Les transporteurs selectifs de cholesterol SR-BI, SR-BII, CD36 et ABCA1 contribuent au maintien de l'homeostasie du cholesterol intratesticulaire.

摘要

The testis is made up of loops of convoluted seminiferous tubules surrounded by interstitial tissue composed of loose connective tissue containing Leydig cells that secrete testosterone into the bloodstream. The seminiferous tubules are lined with a stratified epithelium containing germ cells at various stages of development and the supporting Sertoli cells. Cholesterol is present in both compartments and is crucial for the development of germ cells, the fertility of spermatozoa as well as for testosterone production. In the interstitial compartment, approximately 40% of the cholesterol used for the hormonal production is imported from blood lipoproteins HDL and LDL. In the seminiferous epithelium, Sertoli cells plays key role in the development and maintenance of spermatogenesis. Sertoli cells have the capacity to synthesize cholesterol from acetate in vitro, however, there is no evidence that they do so in vivo. In addition, there is a blood-testis barrier within the seminiferous tubules that prevents the free passage of several blood compounds including cholesterol. We tested the hypothesis that there are ways of blood cholesterol uptake, but also the intratubular cholesterol efflux that by-pass this barrier and contribute to the cholesterol homeostasis within the tubules. We compared expression patterns of the mRNA and proteins for selective cholesterol transporters SR-BI, SR-BII, CD36 and ABCA1 with those of free and esterified cholesterol during the spermatogenesis in normal mice during the postnatal development. To better appreciate the level of involvement of each receptor, we examined the effect of the deletion of the genes for an enzyme (HSL) or for cholesterol transporters (SR-BI, CD36 or NPC1) on the rate of free and esterified cholesterol in both compartments of the testis. At first, we worked out a new technique to separate the testes into interstitial tissue- (ITf) and seminiferous tubule-enriched fractions (STf) that has the advantage of allowing a more faithful detection of the phosphorylated and glycosylated forms of the proteins compared to existing techniques. Our results showed that the expression of SR-BI and CD36 was maximum in the ITf when mice completed their sexual maturity and reached the peak level of testosterone synthesis. In the seminiferous tubule-enriched fractions, the maximum level of SR-BI expression coincided with the highest level of esterified cholesterol during the development at 35 days, as the first wave of the spermatogenetic activity was completed. ABCA1 reached the highest expression level when cholesterol was high and reached the lowest when cholesterol was at its minimum, while the level of CD36 expression was maximal in the adult tubules as the rate of spermiation was the highest. The knockout of the HSL and NPC1, which renders the male mice infertile, was accompanied by the accumulation of free and esterified cholesterol in the seminiferous tubules. On the other hand, the knockout of SR-BI and CD36, linkes to infertility, did not affect the rate of intratubular cholesterol. Here we showed that genetic withdrawal of a cholesterol transporter or of an enzyme involved in cholesterol metabolism was compensated by other transporters or enzymes in order to maintain the level of free cholesterol similar to those measured in the tissue-enriched fractions of wild-type mice. Together, our results showed that the expression of the selective cholesterol transporters SR-BI, SR-BII, CD36 and ABCA1 varied according to the spermatogenesis and intratesticular cholesterol rate, thus suggesting their contribution to the preservation of the intratesticular cholesterol homeostasis.;Keywords: Cholesterol, selective cholesterol transporter, seminiferous tubules, interstitial tissue, spermatogenesis, normal mice, knockout mice.