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Head area measurements of dead, live, X- and Y-bearing bovine spermatozoa
T.
Révay A E,
S.
Nagy B,
A.
Kovács B,
M. E.
Edvi A,
A.
Hidas A,
W.
Rens C,
I.
Gustavsson D
A
Institute for Small Animal Research, Godollo, H-2100, POB 417, Hungary.
B
Research Institute for Animal Breeding and Nutrition, Department of Cell Biology, H-2053 Herceghalom, Gesztenyes u. 1, Hungary.
C
University of Cambridge, Department of Clinical Veterinary Medicine, Madingley Road, Cambridge CB3 OES, UK.
D
Swedish University of Agricultural Sciences, Department of Animal Breeding and Genetics, Centre of Reproductive Biology, Uppsala, Sweden.
E
To whom correspondence should be addressed. email: revay@katki.hu
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Reproduction, Fertility and Development 16(7) 681–687 http://dx.doi.org/10.1071/RD04013
Submitted: 25 February 2004
Accepted: 20 September 2004
Published online: 9 December 2004
Abstract
The head area of bull spermatozoa was measured after viability and acrosome staining using trypan blue and Giemsa stains, followed by X- and Y-chromosome-specific fluorescence in situ hybridisation (FISH). The former staining made possible the categorisation of cells according to morphology and membrane integrity, whereas the latter allowed distinction of spermatozoa bearing X- and Y-chromosomes. Individual spermatozoa could be followed during the consecutive steps of staining, measurement and FISH. Using a high-resolution digital imaging system and measurement software, the head area of more than 3000 cells of five bulls was determined precisely. In all bulls, morphologically normal, viable cells with intact acrosomes were significantly smaller than dead cells with damaged acrosomes. No significant difference in the head area between X- and Y-chromosome-bearing viable, acrosome-intact spermatozoa was found in individual bulls. However, significant between-bull differences were detected in all cell categories.
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