Abstract

Although the mouse embryo can be grown successfully from the 2-cell to the blastocyst stage in a defined medium containing BSA, that development is not completely normal. Only certain F1 hybrid embryos can grow from the 1-cell to the blastocyst stage in vitro, most strains exhibiting a 2-cell block to further development. To determine the mechanisms which govern critical developmental events, embryos must be able to be studied and manipulated in vitro. It is therefore imperative that we improve the current level of in vitro culture such that embryos undergo completely parallel development in vivo and in vitro. It is first necessary to establish criteria for normal in vivo embryonic development and compare in vitro grown embryos to these standards. Among the criteria for assessing normal development will be gross morphological appearance, cleavage rates and cell numbers, ability of blastocysts to outgrow in vitro, size of the inner cell mass, normality of biochemical and cellular differentiation and finally ability of the blastocyst to give rise to a normal fetus upon transfer to pseudopregnant females. Once the criteria for normal development have been established, a variety of media will be tested on CF-1 and F1 hybrid embyros to determine the medium which best supports normal embyronic development. The composition of that medium will then be modified by appropriate additions or substitutions (serum, energy sources, growth factors, EDTA). In addition, the environment of the cultures will be modified with respect to gaseous composition, culture dishes and agitation to see if development can be enhanced by these alterations. Co-culture of embryos with other embryos or certain established cell lines will be undertaken. Embryo or cell line conditioned medium will also be tested for its effect on in vitro embryonic development. The in vivo environment of the embryos, the oviductal fluid, will be analyzed by HPLC and atomic absorption. This analysis will be performed on intact oviducts and oviductal segments to see if there are changes in the embryonic environment as the embryos move down the oviduct into the uterus. Peak fractions can be collected by HPLC and used in in vitro reconstitution experiments using defined media.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
Eunice Kennedy Shriver National Institute of Child Health & Human Development (NICHD)
Type
Research Project--Cooperative Agreements (U01)
Project #
1U01HD021942-01
Application #
3552520
Study Section
(SRC)
Project Start
1986-09-01
Project End
1991-08-31
Budget Start
1986-09-01
Budget End
1986-11-30
Support Year
1
Fiscal Year
1986
Total Cost
Indirect Cost

  Institution

Name
Worcester Foundation for Biomedical Research
Department
Type
DUNS #
City
Shrewsbury
State
MA
Country
United States
Zip Code
01545

  Publications

Chatot, C L; Lawry, J R; Germain, B et al. (1997) Analysis of glutaminase activity and RNA expression in preimplantation mouse embryos. Mol Reprod Dev 47:248-54
Chatot, C L; Lewis-Williams, J; Torres, I et al. (1994) One-minute exposure of 4-cell mouse embryos to glucose overcomes morula block in CZB medium. Mol Reprod Dev 37:407-12
Chatot, C L; Lewis, J L; Torres, I et al. (1990) Development of 1-cell embryos from different strains of mice in CZB medium. Biol Reprod 42:432-40
Ziomek, C A; Chatot, C L; Manes, C (1990) Polarization of blastomeres in the cleaving rabbit embryo. J Exp Zool 256:84-91
Chatot, C L; Tasca, R J; Ziomek, C A (1990) Glutamine uptake and utilization by preimplantation mouse embryos in CZB medium. J Reprod Fertil 89:335-46
Chatot, C L; Ziomek, C A; Bavister, B D et al. (1989) An improved culture medium supports development of random-bred 1-cell mouse embryos in vitro. J Reprod Fertil 86:679-88