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水和氯离子作为WNK激酶渗透压感知中的变构抑制剂。

Water and chloride as allosteric inhibitors in WNK kinase osmosensing.

作者信息

Teixeira Liliana R, Akella Radha, Humphreys John M, He Haixia, Goldsmith Elizabeth J

出版信息

bioRxiv. 2024 Aug 26:2023.08.29.555411. doi: 10.1101/2023.08.29.555411.

DOI:10.1101/2023.08.29.555411
PMID:37693587
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC10491171/
Abstract

Osmotic stress and chloride regulate the autophosphorylation and activity of the WNK1 and WNK3 kinase domains. The kinase domain of unphosphorylated WNK1 (uWNK1) is an asymmetric dimer possessing water molecules conserved in multiple uWNK1 crystal structures. Conserved waters are present in two networks, referred to here as conserved water networks 1 and 2 (CWN1and CWN2). Here we show that PEG400 applied to crystals of dimeric uWNK1 induces de-dimerization. Both the WNK1 the water networks and the chloride binding site and are disrupted by PEG400. CWN1 is surrounded by a cluster of pan-WNK-conserved charged residues. Here we mutagenized these charges in WNK3, a highly active WNK isoform kinase domain, and WNK1, the isoform best studied crystallographically. Mutation of E314 in the Activation Loop of WNK3 (WNK3/E314Q and WNK3/E314A, and the homologous WNK1/E388A) enhanced the rate of autophosphorylation, and reduced chloride sensitivity. Other WNK3 Cluster mutants reduced the rate of autophosphorylation activity coupled with greater chloride sensitivity than wild-type. The water and chloride regulation thus appear linked. The lower activity of some mutants may reflect effects on catalysis. Crystallography showed that activating mutants introduced conformational changes in similar parts of the structure to those induced by PEG400. WNK activating mutations and crystallography support a role for CWN1 in WNK inhibition consistent with water functioning as an allosteric ligand.

摘要

渗透应激和氯离子调节WNK1和WNK3激酶结构域的自磷酸化及活性。未磷酸化的WNK1(uWNK1)的激酶结构域是一种不对称二聚体,在多个uWNK1晶体结构中存在保守的水分子。保守水分子存在于两个网络中,在此称为保守水网络1和2(CWN1和CWN2)。在此我们表明,将聚乙二醇400(PEG400)应用于二聚体uWNK1晶体可诱导去二聚化。PEG400破坏了WNK1的水网络以及氯离子结合位点。CWN1被一组泛WNK保守的带电荷残基所包围。在此我们对WNK3(一种高活性WNK异构体激酶结构域)和WNK1(晶体学研究最多的异构体)中的这些电荷进行了诱变。WNK3激活环中的E314突变(WNK3/E314Q和WNK3/E314A,以及同源的WNK1/E388A)提高了自磷酸化速率,并降低了对氯离子的敏感性。其他WNK3簇突变体降低了自磷酸化活性速率,且比野生型具有更高的氯离子敏感性。因此,水和氯离子调节似乎是相关联的。一些突变体较低的活性可能反映了对催化的影响。晶体学显示,激活突变体在结构的相似部分引入了构象变化,类似于PEG400诱导的变化。WNK激活突变和晶体学支持CWN1在WNK抑制中发挥作用,这与水作为变构配体的功能一致。

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