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P2P-R的功能潜能:与其与结合于DNA基质相关区域的蛋白质相互作用有关,在细胞周期和细胞分化中发挥作用?

Functional potential of P2P-R: a role in the cell cycle and cell differentiation related to its interactions with proteins that bind to matrix associated regions of DNA?

作者信息

Scott Robert E, Giannakouros Thomas, Gao Sizhi, Peidis Philippos

机构信息

Department of Pathology, University of Tennessee Health Science Center, Memphis, Tennessee 38163, USA.

出版信息

J Cell Biochem. 2003 Sep 1;90(1):6-12. doi: 10.1002/jcb.10618.

DOI:10.1002/jcb.10618
PMID:12938151
Abstract

P2P-R is the alternately spliced product of the P2P-R/PACT gene in that P2P-R lacks one exon encoding 34 amino acids. The 250 kDa P2P-R protein is the predominate product expressed in multiple murine cell lines. It is a highly basic protein that contains multiple domains including an N-terminal RING type zinc finger, a proline rich domain, an RS region, and a C-terminal lysine-rich domain. P2P-R binds the p53 and the Rb1 tumor suppressors and is phosphorylated by the cdc2 and SRPK1a protein kinases. P2P-R also interacts with scaffold attachment factor-B (SAF-B), a well characterized MARs (for matrix attachment regions) binding factor, and may interact with nucleolin, another MARs binding factor. In addition, P2P-R binds single strand DNA (ssDNA). The expression of P2P-R is regulated by differentiation and cell cycle events. P2P-R mRNA is markedly repressed during differentiation, whereas immunoreactive P2P-R protein levels are >10-fold higher in mitotic than in G(0) cells. The localization of P2P-R also is modulated during the cell cycle. During interphase, P2P-R is present primarily in nucleoli and nuclear speckles whereas during mitosis, P2P-R associates with the periphery of chromosomes. Overexpression of near full length P2P-R induces mitotic arrest in prometaphase and mitotic apoptosis, and overexpression of selected P2P-R segments also can promote apoptosis. This compendium of data supports the possibility that P2P-R may form complexes with the Rb1 and/or p53 tumor suppressors and MARs-related factors, in a cell cycle and cell differentiation-dependent manner, to influence gene transcription/expression and nuclear organization.

摘要

P2P-R是P2P-R/PACT基因的可变剪接产物,因为P2P-R缺少一个编码34个氨基酸的外显子。250 kDa的P2P-R蛋白是在多种小鼠细胞系中表达的主要产物。它是一种高度碱性的蛋白质,包含多个结构域,包括一个N端RING型锌指、一个富含脯氨酸的结构域、一个RS区域和一个C端富含赖氨酸的结构域。P2P-R与p53和Rb1肿瘤抑制因子结合,并被cdc2和SRPK1a蛋白激酶磷酸化。P2P-R还与支架附着因子-B(SAF-B,一种特征明确的MARs(基质附着区域)结合因子)相互作用,并且可能与另一种MARs结合因子核仁素相互作用。此外,P2P-R结合单链DNA(ssDNA)。P2P-R的表达受分化和细胞周期事件的调节。P2P-R mRNA在分化过程中明显受到抑制,而免疫反应性P2P-R蛋白水平在有丝分裂期比在G(0)期细胞中高10倍以上。P2P-R的定位在细胞周期中也受到调节。在间期,P2P-R主要存在于核仁和核斑中,而在有丝分裂期间,P2P-R与染色体周边相关联。近全长P2P-R的过表达诱导有丝分裂前期的有丝分裂停滞和有丝分裂凋亡,并且所选P2P-R片段的过表达也可以促进凋亡。这些数据汇总支持了P2P-R可能以细胞周期和细胞分化依赖的方式与Rb1和/或p53肿瘤抑制因子以及MARs相关因子形成复合物,以影响基因转录/表达和核组织的可能性。

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