Abstract

Sperm cells are exposed to many different environments in both male and female reproductive tracts. To function in disparate milieus, sperm have evolved into highly polarized, multifunctional cells whose surface is comprised of several large domains. Much of this membrane polarization occurs as sperm pass through the epididymis. For example, while in the epididymis, the plasma membrane surrounding the sperm head polarizes several proteins into either the posterior (PHD) or anterior (AHD) head domain. In many somatic cell systems, membrane polarization precedes a change in the cellular function. Thus redistribution of sperm proteins may be an important prerequisite for functional development of sperm seen in the epididymis. Likewise, maintaining a polarized membrane is critical if these functions are to continue. We are interested in understanding the molecular mechanisms that enable sperm to maintain a polarized membrane. To study this, we have focused on the transmembrane protein fertilin. Fertilin is found distributed over the whole head of testicular sperm. But on sperm that have moved through the epididymis (cauda sperm), it is only found in the PHD. We examined how fertilin is retained within the whole head domain of testicular sperm, and on just the PHD of cauda sperm. Using fluorescence redistribution after photobleaching (FRAP) analysis, we found fertilin is highly restricted from moving within the lipid bilayer of both testicular and cauda sperm, and thus does not diffuse out of these domains. However, when we examined capacitated cauda sperm or acrosome-reacted cauda sperm, fertilin was highly mobile, yet still retained within the PHD. In this proposal we have designed experiments to try answering the following: 1) What is the mechanism(s) responsible for restricting fertilin's diffusion in PHD of cauda sperm? 2) What is the signal during capacitation that causes fertilin to become mobile within the membrane? 3) Is fertilin physically modified during capacitation and/or the acrosome reaction, and if so how? We anticipate these studies will advance understanding of the sperm's cellular architecture and its relationship to cellular function. Information gained may also lead to development of novel male contraceptives and/or treatments for infertility.

  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 #
5R01HD038807-04
Application #
6893368
Study Section
Reproductive Biology Study Section (REB)
Program Officer
Rankin, Tracy L
Project Start
2002-07-01
Project End
2007-06-30
Budget Start
2005-07-01
Budget End
2006-06-30
Support Year
4
Fiscal Year
2005
Total Cost
$265,734
Indirect Cost

  Institution

Name
Population Council
Department
Type
DUNS #
071050090
City
New York
State
NY
Country
United States
Zip Code
10017

  Publications

Kwitny, Susanna; Klaus, Angela V; Hunnicutt, Gary R (2010) The annulus of the mouse sperm tail is required to establish a membrane diffusion barrier that is engaged during the late steps of spermiogenesis. Biol Reprod 82:669-78
Hunnicutt, Gary R; Koppel, Dennis E; Kwitny, Susanna et al. (2008) Cyclic 3',5'-AMP causes ADAM1/ADAM2 to rapidly diffuse within the plasma membrane of guinea pig sperm. Biol Reprod 79:999-1007
Selvaraj, Vimal; Buttke, Danielle E; Asano, Atsushi et al. (2007) GM1 dynamics as a marker for membrane changes associated with the process of capacitation in murine and bovine spermatozoa. J Androl 28:588-99
Buttke, Danielle E; Nelson, Jacquelyn L; Schlegel, Peter N et al. (2006) Visualization of GM1 with cholera toxin B in live epididymal versus ejaculated bull, mouse, and human spermatozoa. Biol Reprod 74:889-95
Kissel, Holger; Georgescu, Maria-Magdalena; Larisch, Sarit et al. (2005) The Sept4 septin locus is required for sperm terminal differentiation in mice. Dev Cell 8:353-64