Group X phospholipase A2 is released during sperm acrosome reaction and controls fertility outcome in mice
Jessica Escoffier, … , Gérard Lambeau, Christophe Arnoult
Jessica Escoffier, … , Gérard Lambeau, Christophe Arnoult
Published April 26, 2010
Citation Information: J Clin Invest. 2010;120(5):1415-1428. https://doi.org/10.1172/JCI40494.
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Research Article

Group X phospholipase A2 is released during sperm acrosome reaction and controls fertility outcome in mice

Abstract

Ejaculated mammalian sperm must undergo a maturation process called capacitation before they are able to fertilize an egg. Several studies have suggested a role for members of the secreted phospholipase A2 (sPLA2) family in capacitation, acrosome reaction (AR), and fertilization, but the molecular nature of these enzymes and their specific roles have remained elusive. Here, we have demonstrated that mouse group X sPLA2 (mGX) is the major enzyme present in the acrosome of spermatozoa and that it is released in an active form during capacitation through spontaneous AR. mGX-deficient male mice produced smaller litters than wild-type male siblings when crossed with mGX-deficient females. Further analysis revealed that spermatozoa from mGX-deficient mice exhibited lower rates of spontaneous AR and that this was associated with decreased in vitro fertilization (IVF) efficiency due to a drop in the fertilization potential of the sperm and an increased rate of aborted embryos. Treatment of sperm with sPLA2 inhibitors and antibodies specific for mGX blocked spontaneous AR of wild-type sperm and reduced IVF success. Addition of lysophosphatidylcholine, a catalytic product of mGX, overcame these deficiencies. Finally, recombinant mGX triggered AR and improved IVF outcome. Taken together, our results highlight a paracrine role for mGX during capacitation in which the enzyme primes sperm for efficient fertilization and boosts premature AR of a likely phospholipid-damaged sperm subpopulation to eliminate suboptimal sperm from the pool available for fertilization.

Authors

Jessica Escoffier, Ikram Jemel, Akemi Tanemoto, Yoshitaka Taketomi, Christine Payre, Christelle Coatrieux, Hiroyasu Sato, Kei Yamamoto, Seiko Masuda, Karin Pernet-Gallay, Virginie Pierre, Shuntaro Hara, Makoto Murakami, Michel De Waard, Gérard Lambeau, Christophe Arnoult

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Figure 4

Endogenous and recombinant mGX sPLA2 both regulate spontaneous AR during capacitation.

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Endogenous and recombinant mGX sPLA2 both regulate spontaneous AR during...
(A) Spontaneous AR of mGX–/– sperm does not progress beyond 55 minutes of in vitro capacitation, in contrast to WT sperm. Addition of mGX during the last 10 minutes of 90-minute capacitation rescues normal spontaneous AR in mGX–/– sperm. Spontaneous AR was quantified during capacitation at 10, 55, and 90 minutes in mGX+/+ littermate sperm (n = 11) and mGX–/– sperm (n = 6). (B) Recombinant mGX sPLA2 is a potent inducer of AR. Dose-response curve for AR of noncapacitated WT sperm triggered by mGX (n = 3–8). (C) Treatment with mGX sPLA2 (200 nM) for 10 minutes triggers AR of both noncapacitated WT sperm (23.7% ± 1.4% to 68.1% ± 2.1% for control and mGX-treated sperm, respectively; n = 23) and WT sperm capacitated for 90 minutes (46.5% ± 6.3% to 81.8% ± 5.4% for control and mGX-treated sperm, respectively; n = 3).