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首页> 外文期刊>Nature Communications >Inner lumen proteins stabilize doublet microtubules in cilia and flagella
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Inner lumen proteins stabilize doublet microtubules in cilia and flagella

机译:内腔蛋白可稳定纤毛和鞭毛中的双态微管

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Motile cilia are microtubule-based organelles that play important roles in most eukaryotes. Although axonemal microtubules are sufficiently stable to withstand their beating motion, it remains unknown how they are stabilized while serving as tracks for axonemal dyneins. To address this question, we have identified two uncharacterized proteins, FAP45 and FAP52, as microtubule inner proteins (MIPs) in Chlamydomonas. These proteins are conserved among eukaryotes with motile cilia. Using cryo-electron tomography (cryo-ET) and high-speed atomic force microscopy (HS-AFM), we show that lack of these proteins leads to a loss of inner protrusions in B-tubules and less stable microtubules. These protrusions are located near the inner junctions of doublet microtubules and lack of both FAP52 and a known inner junction protein FAP20 results in detachment of the B-tubule from the A-tubule, as well as flagellar shortening. These results demonstrate that FAP45 and FAP52 bind to the inside of microtubules and stabilize ciliary axonemes.
机译:运动纤毛是基于微管的细胞器,在大多数真核生物中起重要作用。尽管轴突微管足够稳定以承受其跳动运动,但仍未知如何稳定它们作为轴突动力蛋白的轨迹。为了解决这个问题,我们在衣原体中鉴定了两个未表征的蛋白FAP45和FAP52作为微管内部蛋白(MIP)。这些蛋白质在具有活动纤毛的真核生物中是保守的。使用低温电子断层扫描(cryo-ET)和高速原子力显微镜(HS-AFM),我们显示缺少这些蛋白质会导致B小管内部突起的损失和稳定性较差的微管。这些突起位于双峰微管的内部连接附近,并且缺乏FAP52和已知的内部连接蛋白FAP20导致B管从A管分离,并导致鞭毛缩短。这些结果表明,FAP45和FAP52结合到微管内部并稳定睫状轴突。

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