Abstract

The ultimate goal of this proposal is to identify, characterize, and study the function of genes involved in critical steps in early mammalian development. Initially, we will focus our attention on the Evx-1 gene, a mouse cognate of the Drosophila homeobox-containing even- skipped gene. Based on the observation that Evx-1 is expressed in a gradient in the primitive streak, we have hypothesized that Evx-1 functions in a dose-dependent fashion to provide dorso-ventral patterning of the newly formed mesoderm. To test this hypothesis we will determine the consequences of expressing Evx-1 RNA at high levels throughout the primitive streak, thereby ablating the gradient of Evx-1 RNA that is normally observed. We will also determine the consequences of ablating Evx-1 gene function, by creating embryos homozygous for a null allele of Evx-I. In addition, we will identify the genomic sequences that determine the tissue-specificity of Evx-1 expression in the developing embryo. A second major goal is to identify and isolate the gene encoding a molecule, VE-1, that is expressed in the visceral endoderm overlying the future anterior region of the embryo during the early post-implantation stages of development. Our long-term goal is to determine the function of this earliest known marker of A-P polarity in mouse embryogenesis. In the course of pursuing these experiments, we propose to test the efficacy of a new method (the cre/lox """"""""binary"""""""" transgenic mouse system) based on DNA recombination for manipulating gene expression in vivo. In these experiments the desired effect, e.g. ectopic gene expression, is achieved by mating mice of two different transgenic strains. One (the """"""""target"""""""" mouse) carries a target transgene that is innocuous but has the potential to cause the desired effect, and the other (the """"""""effector"""""""" mouse) carries a DNA recombinase capable of altering the target transgene so that it can produce the desired effect. Because the target transgene has no effect prior to recombination, and the effector (DNA recombinase) alone has no phenotype, both target and effector mice are normal. However, in offspring that inherit both transgenes the target transgene is altered by the effector, producing the desired phenotype. Specifically, the system we propose to test employs the cre gene of bacteriophage P1 as the effector. If this approach is successful, we propose further experiments aimed at increasing its versatility, by generating a standard target mouse strain that can be used with a variable effector strain to produce a new lineage map of the mouse, based on gene expression rather than anatomical position. We hope that in the long-term these experiments will not only lead to greater insights into the basic mechanisms controlling embryonic development, but will make a contribution towards the development of a new genre of transgenic mouse technology.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
Eunice Kennedy Shriver National Institute of Child Health & Human Development (NICHD)
Type
Research Project (R01)
Project #
5R01HD025331-09
Application #
2378509
Study Section
Human Embryology and Development Subcommittee 1 (HED)
Project Start
1989-06-01
Project End
1999-02-28
Budget Start
1997-03-01
Budget End
1998-02-28
Support Year
9
Fiscal Year
1997
Total Cost
Indirect Cost

  Institution

Name
University of California San Francisco
Department
Anatomy/Cell Biology
Type
Schools of Medicine
DUNS #
073133571
City
San Francisco
State
CA
Country
United States
Zip Code
94143

  Publications

Chi, Neil C; Bussen, Markus; Brand-Arzamendi, Koroboshka et al. (2010) Cardiac conduction is required to preserve cardiac chamber morphology. Proc Natl Acad Sci U S A 107:14662-7
Ishimura, Ryuta; Martin, Gail R; Ackerman, Susan L (2008) Loss of apoptosis-inducing factor results in cell-type-specific neurogenesis defects. J Neurosci 28:4938-48
Storm, Elaine E; Garel, Sonia; Borello, Ugo et al. (2006) Dose-dependent functions of Fgf8 in regulating telencephalic patterning centers. Development 133:1831-44
Grieshammer, Uta; Le Ma; Plump, Andrew S et al. (2004) SLIT2-mediated ROBO2 signaling restricts kidney induction to a single site. Dev Cell 6:709-17
Chi, Candace L; Martinez, Salvador; Wurst, Wolfgang et al. (2003) The isthmic organizer signal FGF8 is required for cell survival in the prospective midbrain and cerebellum. Development 130:2633-44
Goldman, D C; Martin, G R; Tam, P P (2000) Fate and function of the ventral ectodermal ridge during mouse tail development. Development 127:2113-23
Grieshammer, U; Lewandoski, M; Prevette, D et al. (1998) Muscle-specific cell ablation conditional upon Cre-mediated DNA recombination in transgenic mice leads to massive spinal and cranial motoneuron loss. Dev Biol 197:234-47
Lewandoski, M; Martin, G R (1997) Cre-mediated chromosome loss in mice. Nat Genet 17:223-5
Rosenquist, T A; Martin, G R (1995) Visceral endoderm-1 (VE-1): an antigen marker that distinguishes anterior from posterior embryonic visceral endoderm in the early post-implantation mouse embryo. Mech Dev 49:117-21
Blanar, M A; Crossley, P H; Peters, K G et al. (1995) Meso1, a basic-helix-loop-helix protein involved in mammalian presomitic mesoderm development. Proc Natl Acad Sci U S A 92:5870-4

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