In this study our aim was to characterise the presence and the role of DNA alterations during sperm decondensation in the mouse. To visualise the changes during decondensation we investigated for the presence of DNase I hypersensitive sites in situ and for a putative role for topoisomerase II by examining the effect of teniposide, a topoisomerase II inhibitor, during fertilisation. In situ nick translation without the previous addition of DNase I failed to reveal the presence of endogenous nicks in decondensing sperm and pronuclei whereas preincubation of fixed oocytes with DNase I indicated that decondensing sperm were sensitive to this enzyme. Addition of 100 mu M teniposide did not completely inhibit pronuclei formation but its addition to the fertilisation medium did lead to the presence of endogenous DNA nicks in decondensing sperm. These observations suggest that DNase I hypersensitivity during sperm decondensation is related to the dramatic conformational changes that the chromatin undergoes during the decondensation process, in which topoisomerase II may be implicated.

Sperm decondensation during fertilization in the mouse: presence of DNaseI hypersensitive sites in situ and a putative role for topoisomerase II / Bizzaro, D; Manicardi, Gian Carlo; Bianchi, P. G.; Sakkas, D.. - In: ZYGOTE. - ISSN 0967-1994. - STAMPA. - 8:(2000), pp. 197-202.

Sperm decondensation during fertilization in the mouse: presence of DNaseI hypersensitive sites in situ and a putative role for topoisomerase II.

MANICARDI, Gian Carlo;
2000

Abstract

In this study our aim was to characterise the presence and the role of DNA alterations during sperm decondensation in the mouse. To visualise the changes during decondensation we investigated for the presence of DNase I hypersensitive sites in situ and for a putative role for topoisomerase II by examining the effect of teniposide, a topoisomerase II inhibitor, during fertilisation. In situ nick translation without the previous addition of DNase I failed to reveal the presence of endogenous nicks in decondensing sperm and pronuclei whereas preincubation of fixed oocytes with DNase I indicated that decondensing sperm were sensitive to this enzyme. Addition of 100 mu M teniposide did not completely inhibit pronuclei formation but its addition to the fertilisation medium did lead to the presence of endogenous DNA nicks in decondensing sperm. These observations suggest that DNase I hypersensitivity during sperm decondensation is related to the dramatic conformational changes that the chromatin undergoes during the decondensation process, in which topoisomerase II may be implicated.
8
197
202
Sperm decondensation during fertilization in the mouse: presence of DNaseI hypersensitive sites in situ and a putative role for topoisomerase II / Bizzaro, D; Manicardi, Gian Carlo; Bianchi, P. G.; Sakkas, D.. - In: ZYGOTE. - ISSN 0967-1994. - STAMPA. - 8:(2000), pp. 197-202.
Bizzaro, D; Manicardi, Gian Carlo; Bianchi, P. G.; Sakkas, D.
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/11380/455158
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