Evidence for an interaction of paracingulin with microtubules.

microPublication biology Pub Date : 2024-10-14 eCollection Date: 2024-01-01 DOI:10.17912/micropub.biology.001341
Arielle Flinois, Annick Mutero-Maeda, Sylvie Montessuit, Sandra Citi
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Abstract

The mechanisms that anchor microtubules to epithelial junctions are poorly understood. Here we show that recombinant purified paracingulin ( CGNL1 , JACOP), a cytoplasmic junctional protein, decorates microtubules by negative staining electron microscopy and co-pellets with microtubules. Co-pelleting experiments using fragments of CGNL1 indicate that this is mediated by a central region of the CGNL1 head domain (residues 250-420). Deletion of a basic amino-acid stretch (365-377) within this fragment, abolishes both co-pelleting with and decoration of microtubules. These results suggest that paracingulin can interact directly with microtubules through a basic amino-acid stretch of its head domain.

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副角蛋白与微管相互作用的证据
人们对将微管锚定在上皮连接处的机制知之甚少。在这里,我们发现重组纯化的paracingulin(CGNL1,JACOP)是一种细胞质连接蛋白,通过负染色电子显微镜可装饰微管,并与微管共同造粒。使用 CGNL1 片段进行的共小球实验表明,这是由 CGNL1 头域的中心区域(残基 250-420)介导的。删除该片段中的一个碱性氨基酸区段(365-377)后,就不能与微管共同造粒,也不能装饰微管。这些结果表明,paracingulin 可通过其头部结构域的一个基本氨基酸段直接与微管相互作用。
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