Literature DB >> 21539828

Functional analyses of vertebrate TCF proteins in C. elegans embryos.

Scott M Robertson1, Miao-Chia Lo, Ranaan Odom, Xiao-Dong Yang, Jessica Medina, Shuyi Huang, Rueyling Lin.   

Abstract

In the canonical Wnt pathway, signaling results in the stabilization and increased levels of β-catenin in responding cells. β-catenin then enters the nucleus, functioning as a coactivator for the Wnt effector, TCF/LEF protein. In the absence of Wnt signaling, TCF is complexed with corepressors, together repressing Wnt target genes. In C. elegans, Wnt signaling specifies the E blastomere to become the endoderm precursor. Activation of endoderm genes in E requires not only an increase in β-catenin level, but a concomitant decrease in the nuclear level of POP-1, the sole C. elegans TCF. A decrease in nuclear POP-1 levels requires Wnt-induced phosphorylation of POP-1 and 14-3-3 protein-mediated nuclear export. Nuclear POP-1 levels remain high in the sister cell of E, MS, where POP-1 represses the expression of endoderm genes. Here we express three vertebrate TCF proteins (human TCF4, mouse LEF1 and Xenopus TCF3) in C. elegans embryos and compare their localization, repression and activation functions to POP-1. All three TCFs are localized to the nucleus in C. elegans embryos, but none undergoes Wnt-induced nuclear export. Although unable to undergo Wnt-induced nuclear export, human TCF4, but not mouse LEF1 or Xenopus TCF3, can repress endoderm genes in MS, in a manner very similar to POP-1. This repressive activity requires that human TCF4 recognizes specific promoter sequences upstream of endoderm genes and interacts with C. elegans corepressors. Domain swapping identified two regions of POP-1 that are sufficient to confer nuclear asymmetry to human TCF4 when swapped with its corresponding domains. Despite undergoing Wnt-induced nuclear export, the human TCF4/POP-1 chimeric protein continues to function as a repressor for endoderm genes in E, a result we attribute to the inability of hTCF4 to bind to C. elegans β-catenin. Our results reveal a higher degree of species specificity among TCF proteins for coactivator interactions than for corepressor interactions, and uncover a basic difference between how POP-1 and human TCF4 steady state nuclear levels are regulated.
Copyright © 2011 Elsevier Inc. All rights reserved.

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Year:  2011        PMID: 21539828      PMCID: PMC3104061          DOI: 10.1016/j.ydbio.2011.04.012

Source DB:  PubMed          Journal:  Dev Biol        ISSN: 0012-1606            Impact factor:   3.582


  36 in total

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4.  Dynamics of a developmental switch: recursive intracellular and intranuclear redistribution of Caenorhabditis elegans POP-1 parallels Wnt-inhibited transcriptional repression.

Authors:  Morris F Maduro; Rueyling Lin; Joel H Rothman
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5.  Phosphorylation by the beta-catenin/MAPK complex promotes 14-3-3-mediated nuclear export of TCF/POP-1 in signal-responsive cells in C. elegans.

Authors:  Miao-Chia Lo; Frédérique Gay; Raanan Odom; Yang Shi; Rueyling Lin
Journal:  Cell       Date:  2004-04-02       Impact factor: 41.582

6.  Binary cell fate specification during C. elegans embryogenesis driven by reiterated reciprocal asymmetry of TCF POP-1 and its coactivator beta-catenin SYS-1.

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2.  Uncoupling different characteristics of the C. elegans E lineage from differentiation of intestinal markers.

Authors:  Scott M Robertson; Jessica Medina; Rueyling Lin
Journal:  PLoS One       Date:  2014-09-02       Impact factor: 3.240

3.  Distinct DNA binding sites contribute to the TCF transcriptional switch in C. elegans and Drosophila.

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4.  Evolutionary Dynamics of the SKN-1 → MED → END-1,3 Regulatory Gene Cascade in Caenorhabditis Endoderm Specification.

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  4 in total

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