The long-term goal of these studies if to determine how the survival
of spermatogenic cells is regulated by the Bcl-2 family of onoproteins.
Although the potential exists for multiple influences on the regulation
of mitotic events in the proliferating germ cells, a significant body of
data has established a correlation between the size of the
spermatogenic compartment and the number of early germ ells that do
not survive to the haploid stage. We recently identified bcl-x as a
member of the bcl-2 family of oncogenes preferentially expressed in
the rat testis. Studies in this proposal concentrate on the regulation
of the expression of two protein isoforms, Bcl-xL and Bcl-xS, and
their roles in determining survival versus death of germ cells. Our
studies will focus on the unique features of bcl-x expression in the
seminiferous tubule. First, the bcl-x gene will be cloned and potential
regulatory elements identified in its proximal promoter by DNA
sequence analysis. Second, the specific regulation of the isolforms of
bcl-x mRNA by androgens and stem cell growth factor will be
evaluated using primary culture models of highly purified
spermatogonia and early spermatocytes. Third, the stage specificity of
bcl-x expression in the seminiferous tubule will be determined and the
effects of stem cell factor and androgens on bcl-x expression and DNA
synthesis in premeiotic germ cells ascertained. Fourth, the effects of
changes in the ratio of the members of the Bcl-2 family of
oncoproteins on programmed cell death in spermatogonia will be
examined. Specific alterations in the balance of suppression versus
induction of cell death will be accomplished by specific inhibition of
Bcl-xL mRNA using an antisense oligonucleotide approach and by
overexpression of Bcl-2 in transfected germ cells. Characterization of
germ cell development and apoptotic processes in the bcl-2 transgenic
mouse will facilitate studies to delineate the role of the bcl-2 family of
genes in the survival of the male germ cells. Since testicular
biopsies rom infertile males often show decreased numbers of
proliferating and developing germ cells, we anticipate that this
research will lead to significant new data on the relevance of
apoptosis and its regulation to human male fertility.
Eunice Kennedy Shriver National Institute of Child Health and Human Development
CFDA Code
DUNS Number
071050090
UEI
WKTLM8NNXDW1
Project Start Date
01-April-2001
Project End Date
31-March-2003
Budget Start Date
Budget End Date
Project Funding Information for 2001
Total Funding
$174,159
Direct Costs
$174,159
Indirect Costs
Year
Funding IC
FY Total Cost by IC
2001
Eunice Kennedy Shriver National Institute of Child Health and Human Development
$174,159
Year
Funding IC
FY Total Cost by IC
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