Wnt target gene activation requires β-catenin separation into biomolecular condensates.

IF 9.8 1区生物学 Q1 Agricultural and Biological Sciences PLoS Biology Pub Date : 2024-09-24 eCollection Date: 2024-09-01 DOI:10.1371/journal.pbio.3002368

Richard A Stewart, Zhihao Ding, Ung Seop Jeon, Lauren B Goodman, Jeannine J Tran, John P Zientko, Malavika Sabu, Ken M Cadigan

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Abstract

The Wnt/β-catenin signaling pathway plays numerous essential roles in animal development and tissue/stem cell maintenance. The activation of genes regulated by Wnt/β-catenin signaling requires the nuclear accumulation of β-catenin, a transcriptional co-activator. β-catenin is recruited to many Wnt-regulated enhancers through direct binding to T-cell factor/lymphoid enhancer factor (TCF/LEF) family transcription factors. β-catenin has previously been reported to form phase-separated biomolecular condensates (BMCs), which was implicated as a component of β-catenin's mechanism of action. This function required aromatic amino acid residues in the intrinsically disordered regions (IDRs) at the N- and C-termini of the protein. In this report, we further explore a role for β-catenin BMCs in Wnt target gene regulation. We find that β-catenin BMCs are miscible with LEF1 BMCs in vitro and in cultured cells. We characterized a panel of β-catenin mutants with different combinations of aromatic residue mutations in human cell culture and Drosophila melanogaster. Our data support a model in which aromatic residues across both IDRs contribute to BMC formation and signaling activity. Although different Wnt targets have different sensitivities to loss of β-catenin's aromatic residues, the activation of every target examined was compromised by aromatic substitution. These mutants are not defective in nuclear import or co-immunoprecipitation with several β-catenin binding partners. In addition, residues in the N-terminal IDR with no previously known role in signaling are clearly required for the activation of various Wnt readouts. Consistent with this, deletion of the N-terminal IDR results in a loss of signaling activity, which can be rescued by the addition of heterologous IDRs enriched in aromatic residues. Overall, our work supports a model in which the ability of β-catenin to form biomolecular condensates in the nucleus is tightly linked to its function as a transcriptional co-regulator.

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Wnt靶基因的激活需要β-catenin分离成生物分子凝聚体。

Wnt/β-catenin信号通路在动物发育和组织/干细胞维持中发挥着许多重要作用。激活受 Wnt/β-catenin 信号调控的基因需要β-catenin（一种转录共激活因子）的核积累。β-catenin通过与T细胞因子/淋巴细胞增强因子（TCF/LEF）家族转录因子直接结合，被招募到许多Wnt调控的增强子上。据报道，β-catenin 可形成相分离的生物分子凝集物（BMC），这被认为是 β-catenin 作用机制的一个组成部分。这一功能需要蛋白质 N 端和 C 端内在无序区（IDR）中的芳香族氨基酸残基。在本报告中，我们进一步探讨了β-catenin BMC在Wnt靶基因调控中的作用。我们发现，在体外和培养细胞中，β-catenin BMC 与 LEF1 BMC 是混杂的。我们在人类细胞培养和黑腹果蝇中鉴定了一组具有不同芳香残基突变组合的β-catenin突变体。我们的数据支持这样一个模型，即两个 IDR 的芳香残基都有助于 BMC 的形成和信号活性。虽然不同的 Wnt 靶标对β-catenin芳香残基的缺失有不同的敏感性，但芳香取代会影响所研究的每个靶标的激活。这些突变体在核导入或与β-catenin的几个结合伙伴共免疫沉淀方面没有缺陷。此外，N-末端 IDR 的残基以前在信号传导中没有已知的作用，但在激活各种 Wnt 读出时显然是必需的。与此相一致的是，缺失 N 端 IDR 会导致信号活性丧失，而添加富含芳香族残基的异源 IDR 则可以挽救信号活性。总之，我们的工作支持这样一个模型，即β-catenin在细胞核中形成生物分子凝聚体的能力与其作为转录协同调控因子的功能密切相关。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

PLoS Biology BIOCHEMISTRY & MOLECULAR BIOLOGY-BIOLOGY

CiteScore

15.40

自引率

2.00%

发文量

359

审稿时长

3-8 weeks

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