Protein dynamics in sperm surface membrane domains
Project Number5R01HD038807-03
Contact PI/Project LeaderHUNNICUTT, GARY R
Awardee OrganizationPOPULATION COUNCIL
Description
Abstract Text
DESCRIPTION: (provided by applicant) 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.
Public Health Relevance Statement
Data not available.
NIH Spending Category
No NIH Spending Category available.
Project Terms
SDS polyacrylamide gel electrophoresisUrodelaacrosomebiological signal transductionbiophysicscalciumcellular polaritycholesterolcrosslinkcyclic AMPepididymishigh performance liquid chromatographyimmunoprecipitationlipid bilayer membranemass spectrometrymembrane permeabilitymembrane transport proteinsphosphomonoesterasesphosphorylationprotein bindingprotein structure functionsolubilityspermsperm capacitationwestern blottingsyeast two hybrid system
Eunice Kennedy Shriver National Institute of Child Health and Human Development
CFDA Code
865
DUNS Number
071050090
UEI
WKTLM8NNXDW1
Project Start Date
01-July-2002
Project End Date
30-June-2007
Budget Start Date
01-July-2004
Budget End Date
30-June-2005
Project Funding Information for 2004
Total Funding
$265,734
Direct Costs
$157,500
Indirect Costs
$108,234
Year
Funding IC
FY Total Cost by IC
2004
Eunice Kennedy Shriver National Institute of Child Health and Human Development
$265,734
Year
Funding IC
FY Total Cost by IC
Sub Projects
No Sub Projects information available for 5R01HD038807-03
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Clinical Studies
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