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β-连环蛋白的末端区域对于调节其黏附功能和转录功能至关重要。

Terminal regions of β-catenin are critical for regulating its adhesion and transcription functions.

作者信息

Dar Mohd Saleem, Singh Paramjeet, Singh Gurjinder, Jamwal Gayatri, Hussain Syed Sajad, Rana Aarti, Akhter Yusuf, Monga Satdarshan P, Dar Mohd Jamal

机构信息

Academy of Scientific and Innovative Research (AcSIR), New Delhi, India; Cancer Pharmacology Division, CSIR-Indian Institute of Integrative Medicine, Jammu, J&K, India.

School of Life Sciences, Central University of Himachal Pradesh, Himachal Pradesh, India.

出版信息

Biochim Biophys Acta. 2016 Sep;1863(9):2345-57. doi: 10.1016/j.bbamcr.2016.06.010. Epub 2016 Jun 29.

DOI:10.1016/j.bbamcr.2016.06.010
PMID:27368802
Abstract

β-Catenin, the central molecule of canonical Wnt signaling pathway, has multiple binding partners and performs many roles in the cell. Apart from being a transcriptional activator, β-catenin acts as a crucial effector component of cadherin/catenin complex to physically interact with actin cytoskeleton along with α-catenin and E-cadherin for regulating cell-cell adhesion. Here, we have generated a library of β-catenin point and deletion mutants to delineate regions within β-catenin that are important for α-catenin-β-catenin interaction, nuclear localization, and transcriptional activity of β-catenin. We observed a unique mechanism for nuclear localization of β-catenin and its mutants and show that N-terminal exon-3 region and C-terminal domain of β-catenin are critical for this activity of β-catenin. Furthermore, we show HepG2 cells have high β-catenin mediated transcriptional activity due to the presence of an interstitial deletion at the N-terminal region of β-catenin. Due to this deletion mutant (hereupon called TM), GSK3β and HDAC inhibitors failed to show any impact whereas curcumin significantly inhibited β-catenin mediated transcriptional activity reiterating that TM is primarily responsible for the high transcriptional activity of HepG2 cells. Moreover, we show the recombinant TM does not physically interact with α-catenin, localizes predominantly in the nucleus, and has nearly two-fold higher transcriptional activity than the wildtype β-catenin.

摘要

β-连环蛋白是经典Wnt信号通路的核心分子,有多个结合伴侣,在细胞中发挥多种作用。除了作为转录激活因子外,β-连环蛋白还是钙黏蛋白/连环蛋白复合体的关键效应成分,与α-连环蛋白和E-钙黏蛋白一起与肌动蛋白细胞骨架进行物理相互作用,以调节细胞间黏附。在此,我们构建了一个β-连环蛋白点突变和缺失突变体文库,以确定β-连环蛋白中对α-连环蛋白-β-连环蛋白相互作用、核定位以及β-连环蛋白转录活性重要的区域。我们观察到β-连环蛋白及其突变体核定位的独特机制,并表明β-连环蛋白的N端外显子3区域和C端结构域对β-连环蛋白的这一活性至关重要。此外,我们发现由于β-连环蛋白N端区域存在间隙缺失,HepG2细胞具有较高的β-连环蛋白介导的转录活性。由于这种缺失突变体(以下称为TM),GSK3β和HDAC抑制剂未显示出任何影响,而姜黄素显著抑制了β-连环蛋白介导的转录活性,这再次表明TM是HepG2细胞高转录活性的主要原因。此外,我们发现重组TM不与α-连环蛋白进行物理相互作用,主要定位于细胞核,并且转录活性比野生型β-连环蛋白高近两倍。

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