Mouse and human spermatozoa can be freeze-dried without damaging their chromosomes

doi:10.1093/humrep/dem252

Hum. Reprod. Advance Access originally published online on December 1, 2007
Human Reproduction 2008 23(2):233-239; doi:10.1093/humrep/dem252

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© The Author 2007. Published by Oxford University Press on behalf of the European Society of Human Reproduction and Embryology. All rights reserved. For Permissions, please email: journals.permissions@oxfordjournals.org

Mouse and human spermatozoa can be freeze-dried without damaging their chromosomes

H. Kusakabe¹^,3, R. Yanagimachi² and Y. Kamiguchi¹

¹ Department of Biological Sciences, Asahikawa Medical College, 2-1-1-1 Midorigaoka-higashi, Asahikawa 078-8510, Japan ² Institute for Biogenesis Research, University of Hawaii Medical School, 1960 East-West Road, Honolulu, Hawaii 96822, USA

³ Correspondence address. E-mail: hkusa55{at}asahikawa-med.ac.jp

BACKGROUND: Although mouse spermatozoa can be freeze-dried without losingtheir reproductive capacity, the technique needs further improvementsto reduce the incidence of chromosomal damage to spermatozoa.Effects of freeze-drying on human spermatozoa are unknown.

METHODS: Mouse spermatozoa were suspended in a Tris-buffered EGTA solutionbriefly (10 min at 37°C) or for 1–7 days at 4°Cbefore freeze-drying. Freeze-dried spermatozoa were maintainedfor up to 1 year at 4°C before injection. Sperm chromosomeswere examined during the first mitosis (cleavage) of zygotes.The ability of sperm to support embryo development was assessedby examining mid-gestation fetuses (Day 14) after transfer of2-cell embryos to surrogate mothers. Chromosome integrity offreeze-dried human spermatozoa was examined by injecting individualspermatozoa into mouse oocytes which were previously enucleated.

RESULTS: When mouse spermatozoa were freeze-dried immediately after suspensionin Tris-buffered EGTA solution, only c.40% had normal chromosomes.When the mouse spermatozoa were kept in the same solution for3–7 days before freeze-drying, 85–95% had normalchromosomes and they were able to support embryo developmentbetter than those which were in the solution briefly (P <0.05). Freeze-dried human spermatozoa well maintained theirchromosomes regardless of the duration of pre-freeze-dryingincubation of spermatozoa in the Tris-buffered EGTA solution.

CONCLUSIONS: Prior incubation of mouse spermatozoa in Tris-buffered EGTAsolution for several days makes sperm chromosomes more resistantto freeze-drying. As the consequence, spermatozoa freeze-driedthis way support embryo development better than those exposedto Tris-buffered EGTA solution only briefly. Freeze-dried humanspermatozoa well maintained their chromosomes without pre-freeze-dryingincubation in Tris-buffered EGTA solution.

Key words: ICSI/freeze-drying/human sperm/mouse sperm/chromosome

Submitted on January 9, 2007; resubmitted on June 28, 2007; accepted on July 11, 2007.

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