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Australian Mammalogy Australian Mammalogy Society
Journal of the Australian Mammal Society
RESEARCH ARTICLE

Gamete cryopreservation of Australian ‘old endemic’ rodents – spermatozoa from the plains mouse (Pseudomys australis) and spinifex hopping mouse (Notomys alexis)

Kathrine M. Ferres A B C , Nicole O. McPherson B D E , Michelle Lane B D E F , Hassan W. Bakos B D , Karen L. Kind C and William G. Breed A D G H
+ Author Affiliations
- Author Affiliations

A Discipline of Anatomy and Pathology, Adelaide Medical School, Faculty of Health Sciences, The University of Adelaide, SA 5005, Australia.

B Discipline of Obstetrics and Gynaecology, Adelaide Medical School, Faculty of Health Sciences, The University of Adelaide, SA 5005, Australia.

C School of Animal and Veterinary Sciences, Faculty of Sciences, The University of Adelaide, SA 5005, Australia.

D Robinson Research Institute, University of Adelaide, Adelaide, SA 5005, Australia.

E Freemasons Centre for Men’s Health, The University of Adelaide, SA 5005, Australia.

F Repromed, 180 Fullarton Road, Dulwich, SA 5065, Australia.

G School of Biological Sciences, Faculty of Sciences, The University of Adelaide, SA 5005, Australia.

H Corresponding author. Email: bill.breed@adelaide.edu.au

Australian Mammalogy 40(1) 76-83 https://doi.org/10.1071/AM16055
Submitted: 20 November 2016  Accepted: 6 April 2017   Published: 7 July 2017

Abstract

Most of the Australian ‘old endemic’ rodents have greatly reduced distributions with several species now threatened with extinction. Application of assisted reproductive technology has the potential to assist in their conservation programs in at least a few species. Here we describe an attempt to cryopreserve spermatozoa from two of these species – those of the plains mouse (Pseudomys australis) and spinifex hopping mouse (Notomys alexis), which have dramatic differences in sperm morphology. Slow and rapid freezing and three different cryoprotectant media with either raffinose, glycerol and/or skim milk were used and the results compared with those of house mouse sperm, which were used as controls. Sperm morphology, motility, membrane integrity and DNA damage were determined. Prior to cryopreservation there was a higher percentage of morphologically normal, motile, P. australis sperm than in those from N. alexis. Following cryopreservation, regardless of treatment, the percentage of motile sperm was low but it was higher when raffinose with skim milk was used as a cryoprotectant than in raffinose with glycerol albeit that minimal differences in membrane integrity or DNA damage were evident. Raffinose with skim milk should thus be used as a cryoprotectant for storing sperm of these Australian rodents in the future.

Additional keywords: cryostorage, hydromyine rodents, male gamete.


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