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用针对小鼠透明带糖蛋白2(mZP2)和小鼠透明带糖蛋白3(mZP3)的表位标记互补DNA(cDNA)显微注射生长中的小鼠卵母细胞后,其透明带糖蛋白的分泌与组装。

Secretion and assembly of zona pellucida glycoproteins by growing mouse oocytes microinjected with epitope-tagged cDNAs for mZP2 and mZP3.

作者信息

Qi Huayu, Williams Zev, Wassarman Paul M

机构信息

Department of Biochemistry and Molecular Biology, Mount Sinai School of Medicine, New York, New York 10029-6574, USA.

出版信息

Mol Biol Cell. 2002 Feb;13(2):530-41. doi: 10.1091/mbc.01-09-0440.

Abstract

The zona pellucida (ZP) is a highly organized extracellular coat that surrounds all mammalian eggs. The mouse egg ZP is composed of three glycoproteins, called mZP1-3, that are synthesized, secreted, and assembled into a ZP exclusively by growing oocytes. Here, we microinjected epitope-tagged (Myc and Flag) cDNAs for mZP2 and mZP3 into the germinal vesicle (nucleus) of growing oocytes isolated from juvenile mice. Specific antibodies and laser scanning confocal microscopy were used to follow nascent, recombinant ZP glycoproteins in both permeabilized and nonpermeabilized oocytes. When such cDNAs were injected, epitope-tagged mZP2 (Myc-mZP2) and mZP3 (Flag-mZP3) were synthesized, packaged into large intracellular vesicles, and secreted by the vast majority of oocytes. Secreted glycoproteins were incorporated into only the innermost layer of the thickening ZP, and the amount of nascent glycoprotein in this region increased with increasing time of oocyte culture. Consistent with prior observations, the putative transmembrane domain at the C terminus of mZP2 and mZP3 was missing from nascent glycoprotein incorporated into the ZP. When the consensus furin cleavage site near the C terminus of mZP3 was mutated, such that it should not be cleaved by furin, secretion and assembly of mZP3 was reduced. On the other hand, mZP3 incorporated into the ZP lacked the transmembrane domain downstream of the mutated furin cleavage site, suggesting that some other protease(s) excised the domain. These results strongly suggest that nascent mZP2 and mZP3 are incorporated into only the innermost layer of the ZP and that excision of the C-terminal region of the glycoproteins is required for assembly into the oocyte ZP.

摘要

透明带(ZP)是一种高度有序的细胞外被膜,包裹着所有哺乳动物的卵子。小鼠卵子的透明带由三种糖蛋白组成,称为mZP1 - 3,它们由生长中的卵母细胞专门合成、分泌并组装成透明带。在这里,我们将带有表位标签(Myc和Flag)的mZP2和mZP3的cDNA显微注射到从幼年小鼠分离出的生长中卵母细胞的生发泡(细胞核)中。使用特异性抗体和激光扫描共聚焦显微镜追踪通透和未通透卵母细胞中新生的重组透明带糖蛋白。当注射此类cDNA时,带有表位标签的mZP2(Myc - mZP2)和mZP3(Flag - mZP3)被合成,包装到大型细胞内囊泡中,并被绝大多数卵母细胞分泌。分泌的糖蛋白仅整合到增厚透明带的最内层,并且该区域新生糖蛋白的量随着卵母细胞培养时间的增加而增加。与先前的观察结果一致,整合到透明带中的新生糖蛋白中缺少mZP2和mZP3 C末端的推定跨膜结构域。当mZP3 C末端附近的共有弗林蛋白酶切割位点发生突变,使其不应被弗林蛋白酶切割时,mZP3的分泌和组装减少。另一方面,整合到透明带中的mZP3缺少突变的弗林蛋白酶切割位点下游的跨膜结构域,这表明其他一些蛋白酶切除了该结构域。这些结果强烈表明,新生的mZP2和mZP3仅整合到透明带的最内层中,并且糖蛋白C末端区域的切除是组装到卵母细胞透明带中所必需的。

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