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The nuclear RNA-binding protein Sam68 translocates to the cytoplasm and associates with the polysomes in mouse spermatocytes

机译:核RNA结合蛋白Sam68易位至细胞质,并与小鼠精母细胞中的多核糖体结合

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摘要

Translational control plays a crucial role during gametogenesis in organisms as different as worms and mammals. Mouse knockout models have highlighted the essential function of many RNA-binding proteins during spermatogenesis. Herein we have investigated the expression and function during mammalian male meiosis of Sam68, an RNA-binding protein implicated in several aspects of RNA metabolism. Sam68 expression and localization within the cells is stage specific: it is expressed in the nucleus of spermatogonia, it disappears at the onset of meiosis (leptotene/zygotene stages), and it accumulates again in the nucleus of pachytene spermatocytes and round spermatids. During the meiotic divisions, Sam68 translocates to the cytoplasm where it is found associated with the polysomes. Translocation correlates with serine/ threonine phosphorylation and it is blocked by inhibitors of the mitogen activated protein kinases ERK1/2 and of the maturation promoting factor cyclinB-cdc2 complex. Both kinases associate with Sam68 in pachytene spermatocytes and phosphorylate the regulatory regions upstream and downstream of the Sam68 RNA-binding motif. Molecular cloning of the mRNAs associated with Sam68 in mouse spermatocytes reveals a subset of genes that might be posttranscriptionally regulated by this RNA-binding protein during spermatogenesis. We also demonstrate that Sam68 shuttles between the nucleus and the cytoplasm in secondary spermatocytes, suggesting that it may promote translation of specific RNA targets during the meiotic divisions.
机译:在蠕虫和哺乳动物等不同生物的配子发生过程中,翻译控制起着至关重要的作用。小鼠基因敲除模型突出了精子发生过程中许多RNA结合蛋白的基本功能。在本文中,我们研究了哺乳动物雄性减数分裂过程中Sam68的表达和功能,Sam68是一种涉及RNA代谢几个方面的RNA结合蛋白。 Sam68在细胞内的表达和定位是特定于阶段的:它在精原细胞核中表达,在减数分裂开始时消失(瘦素/合子阶段),并再次在粗精子细胞和圆形精子细胞核中积累。在减数分裂分裂过程中,Sam68易位至细胞质,并与多核糖体相关。易位与丝氨酸/苏氨酸磷酸化相关,并被促分裂原活化蛋白激酶ERK1 / 2和成熟促进因子cyclinB-cdc2复合物的抑制剂所阻断。两种激酶均与粗线精​​子细胞中的Sam68结合并磷酸化Sam68 RNA结合基序上游和下游的调节区。小鼠精母细胞中与Sam68相关的mRNA的分子克隆揭示了在精子发生过程中可能受该RNA结合蛋白转录后调控的基因子集。我们还证明了Sam68在次生精细胞的细胞核和细胞质之间穿梭,提示它可能在减数分裂分裂过程中促进特定RNA靶标的翻译。

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