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Abstract
In the course of mammalian spermiogenesis, a unique
chromatin remodeling process takes place within elongating
and condensing spermatid nuclei. The histone-to-protamine
exchange results in efficient packaging and increased
stability of the paternal genome. Although not fully
understood, this change in chromatin architecture must
require a global but transient appearance of endogenous
DNA strand breaks since most of DNA supercoiling is
eliminated in the mature sperm. To establish the extent of
DNA strand breakage and the stage-specificity at which
these breaks are created and repaired, we performed a
sensitive terminal deoxynucleotidyl transferase
(TdT)-mediated dUTP nick-end labeling (TUNEL) assay to
detect in situ DNA strand breaks on both mice and human
testis cross sections. In the mouse, we established that
DNA strand breaks are indeed detected in the whole
population of elongating spermatids between stages IX and
XI of the seminiferous epithelium cycle perfectly
coincident with the chromatin remodeling as revealed by
histone H4 hyperacetylation. Similarly, TUNEL analyses
performed on human testis sections revealed an elevated
and global increase in the levels of DNA strand breaks
present in nuclei of round-shaped spermatids also
coincident with chromatin remodeling. The demonstration
of the global character of the transient DNA strand breaks
in mammalian spermiogenesis suggests that deleterious
consequences on genetic integrity of the male gamete may
arise from any disturbance in the process. In addition,
this investigation may shed some light on the origin of
the low success rate that has been encountered so far with
intracytoplasmic injection procedures making use of round
spermatids in humans.
Key words:
Gamete Biology
Gametogenesis
Sperm maturation
Spermatid
Spermatogenesis
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