and endothelial cell survival in vivo. Proc Natl Acad Sci U S A 99:11205-10
Faber, S C; Dimanlig, P; Makarenkova, H P et al. (2001) Fgf receptor signaling plays a role in lens induction. Development 128:4425-38
Shirke, S; Faber, S C; Hallem, E et al. (2001) Misexpression of IGF-I in the mouse lens expands the transitional zone and perturbs lens polarization. Mech Dev 101:167-74
Govindarajan, V; Ito, M; Makarenkova, H P et al. (2000) Endogenous and ectopic gland induction by FGF-10. Dev Biol 225:188-200
Makarenkova, H P; Ito, M; Govindarajan, V et al. (2000) FGF10 is an inducer and Pax6 a competence factor for lacrimal gland development. Development 127:2563-72
Chow, R L; Altmann, C R; Lang, R A et al. (1999) Pax6 induces ectopic eyes in a vertebrate. Development 126:4213-22

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