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Tpr是一种大型卷曲螺旋蛋白,其氨基末端参与致癌激酶的激活,定位于核孔复合体的细胞质表面。

Tpr, a large coiled coil protein whose amino terminus is involved in activation of oncogenic kinases, is localized to the cytoplasmic surface of the nuclear pore complex.

作者信息

Byrd D A, Sweet D J, Panté N, Konstantinov K N, Guan T, Saphire A C, Mitchell P J, Cooper C S, Aebi U, Gerace L

机构信息

Department of Cell Biology, Scripps Research Institute, La Jolla, California 92037.

出版信息

J Cell Biol. 1994 Dec;127(6 Pt 1):1515-26. doi: 10.1083/jcb.127.6.1515.

DOI:10.1083/jcb.127.6.1515
PMID:7798308
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2120283/
Abstract

From a panel of monoclonal antibodies raised against fractions of rat liver nuclear envelopes (NEs), we have identified an antibody, RL30, which reacts with novel nuclear pore complex (NPC) antigens that are not O-glycosylated. By immunofluorescence staining of cultured cells, RL30 reacts exclusively with the NE in a punctate pattern that largely coincides with that of identified NPC proteins. RL30 labels only the cytoplasmic surface of the NPC in immunogold electron microscopy, predominantly in peripheral regions nearby the cytoplasmic ring. In immunoblots of isolated rat liver NEs and cultured rat cells, RL30 recognizes a 265-kD band, as well as a series of 175-265-kD bands in rat liver NEs that are likely to be proteolytic products of p265. Sequencing of peptides from the 175- and 265-kD RL30 antigens of rat liver revealed that they are both closely related to human Tpr, a protein whose amino-terminal 150-250 amino acids appear in oncogenic fusions with the kinase domains of the met, trk, and raf protooncogenes. We found that in vitro translation of human Tpr mRNA yields a major 265-kD band. Considered together, these data indicate that the 265-kD RL30 antigen in the NPC is the rat homologue of Tpr. Interestingly, Tpr contains an exceptionally long predicted coiled coil domain (approximately 1600 amino acids). The localization and predicted structure of Tpr suggest that it is a component of the cytoplasmic fibrils of the NPC implicated in nuclear protein import. Immunofluorescence microscopy shows that during NPC reassembly at the end of mitosis, Tpr becomes concentrated at the NE significantly later than O-linked glycoproteins, including p62. This indicates that reassembly of the NPC after mitosis is a stepwise process, and that the Tpr-containing peripheral structures are assembled later than p62.

摘要

从一组针对大鼠肝细胞核被膜(NE)组分产生的单克隆抗体中,我们鉴定出一种抗体RL30,它能与非O-糖基化的新型核孔复合体(NPC)抗原发生反应。通过对培养细胞进行免疫荧光染色,RL30仅以点状模式与核被膜发生反应,这与已鉴定的NPC蛋白的模式基本一致。在免疫金电子显微镜下,RL30仅标记NPC的胞质表面,主要位于胞质环附近的周边区域。在分离的大鼠肝细胞核被膜和培养的大鼠细胞的免疫印迹中,RL30识别出一条265-kD的条带,以及大鼠肝细胞核被膜中一系列175 - 265-kD的条带,这些条带可能是p265的蛋白水解产物。对大鼠肝中175-kD和265-kD RL30抗原的肽段进行测序发现,它们都与人类Tpr密切相关,Tpr是一种蛋白质,其氨基末端150 - 250个氨基酸出现在与met、trk和raf原癌基因的激酶结构域形成的致癌融合体中。我们发现,人Tpr mRNA的体外翻译产生一条主要的265-kD条带。综合这些数据表明,NPC中265-kD的RL30抗原是Tpr的大鼠同源物。有趣的是,Tpr包含一个异常长的预测卷曲螺旋结构域(约1600个氨基酸)。Tpr的定位和预测结构表明它是NPC胞质纤维的一个组分,参与核蛋白的输入。免疫荧光显微镜显示,在有丝分裂末期NPC重新组装过程中,Tpr比包括p62在内的O-连接糖蛋白显著更晚地聚集在核被膜处。这表明有丝分裂后NPC的重新组装是一个逐步的过程,并且含Tpr的周边结构比p62组装得更晚。

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