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微管酪氨酸连接酶样基因 ttll3 和 ttll6 维持斑马鱼纤毛结构和运动。

Tubulin tyrosine ligase-like genes ttll3 and ttll6 maintain zebrafish cilia structure and motility.

机构信息

Nephrology Division, Massachusetts General Hospital, Charlestown, Massachusetts 02129, USA.

出版信息

J Biol Chem. 2011 Apr 1;286(13):11685-95. doi: 10.1074/jbc.M110.209817. Epub 2011 Jan 24.

DOI:10.1074/jbc.M110.209817
PMID:21262966
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3064220/
Abstract

Tubulin post-translational modifications generate microtubule heterogeneity and modulate microtubule function, and are catalyzed by tubulin tyrosine ligase-like (TTLL) proteins. Using antibodies specific to monoglycylated, polyglycylated, and glutamylated tubulin in whole mount immunostaining of zebrafish embryos, we observed distinct, tissue-specific patterns of tubulin modifications. Tubulin modification patterns in cilia correlated with the expression of ttll3 and ttll6 in ciliated cells. Expression screening of all zebrafish tubulin tyrosine ligase-like genes revealed additional tissue-specific expression of ttll1 in brain neurons, ttll4 in muscle, and ttll7 in otic placodes. Knockdown of ttll3 eliminated cilia tubulin glycylation but had surprisingly mild effects on cilia structure and motility. Similarly, knockdown of ttll6 strongly reduced cilia tubulin glutamylation but only partially affected cilia structure and motility. Combined loss of function of ttll3 and ttll6 caused near complete loss of cilia motility and induced a variety of axonemal ultrastructural defects similar to defects previously observed in zebrafish fleer mutants, which were shown to lack tubulin glutamylation. Consistently, we find that fleer mutants also lack tubulin glycylation. These results indicate that tubulin glycylation and glutamylation have overlapping functions in maintaining cilia structure and motility and that the fleer/dyf-1 TPR protein is required for both types of tubulin post-translational modification.

摘要

微管蛋白翻译后修饰产生微管异质性并调节微管功能,由微管酪氨酸连接酶样(TTLL)蛋白催化。使用针对单糖基化、多糖基化和谷氨酸化微管蛋白的特异性抗体,对斑马鱼胚胎的全胚胎免疫染色进行研究,我们观察到了微管蛋白修饰的独特、组织特异性模式。纤毛中的微管修饰模式与纤毛细胞中 ttll3 和 ttll6 的表达相关。对所有斑马鱼微管酪氨酸连接酶样基因的表达筛选显示,ttll1 在脑神经元中、ttll4 在肌肉中、ttll7 在耳胚盘中具有额外的组织特异性表达。ttll3 的敲低消除了纤毛微管糖基化,但对纤毛结构和运动仅有轻微影响。同样,ttll6 的敲低强烈降低了纤毛微管谷氨酸化,但仅部分影响了纤毛结构和运动。ttll3 和 ttll6 的功能丧失会导致纤毛运动几乎完全丧失,并引起各种轴丝超微结构缺陷,类似于先前在缺乏微管谷氨酸化的斑马鱼 fleer 突变体中观察到的缺陷。同样,我们发现 fleer 突变体也缺乏微管糖基化。这些结果表明,微管糖基化和谷氨酸化在维持纤毛结构和运动方面具有重叠功能,fleer/dyf-1 TPR 蛋白是这两种微管翻译后修饰所必需的。

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本文引用的文献

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Post-translational modifications of microtubules.微管的翻译后修饰。
J Cell Sci. 2010 Oct 15;123(Pt 20):3447-55. doi: 10.1242/jcs.063727.
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Tubulin polyglutamylation is essential for airway ciliary function through the regulation of beating asymmetry.微管多聚谷氨酸化通过调节纤毛摆动不对称对于气道纤毛功能是必需的。
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Tubulin glutamylation regulates ciliary motility by altering inner dynein arm activity.微管谷氨酸化通过改变内动力蛋白臂的活性来调节纤毛运动。
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Tubulin polyglutamylation regulates axonemal motility by modulating activities of inner-arm dyneins.微管多聚谷氨酸化通过调节动纤丝内臂动力蛋白的活性来调节轴突运动。
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Hyperglutamylation of tubulin can either stabilize or destabilize microtubules in the same cell.微管蛋白的高谷氨酰胺化作用在同一细胞中既能使微管稳定,也能使其不稳定。
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DYF-1 Is required for assembly of the axoneme in Tetrahymena thermophila.嗜热四膜虫轴丝的组装需要DYF-1。
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TTLL3 Is a tubulin glycine ligase that regulates the assembly of cilia.TTLL3是一种微管蛋白甘氨酸连接酶,可调节纤毛的组装。
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Synaptic activation modifies microtubules underlying transport of postsynaptic cargo.突触激活会改变突触后货物运输所依赖的微管。
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