Analysis and significance of mRNA in human ejaculated sperm from normozoospermic donors: relationship to sperm motility and capacitation

doi:10.1093/molehr/gah064

Mol. Hum. Reprod. Advance Access published online on April 20, 2004
Molecular Human Reproduction, doi:10.1093/molehr/gah064
© 2004 by Oxford University Press

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Received February 17, 2004
Revised March 24, 2004
Accepted March 30, 2004

Article

Analysis and significance of mRNA in human ejaculated sperm from normozoospermic donors: relationship to sperm motility and capacitation

S. Lambard ¹, I. Galeraud-Denis ², G. Martin ³, R. Levy ³, A. Chocat ⁴, S. Carreau ⁵^*

¹ UPRES EA 2608-USC INRA, University of Caen, France
² Department of Genetics and Reproduction, CHRU Clemenceau, Caen 14032 France
³ Laboratory of Reproductive Biology, Hopital Nord, 42055 Saint-Etienne, France
⁴ Department of Genetics and Reproduction, CHRU Clemenceau, Caen 14032 ,France
⁵ UPRES EA 2608-USC INRA, University of Caen,France

^* To whom correspondence should be addressed. E-mail: carreau{at}ibba.unicaen.fr.

Abstract

The existence of a complex population of mRNA in human spermis well documented but their role is not yet elucidated. Usingdiscontinuous density gradients, we have isolated high and lowmotile sperm from the same semen sample. The levels of differenttranscripts coding for molecules either involved in nuclearcondensation (protamines 1 and 2) or in capacitation [endothelialnitric oxide synthase (eNOS), neuronal nitric oxide synthase(nNOS) and c-myc] were then assessed in the two populationsusing semi-quantitative RT-PCR. Sperm viability was estimatedby eosin-nigrosin staining and by hypo-osmotic swelling test;apoptosis percentage was measured by the TdT (terminal deoxynucleotidyltransferase)-mediated dUDP nick-end labelling technique. Thecontamination by somatic and germ cells was assessed by lookingfor specific molecular markers of these cells, respectivelyCD-45 and E-cadherin for somatic cells and c-kit for germ cells.The viability of sperm was unchanged in high and low motilefractions, as well as DNA fragmentation percentage. The amountof Prm-1 mRNA was significantly higher in low density motilethan in the high motile fraction. In most of high motile spermsamples eNOS and nNOS transcripts were undetectable whereasthey were present in the low motile sperm. In contrast, no significantvariation was found in the c-myc/Prm-2 mRNA ratio between thetwo populations. Moreover, a partial or complete disappearanceof c-myc transcripts was observed after capacitation. Thus analysingmRNA profiles could be helpful as a diagnostic tool and prognosisvalue for fertilization.

Key Words: Keywords: capacitation, human, motility, RNA, sperm

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