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小鼠皮质颗粒蛋白p75在卵母细胞生长和成熟过程中的合成时间模式。

Temporal pattern of synthesis of the mouse cortical granule protein, p75, during oocyte growth and maturation.

作者信息

Pierce K E, Grunvald E L, Schultz R M, Kopf G S

机构信息

Department of Biology, University of Pennsylvania, Philadelphia 19104.

出版信息

Dev Biol. 1992 Jul;152(1):145-51. doi: 10.1016/0012-1606(92)90164-c.

Abstract

We previously demonstrated that a protein of M(r) 75,000 (p75) is localized to cortical granules (CGs) in mouse oocytes and eggs and is released upon activation or fertilization of eggs (K.E. Pierce, M. C. Siebert, G. S. Kopf, R. M. Schultz, and P. G. Calarco, 1990, Dev. Biol. 141, 381-392). To examine the temporal pattern of synthesis of p75 during the early stages of CG formation, growing oocytes, which were isolated from juvenile mice, were incubated for 4 hr in medium containing [35S]methionine, and radiolabeled proteins were immunoprecipitated using an antiserum that detects p75. Synthesis of p75 is detected at low levels in the smallest oocytes examined (less than 20 microns). Synthesis of p75 relative to total protein synthesis increases about 12-fold during oocyte growth from the 20-40 microns size and then remains constant throughout the remaining period of oocyte growth (40-70 microns). In the fully grown, germinal vesicle (GV)-intact oocyte (70-80 microns), immunoprecipitated p75 comprises approximately 1.5% of the total amount of radiolabeled protein. Three hours after the transfer of these oocytes to a medium that supports resumption of meiosis and GV breakdown in vitro, oocytes subjected to a 1-hr labeling pulse display a 35% decrease in the relative level of p75 synthesis. By 15 hr of maturation, p75 synthesis was reduced to 14% of that in the fully grown, GV-intact oocyte and this is similar to the level of p75 synthesis in ovulated eggs. The level of p75 synthesis following in vitro translation of total egg RNA is only 38% lower than that obtained from total oocyte RNA. In addition, synthesis of p75 is observed following in vitro translation of oocyte, but not egg, poly(A)+ RNA. These results are consistent with p75 synthesis during oocyte maturation being under translational control.

摘要

我们先前证明,一种分子量为75,000的蛋白质(p75)定位于小鼠卵母细胞和卵子的皮质颗粒(CGs)中,并在卵子激活或受精时释放(K.E.皮尔斯、M.C.西伯特、G.S.科普夫、R.M.舒尔茨和P.G.卡拉尔科,1990年,《发育生物学》141卷,第381 - 392页)。为了研究在CG形成早期p75的合成时间模式,从幼年小鼠分离出的生长中的卵母细胞在含有[35S]甲硫氨酸的培养基中孵育4小时,然后使用检测p75的抗血清对放射性标记的蛋白质进行免疫沉淀。在检测到的最小的卵母细胞(小于20微米)中,p75的合成水平较低。从20 - 40微米大小的卵母细胞生长过程中,相对于总蛋白质合成,p75的合成增加约12倍,然后在卵母细胞生长的剩余阶段(40 - 70微米)保持恒定。在完全成熟、生发泡(GV)完整的卵母细胞(70 - 80微米)中,免疫沉淀的p75约占放射性标记蛋白质总量的1.5%。将这些卵母细胞转移到支持体外减数分裂恢复和GV破裂的培养基中3小时后,接受1小时标记脉冲的卵母细胞中p75合成的相对水平下降了35%。到成熟15小时时,p75合成降至完全成熟、GV完整的卵母细胞中的14%,这与排卵卵子中p75的合成水平相似。从总卵子RNA进行体外翻译后p75的合成水平仅比从总卵母细胞RNA获得的水平低38%。此外,在卵母细胞而非卵子的多聚腺苷酸(poly(A)+)RNA进行体外翻译后观察到了p75的合成。这些结果与卵母细胞成熟过程中p75的合成受翻译控制一致。

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