Rankin T L, Tsuruta K J, Holland M K, Griswold M D, Orgebin-Crist M C
Department of Cell Biology, Vanderbilt University, Nashville, Tennessee 37232.
Biol Reprod. 1992 May;46(5):747-66. doi: 10.1095/biolreprod46.5.747.
Three murine epididymal secretory proteins have been characterized by their site of synthesis, sperm association, and tissue localization by use of polyclonal antisera and immunochemistry. Mouse epididymal protein 7 (MEP 7) was localized initially within the supranuclear regions of some principal epithelial cells in the proximal corpus while other cells remained unstained. In the mid-proximal corpus, all principal cells and stereocilia were stained, and luminal staining increased from corpus to cauda. Some clear cells in the distal corpus and cauda also showed immunoperoxidase staining. Sequential extraction of caudal spermatozoa indicated that MEP 7 was predominantly loosely associated with spermatozoa and that only a small amount of MEP 7 required detergent to extract it from spermatozoa. Examination of other rodent caudal fluids revealed a related protein in rat caudal fluid of 32 kDa, and amino acid sequence analysis of MEP 7 showed a 68% sequence similarity with rat proteins AEG and D/E. MEP 9 immunolocalized within the cytoplasm of all principal cells of the distal caput. In a transition zone between the distal caput and the corpus, some principal cells were stained while others were not. Distal to the corpus, the principal cell staining gradually decreased. In the distal caput and proximal corpus, large heavily stained droplets associated with spermatozoa were seen in the lumen. The staining intensity of these droplets also decreased from corpus to cauda. The clear cells of the distal corpus and cauda did not stain with the antibody to MEP 9. Sequential extraction of caudal spermatozoa showed that some MEP 9 was extractable under low-salt conditions, whereas extraction with 0.1% Triton X-100 was required to remove all MEP 9, indicating it was firmly associated with spermatozoa. The antibody to MEP 9 cross-reacted with a 25-kDa protein present in rat caudal fluid. MEP 10 was localized within the cytoplasm of the principal cells, the stereocilia, and the lumen of the epididymis at the junction of the distal caput and corpus. In the distal corpus, a large number of clear cells were stained, but very few of these cells stained in the cauda. MEP 10 dissociated completely from caudal spermatozoa under low-salt conditions, indicating that it was not firmly bound to spermatozoa. The antiserum to MEP 10 cross-reacted with proteins present in rat and guinea pig caudal fluid. The related rat protein migrated at approximately 20 kDa. Amino acid sequence analysis of MEP 10 revealed an 86% sequence similarity with rat proteins B and C.(ABSTRACT TRUNCATED AT 400 WORDS)
通过使用多克隆抗血清和免疫化学方法,对三种小鼠附睾分泌蛋白的合成位点、与精子的结合情况以及组织定位进行了表征。小鼠附睾蛋白7(MEP 7)最初定位于近端体部一些主上皮细胞的核上区域,而其他细胞未染色。在近端体部中部,所有主细胞和静纤毛均被染色,管腔染色从体部到尾部逐渐增加。远端体部和尾部的一些透明细胞也显示出免疫过氧化物酶染色。对尾部精子进行顺序提取表明,MEP 7主要与精子松散结合,只有少量MEP 7需要去污剂才能从精子中提取出来。对其他啮齿动物尾部液体的检测发现,大鼠尾部液体中有一种32 kDa的相关蛋白,MEP 7的氨基酸序列分析显示与大鼠蛋白AEG和D/E有68%的序列相似性。MEP 9免疫定位于远端头部所有主细胞的细胞质内。在远端头部和体部之间的过渡区,一些主细胞被染色,而其他细胞未被染色。在体部远端,主细胞染色逐渐减少。在远端头部和近端体部,管腔内可见与精子相关的大量深色大液滴。这些液滴的染色强度也从体部到尾部逐渐降低。远端体部和尾部的透明细胞未被MEP 9抗体染色。对尾部精子进行顺序提取表明,一些MEP 9在低盐条件下可被提取,而用0.1% Triton X-100提取才能去除所有MEP 9,这表明它与精子紧密结合。MEP 9抗体与大鼠尾部液体中存在的一种25 kDa蛋白发生交叉反应。MEP 10定位于远端头部和体部交界处附睾主细胞的细胞质、静纤毛和管腔内。在远端体部,大量透明细胞被染色,但在尾部这些细胞很少被染色。MEP 10在低盐条件下与尾部精子完全解离,表明它没有牢固地结合在精子上。MEP 10抗血清与大鼠和豚鼠尾部液体中存在的蛋白发生交叉反应。相关的大鼠蛋白迁移率约为20 kDa。MEP 10的氨基酸序列分析显示与大鼠蛋白B和C有
