Abstract

The number of genetically engineered strains of mice is increasing at an exponential rate, creating a critical need for improved, cost-effective methods to store and archive these mouse strains. Use of cryopreserved spermatozoa would provide such a method. However, although mouse spermatozoa were """"""""successfully"""""""" frozen in 1990, the fundamental cryobiological factors that affect the ability of spermatozoa to participate in fertilization after freezing-thawing remain largely unknown. Current methods used to cryopreserve murine spermatozoa result in less than about 5% to 10% cryosurvival. This causes a reduction in efficiency (more sperm used per insemination) and/or efficacy (suboptimal pregnancy rates). The thesis of this application is that an understanding of the fundamental data with murine sperm have provided basic information regarding permeability and osmotic and mechanical properties of these cells. Knowledge of the water and cryoprotectant permeability is needed to predict the optimal values for major steps involved in cryopreservation. From the cryoprotectant permeability coefficient, the optimum procedure for adding and removing the cryoprotectant can be determined. Knowledge of cell water permeability and its temperature coefficient allows determination of the cooling rate that is low enough to preclude lethal intracellular freezing. Knowledge of mechanical sensitivity is required to take steps to circumvent it. The experimental approach proposed is to: a) perform experiments to determine effects of extender components on osmotic tolerance limits of murine sperm; b) use the permeability values of mouse sperm to water and various cryoprotectant solutes, to predict optimum conditions for adding and removing cryoprotectants and to optimize the cooling and thawing rate; c) develop an optimal cryopreservation procedure based on these fundamental biophysical properties; and d) experimentally test these predictions through in vitro fertilization and embryo transfer. Information gained from these experiments should aid in defining and minimizing loss of sperm function after cryopreservation, and provide a foundation for improvement in breeding efficiency when using frozen semen.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Center for Research Resources (NCRR)
Type
Resource-Related Research Projects (R24)
Project #
1R24RR013194-01
Application #
2595718
Study Section
National Center for Research Resources Initial Review Group (RIRG)
Project Start
1998-04-15
Project End
1998-06-30
Budget Start
1998-04-15
Budget End
1998-06-30
Support Year
1
Fiscal Year
1998
Total Cost
Indirect Cost

  Institution

Name
Purdue University
Department
Engineering (All Types)
Type
Schools of Engineering
DUNS #
072051394
City
West Lafayette
State
IN
Country
United States
Zip Code
47907

  Publications

Walters, Eric M; Bauer, Beth A; Franklin, Craig L et al. (2009) Mutational insertion of a ROSA26-EGFP transgene leads to defects in spermiogenesis and male infertility in mice. Comp Med 59:545-52
Jiao, Anjun; Han, Xu; Critser, John K et al. (2006) Numerical investigations of transient heat transfer characteristics and vitrification tendencies in ultra-fast cell cooling processes. Cryobiology 52:386-92
Benson, James D; Chicone, Carmen C; Critser, John K (2005) Exact solutions of a two parameter flux model and cryobiological applications. Cryobiology 50:308-16
Walters, Eric M; Men, Hongsheng; Agca, Yuksel et al. (2005) Osmotic tolerance of mouse spermatozoa from various genetic backgrounds: acrosome integrity, membrane integrity, and maintenance of motility. Cryobiology 50:193-205
Benson, James D; Haidekker, Mark A; Benson, Corinna M K et al. (2005) Mercury free operation of the Coulter counter MultiSizer II sampling stand. Cryobiology 51:344-7
Woods, Erik J; Benson, James D; Agca, Yuksel et al. (2004) Fundamental cryobiology of reproductive cells and tissues. Cryobiology 48:146-56
Koshimoto, Chihiro; Mazur, Peter (2002) Effects of cooling and warming rate to and from -70 degrees C, and effect of further cooling from -70 to -196 degrees C on the motility of mouse spermatozoa. Biol Reprod 66:1477-84
Koshimoto, Chihiro; Mazur, Peter (2002) Effects of warming rate, temperature, and antifreeze proteins on the survival of mouse spermatozoa frozen at an optimal rate. Cryobiology 45:49-59
Koshimoto, Chihiro; Mazur, Peter (2002) The effect of the osmolality of sugar-containing media, the type of sugar, and the mass and molar concentration of sugar on the survival of frozen-thawed mouse sperm. Cryobiology 45:80-90
Agca, Yuksel; Gilmore, Julie; Byers, Michael et al. (2002) Osmotic characteristics of mouse spermatozoa in the presence of extenders and sugars. Biol Reprod 67:1493-501

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