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核仁素,在MPF磷酸化方面存在缺陷,在有丝分裂和核仁形成过程中正常定位。

Nucleolin, defective for MPF phosphorylation, localizes normally during mitosis and nucleologenesis.

作者信息

Zhu Y, Lu D, DiMario P

机构信息

Department of Biological Sciences, Louisiana State University, Baton Rouge 70803-1806, USA.

出版信息

Histochem Cell Biol. 1999 Jun;111(6):477-87. doi: 10.1007/s004180050384.

DOI:10.1007/s004180050384
PMID:10429970
Abstract

To determine what effect maturation promoting factor (MPF, p34(cdc2) kinase/cyclin B) phosphorylation has on nucleolin's distribution during mitotic nucleolar disassembly and reassembly, we altered Chinese hamster ovary (CHO) nucleolin (the N protein) such that it cannot be phosphorylated by p34(cdc2). As expected, the transiently expressed epitope-tagged N protein showed no apparent defect in nucleolar localization in interphase CHO cells, even after hypotonic shock and recovery to quickly disassemble and then reassemble interphase nucleoli. In mitotic CHO cells, the N protein localized to the perichromosomal sheath and the cytoplasm, as is typical for nucleolin. Similar to epitope-tagged wild-type nucleolin, the N protein also maintained its association with persistent nucleoli characteristic of mitotic Chinese hamster lung (Dede) cells. In synchronized HeLa cells, the N protein again localized to the perichromosomal sheath and the cytoplasm as nucleoli disassembled during prophase. In HeLa cell telophase, the N protein localized normally to nucleolus-derived foci within the cytoplasm and prenucleolar bodies within reforming nuclei. The observations indicate that MPF phosphorylation is not essential for nucleolin's localizations to the perichromosomal sheath and the cytoplasm during prophase and metaphase, and that functional MPF phosphorylation sites are not essential for nucleolin's localizations during nucleologenesis.

摘要

为了确定成熟促进因子(MPF,p34(cdc2)激酶/细胞周期蛋白B)磷酸化在有丝分裂核仁解体和重新组装过程中对核仁素分布有何影响,我们对中国仓鼠卵巢(CHO)核仁素(N蛋白)进行了改造,使其不能被p34(cdc2)磷酸化。正如预期的那样,即使在经过低渗休克和恢复以快速拆解然后重新组装间期核仁之后,瞬时表达的表位标记N蛋白在间期CHO细胞的核仁定位中也没有明显缺陷。在有丝分裂的CHO细胞中,N蛋白定位于染色体周围鞘和细胞质,这是核仁素的典型定位。与表位标记的野生型核仁素相似,N蛋白也与有丝分裂的中国仓鼠肺(Dede)细胞特有的持续核仁保持关联。在同步化的HeLa细胞中,随着前期核仁解体,N蛋白再次定位于染色体周围鞘和细胞质。在HeLa细胞末期,N蛋白正常定位于细胞质中的核仁衍生灶和正在重新形成的细胞核内的前核仁体。这些观察结果表明,MPF磷酸化对于前期和中期核仁素定位于染色体周围鞘和细胞质并非必不可少,并且功能性MPF磷酸化位点对于核仁形成过程中核仁素的定位也不是必需的。

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