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Serial analysis of chromatin occupancy identifies beta-catenin target genes in colorectal carcinoma cells.染色质占据的序列分析鉴定结直肠癌细胞中的β-连环蛋白靶基因。
Proc Natl Acad Sci U S A. 2007 Feb 27;104(9):3324-9. doi: 10.1073/pnas.0611576104. Epub 2007 Feb 21.
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Diversity of LEF/TCF action in development and disease.淋巴样增强因子/转录因子(LEF/TCF)在发育和疾病中的作用多样性。
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Structural basis of DNA recognition by p53 tetramers.p53四聚体识别DNA的结构基础。
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Beta-catenin directly displaces Groucho/TLE repressors from Tcf/Lef in Wnt-mediated transcription activation.在Wnt介导的转录激活过程中,β-连环蛋白直接从Tcf/Lef上取代Groucho/TLE阻遏物。
Nat Struct Mol Biol. 2005 Apr;12(4):364-71. doi: 10.1038/nsmb912. Epub 2005 Mar 13.
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PITX2, beta-catenin and LEF-1 interact to synergistically regulate the LEF-1 promoter.PITX2、β-连环蛋白和淋巴样增强因子-1相互作用,协同调节淋巴样增强因子-1启动子。
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Role of the proto-oncogene Pokemon in cellular transformation and ARF repression.原癌基因Pokemon在细胞转化和ARF抑制中的作用。
Nature. 2005 Jan 20;433(7023):278-85. doi: 10.1038/nature03203.
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p53 linear diffusion along DNA requires its C terminus.p53沿DNA的线性扩散需要其C末端。
Mol Cell. 2004 Nov 5;16(3):413-24. doi: 10.1016/j.molcel.2004.09.032.
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Tcf binding sequence and position determines beta-catenin and Lef-1 responsiveness of MMP-7 promoters.Tcf结合序列和位置决定MMP-7启动子的β-连环蛋白和Lef-1反应性。
Mol Carcinog. 2004 Nov;41(3):125-39. doi: 10.1002/mc.20049.
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The LEF-1 high-mobility group domain undergoes a disorder-to-order transition upon formation of a complex with cognate DNA.LEF-1高迁移率族结构域在与同源DNA形成复合物时会经历从无序到有序的转变。
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一个独特的DNA结合结构域将T细胞因子转化为强大的Wnt效应器。

A unique DNA binding domain converts T-cell factors into strong Wnt effectors.

作者信息

Atcha Fawzia A, Syed Adeela, Wu Beibei, Hoverter Nate P, Yokoyama Noriko N, Ting Ju-Hui T, Munguia Jesus E, Mangalam Harry J, Marsh J Lawrence, Waterman Marian L

机构信息

Department of Microbiology and Molecular Genetics, University of California, Irvine, Irvine, CA 92697, USA.

出版信息

Mol Cell Biol. 2007 Dec;27(23):8352-63. doi: 10.1128/MCB.02132-06. Epub 2007 Sep 24.

DOI:10.1128/MCB.02132-06
PMID:17893322
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2169181/
Abstract

Wnt regulation of gene expression requires binding of LEF/T-cell factor (LEF/TCF) transcription factors to Wnt response elements (WREs) and recruitment of the activator beta-catenin. There are significant differences in the abilities of LEF/TCF family members to regulate Wnt target genes. For example, alternatively spliced isoforms of TCF-1 and TCF-4 with a C-terminal "E" tail are uniquely potent in their activation of LEF1 and CDX1. Here we report that the mechanism responsible for this unique activity is an auxiliary 30-amino-acid DNA interaction motif referred to here as the "cysteine clamp" (or C-clamp). The C-clamp contains invariant cysteine, aromatic, and basic residues, and surface plasmon resonance (SPR) studies with recombinant C-clamp protein showed that it binds double-stranded DNA but not single-stranded DNA or RNA (equilibrium dissociation constant = 16 nM). CASTing (Cyclic Amplification and Selection of Targets) experiments were used to test whether this motif influences WRE recognition. Full-length LEF-1, TCF-1E, and TCF-1E with a mutated C-clamp all bind nearly identical WREs (TYYCTTTGATSTT), showing that the C-clamp does not alter WRE specificity. However, a GC element downstream of the WRE (RCCG) is enriched in wild-type TCF-1E binding sites but not in mutant TCF-1E binding sites. We conclude that the C-clamp is a sequence-specific DNA binding motif. C-clamp mutations destroy the ability of beta-catenin to regulate the LEF1 promoter, and they severely impair the ability of TCF-1 to regulate growth in colon cancer cells. Thus, E-tail isoforms of TCFs utilize two DNA binding activities to access a subset of Wnt targets important for cell growth.

摘要

Wnt对基因表达的调控需要淋巴样增强因子/T细胞因子(LEF/TCF)转录因子与Wnt反应元件(WREs)结合,并募集激活剂β-连环蛋白。LEF/TCF家族成员调控Wnt靶基因的能力存在显著差异。例如,具有C端“E”尾的TCF-1和TCF-4的可变剪接异构体在激活LEF1和CDX1方面具有独特的高效性。在此我们报告,负责这种独特活性的机制是一个辅助性的30个氨基酸的DNA相互作用基序,在此称为“半胱氨酸钳”(或C-钳)。C-钳包含不变的半胱氨酸、芳香族和碱性残基,对重组C-钳蛋白进行的表面等离子体共振(SPR)研究表明,它结合双链DNA,但不结合单链DNA或RNA(平衡解离常数 = 16 nM)。采用循环扩增和靶标选择(CASTing)实验来测试该基序是否影响WRE识别。全长LEF-1、TCF-1E以及具有突变C-钳的TCF-1E均结合几乎相同的WRE(TYYCTTTGATSTT),表明C-钳不会改变WRE特异性。然而,WRE下游的一个GC元件(RCCG)在野生型TCF-1E结合位点中富集,但在突变型TCF-1E结合位点中未富集。我们得出结论,C-钳是一个序列特异性DNA结合基序。C-钳突变破坏了β-连环蛋白调控LEF1启动子的能力,并且严重损害了TCF-1调控结肠癌细胞生长的能力。因此,TCF的E-尾异构体利用两种DNA结合活性来作用于对细胞生长重要的一部分Wnt靶标。