Published-Ahead-of-Print July 3, 2007, DOI:10.2164/jandrol.107.003350
Journal of Andrology, Vol. 28, No. 6, November/December 2007
Copyright © American Society of Andrology
DOI: 10.2164/jandrol.107.003350
The Relationship Between Sperm Morphology and Chromatin Integrity in the Koala (Phascolarctos cinereus) as Assessed by the Sperm Chromatin Dispersion Test (SCDt)
STEPHEN D. JOHNSTON*,
CARMEN LÓPEZ-FERNÁNDEZ
,
ALTEA GOSÁLBEZ
,
YENGPENG ZEE*,
WILLIAM V. HOLT
,
CAMRYN ALLEN* AND
JAIME GOSÁLVEZ
From the * School of Animal Studies, The
University of Queensland, Gatton, Australia;
Departamento de Biología, Unidad de
Genética, Edificio de Biología, Universidad Autónoma de
Madrid, Madrid, Spain; and the
Institute of
Zoology, Zoological Society of London, Regent's Park, London, United
Kingdom
|
Correspondence to: Dr Stephen Johnston, School of Animal Studies, The
University of Queensland, Gatton 4343, Australia (e-mail:
stevejohnston{at}uqconnect.net). |
Koala (Phascolarctos cinereus) sperm nuclei show a tendency to
swell after cryopreservation, but it is uncertain whether this phenomenon is
associated with DNA fragmentation. In this study, we validated a modified
version of the sperm chromatin dispersion test (SCDt) for use with koala
spermatozoa, which is the first use of the test for a marsupial. Cryopreserved
spermatozoa (multiple straws) from a single koala were used to explore the
relationship between sperm morphology, viability, chromatin dispersion, and
DNA fragmentation. A SCDt prototype kit (Sperm Halomax) was specifically
developed for koala spermatozoa with the use of a lysing solution that did not
contain dithiothreitol. DNA fragmentation of lysed and nonlysed spermatozoa
was examined in microgel slides and validated by means of in situ nick
translation (ISNT). The SCDt was then applied to the analysis of extended and
frozen-thawed semen samples of 3 different koalas. Spermatozoa were classified
into 3 distinct koala sperm morphotypes (KSMs) after the SCDt: 1) KSM-1,
rod-shaped cells with no halo of DNA; 2) KSM-2, rounded nuclei with various
degrees of halo formation about a dense chromatin core; and 3) KSM-3,
rod-shaped or rounded nuclei consisting of an inner chromatin core but with
large dispersed halos of stellar chromatin. Although ISNT after the SCDt did
not label KSM-1, both KSM-2 and KSM-3 stained positively for DNA
fragmentation. ISNT was not able to differentiate between KSM-2 and KSM-3.
Although application of the SCDt to the spermatozoa of another 3 koalas showed
no difference in the percentage of the 3 sperm morphotypes found between
extended and frozen-thawed semen, thawed spermatozoa incubated at 35°C for
2 hours showed an increase in the incidence of KSM-3 and a corresponding
decrease in KSM-2. We propose that KSM-1 and KSM-2 represent nuclei that show
either no, or only limited, sperm DNA fragmentation, respectively. It is
likely that the halos formed around KSM-2 are from DNA that is damaged as part
of the normal processing of the spermatozoa and is a consequence of the lack
of cysteine residues and associated stabilizing disulfide bonds in marsupial
sperm DNA. "True" sperm DNA damage is most likely associated with
KSM-3, which shows a massive dispersion of chromatin similar to that described
in other species. A model of koala sperm chromatin structure is proposed to
explain the behavior of the sperm nuclei after the SCDt. Further studies are
required to determine whether DNA damage found in KSM-2 is indicative of
single-stranded DNA breakage associated with an inherent lack of cysteine
residues in marsupial sperm chromatin. Conversely, it will also be important
to establish whether KSM-3 is caused by an increased incidence of
double-stranded DNA breakage and whether this abnormality is correlated with
impaired fertility as it is in other species.
Key words: DNA damage, marsupial
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Copyright © 2007 by The American Society of Andrology.