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钙对于输卵管液蛋白与牛精子细胞膜结合的重要性。

Importance of calcium for the binding of oviductal fluid proteins to the membranes of bovine spermatozoa.

作者信息

Lapointe S, Sirard M A

机构信息

Département des Sciences Animales, Université Laval, Québec, Canada.

出版信息

Mol Reprod Dev. 1996 Jun;44(2):234-40. doi: 10.1002/(SICI)1098-2795(199606)44:2<234::AID-MRD13>3.0.CO;2-2.

Abstract

Our laboratory has recently shown that in vitro-cultured oviductal cells secrete sperm motility maintaining factor(s). Since the binding of oviductal proteins to spermatozoa (SPZ) has been demonstrated in many species, the motility factor was postulated to bind the membranes of SPZ. Therefore, the current study was performed to evaluate which proteins from in vivo oviductal secretions bind to sperm membranes, to characterize binding conditions, and to evaluate the effect of this binding on sperm survival. Bovine oviducts were dissected, and oviductal cells and fluid were collected by pressing the oviductal tube with a glass slide. This mixture was incubated in Tris-EDTA buffer at 37 degrees C for 30 min, and the cells were washed twice by centrifugation. The supernatant containing oviductal fluid proteins (OFP) was reserved, filtered, frozen (for later motility tests), or lyophilized and labeled with 125I. Frozen-thawed SPZ were incubated either immediately, following capacitation, ionophore-induced acrosome reaction, death by heating, or flagellar removal with labeled OFP for 30 min. The resulting pellet after three washes was dissolved in SDS and submitted to 10% SDS-PAGE. An autoradiogram showed that 72, 66, 39, 38, and 36 kDa proteins bind strongly to the five types of SPZ used, and that this binding is very specific, since unlabeled OFP inhibited binding while serum proteins did not. Furthermore, for 39, 38, and 36 kDa proteins, the presence of calcium in the incubation medium was essential for dose-dependent binding, whereas magnesium was not. Preincubation of SPZ for 30 min at 37 degrees C with oviductal fluid, followed by one wash and 6 hr of incubation in control media, showed that the percentage of motile SPZ is significantly higher (52 +/- 6%) compared with SPZ not preincubated with oviductal fluid (24 +/- 6%; P < 0.01). In summary, a limited number of proteins from oviductal secretions bind to the surface of bovine SPZ only in the presence of calcium, and this binding appears to be important for subsequent sperm viability.

摘要

我们实验室最近发现,体外培养的输卵管细胞会分泌精子活力维持因子。由于在许多物种中都已证实输卵管蛋白与精子(SPZ)存在结合,因此推测活力因子会与SPZ的膜结合。所以,开展了本研究以评估体内输卵管分泌物中的哪些蛋白会与精子膜结合,确定结合条件,并评估这种结合对精子存活的影响。解剖牛的输卵管,用载玻片挤压输卵管收集输卵管细胞和液体。将该混合物在Tris - EDTA缓冲液中于37℃孵育30分钟,然后通过离心洗涤细胞两次。保留含有输卵管液蛋白(OFP)的上清液,过滤、冷冻(用于后续活力测试),或冻干并用125I标记。将冻融后的SPZ立即与标记的OFP孵育,或者在获能、离子载体诱导顶体反应、加热致死或去除鞭毛后孵育30分钟。三次洗涤后得到的沉淀溶解于SDS中,并进行10% SDS - 聚丙烯酰胺凝胶电泳。放射自显影片显示,72、66、39、38和36 kDa的蛋白与所使用的五种类型的SPZ强烈结合,并且这种结合具有高度特异性,因为未标记的OFP会抑制结合,而血清蛋白则不会。此外,对于39、38和36 kDa的蛋白,孵育培养基中钙的存在对于剂量依赖性结合至关重要,而镁并非如此。将SPZ在37℃下与输卵管液预孵育30分钟,然后洗涤一次并在对照培养基中孵育6小时,结果显示,与未用输卵管液预孵育的SPZ(24±6%)相比,有活力的SPZ百分比显著更高(52±6%;P<0.01)。总之,输卵管分泌物中只有有限数量的蛋白仅在有钙存在的情况下与牛SPZ表面结合,并且这种结合似乎对随后的精子活力很重要。

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