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Chlamydomonas ODA10 is a conserved axonemal protein that plays a unique role in outer dynein arm assembly

机译:衣藻ODA10是一种保守的轴突蛋白在外部动力蛋白臂装配中起独特作用

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摘要

Assembly of outer dynein arms (ODAs) requires multiple steps and involves multiple proteins in addition to dynein subunits. The Chlamydomonas ODA10, ODA5, and ODA8 loci genetically interact and are hypothesized to function as an axonemal accessory complex, but only ODA5p was previously characterized. We positionally cloned ODA10 and identified the gene by rescuing an oda10 mutant with a hemagglutinin-tagged cDNA. ODA10 sequence predicts a conserved coiled-coil protein homologous to mouse ccdc151. ODA10p is present in cytoplasm and flagella, remains axonemal after detergent treatment, and is extracted with 0.6 M NaCl. Both outer arm dynein and ODA10p rebound to the axonemes when desalted extracts are mixed with oda10-mutant axonemes. Sucrose gradient separation of these extracts shows that ODA10p sediments near the top of the gradient, not with 23S outer dynein arm proteins. Unexpectedly, dynein and ODA10p fractions are able to bind individually to oda10 axonemes. ODA10p is present on oda8-mutant flagella at wild-type levels. However, ODA10p does not assemble into oda5 flagella and is absent from oda5 cytoplasm, suggesting a necessity of ODA5p for stability of ODA10p in vivo. The results suggest that ODA10p does not function as a part of a traditionally defined docking complex.
机译:动力蛋白外臂(ODA)的组装需要多个步骤,并且除了动力蛋白亚基外还涉及多种蛋白质。衣藻的ODA10,ODA5和ODA8基因座通过基因相互作用而被认为具有轴突辅助复合体的功能,但以前仅鉴定了ODA5p。我们在位置上克隆了ODA10,并通过用血凝素标记的cDNA拯救oda10突变体来鉴定了该基因。 ODA10序列预测与小鼠ccdc151同源的保守的卷曲螺旋蛋白。 ODA10p存在于细胞质和鞭毛中,在去污剂处理后仍保持轴突,并用0.6 M NaCl萃取。将脱盐提取物与oda10突变型轴突混合后,外臂动力蛋白和ODA10p均会反弹至轴突。这些提取物的蔗糖梯度分离表明,ODA10p沉淀物靠近梯度顶部,而不带有23S外部动力蛋白臂蛋白。出乎意料的是,动力蛋白和ODA10p组分能够分别与oda10轴突结合。 ODA10p以野生型水平存在于oda8突变鞭毛上。然而,ODA10p不能组装到oda5鞭毛中,而在oda5细胞质中却不存在,这表明ODA5p对于ODA10p体内稳定性的必要性。结果表明,ODA10p不能用作传统定义的对接复合体的一部分。

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