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去除微管后纤毛九倍体结构的保留

Retention of ciliary ninefold structure after removal of microtubules.

作者信息

Stephens R E, Oleszko-Szuts S, Linck R W

机构信息

Marine Biological Laboratory, Woods Hole, MA 02543.

出版信息

J Cell Sci. 1989 Mar;92 ( Pt 3):391-402. doi: 10.1242/jcs.92.3.391.

DOI:10.1242/jcs.92.3.391
PMID:2592445
Abstract

When axonemes of isolated gill cilia from the bay scallop Aequipecten irradians are heated at 45 degrees C for a minimum of 8 min in a 10 mM-Tris-HCl (pH 8), 1 mM-EDTA solution, nearly 80% of the tubulin is solubilized but most minor structural proteins are retained in a ninefold symmetrical configuration. This remnant consists of the junctional protofilaments, derived from outer doublet tubules, interconnected by nexin linkages, with radial spoke components still directed inwards. The remnant is of the same length as the original cilium, with the junctional protofilaments attached at the distal end to the ciliary tip and at the proximal end to the basal plate. Virtually identical fractionations can be achieved with blastula cilia isolated from both arctic and tropical sea-urchin embryos. The remnant is resistant to salt up to at least 1 M concentration, judged by the constancy of protein composition. Immunoblotting with antibodies against sea-urchin sperm flagellar tektins indicates that the tektins remain within the ciliary remnant, supporting their location within the junctional protofilament domain. The fractionation is inhibited by low pH, by magnesium or calcium ions in the millimolar range, and by monovalent ions at 10-fold higher concentrations. About a quarter of the total ciliary calmodulin is bound to the axoneme at micromolar calcium levels but most is released upon thermal fractionation. Polymerization of tubulin in the presence of the remnant results in singlet microtubules, separate from the remnant proper, suggesting that doublet formation may require coordinate co-assembly of tubulin with skeletal proteins. These observations demonstrate the existence of a fibrous skeleton in the axoneme, composed largely of ciliary tektins, nexin linkages, and other structural proteins.

摘要

将海湾扇贝辐肛扇贝分离出的鳃纤毛轴丝,在10 mM - Tris - HCl(pH 8)、1 mM - EDTA溶液中于45℃加热至少8分钟,近80%的微管蛋白会溶解,但大多数次要结构蛋白会保留在九倍对称结构中。这个残余物由来自外双联微管的连接原纤维组成,通过连接蛋白连接在一起,径向辐条成分仍向内指向。残余物与原始纤毛长度相同,连接原纤维在远端附着于纤毛尖端,在近端附着于基板。从北极和热带海胆胚胎分离出的囊胚纤毛也能实现几乎相同的分级分离。根据蛋白质组成的稳定性判断,残余物对至少1 M浓度的盐具有抗性。用抗海胆精子鞭毛轴纤丝蛋白的抗体进行免疫印迹表明,轴纤丝蛋白保留在纤毛残余物中,这支持了它们在连接原纤维区域内的位置。低pH、毫摩尔范围内的镁或钙离子以及浓度高10倍的单价离子会抑制分级分离。在微摩尔钙水平下,约四分之一的总纤毛钙调蛋白与轴丝结合,但在热分级分离时大部分会释放。在残余物存在的情况下微管蛋白聚合会形成单微管,并与残余物本身分离,这表明双联微管的形成可能需要微管蛋白与骨架蛋白协同共组装。这些观察结果证明了轴丝中存在纤维骨架,其主要由纤毛轴纤丝蛋白、连接蛋白和其他结构蛋白组成。

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Retention of ciliary ninefold structure after removal of microtubules.去除微管后纤毛九倍体结构的保留
J Cell Sci. 1989 Mar;92 ( Pt 3):391-402. doi: 10.1242/jcs.92.3.391.
2
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At least one of the protofilaments in flagellar microtubules is not composed of tubulin.鞭毛微管中的原纤维至少有一根不是由微管蛋白组成的。
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Specific localization of scallop gill epithelial calmodulin in cilia.扇贝鳃上皮钙调蛋白在纤毛中的特异性定位。
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Tektins are heterodimeric polymers in flagellar microtubules with axial periodicities matching the tubulin lattice.纤毛蛋白是鞭毛微管中的异二聚体聚合物,其轴向周期性与微管蛋白晶格相匹配。
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Flagellar doublet microtubules: fractionation of minor components and alpha-tubulin from specific regions of the A-tubule.鞭毛双联体微管:从小管A的特定区域分离次要成分和α-微管蛋白。
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Proteins closely similar to flagellar tektins are detected in cilia but not in cytoplasmic microtubules.在纤毛中检测到与鞭毛轴纤丝蛋白密切相似的蛋白质,但在细胞质微管中未检测到。
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Major membrane protein differences in cilia and flagella: evidence for a membrane-associated tubulin.纤毛和鞭毛中主要膜蛋白的差异:膜相关微管蛋白的证据。
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Mol Biol Cell. 2013 Apr;24(8):1134-52. doi: 10.1091/mbc.E12-11-0801. Epub 2013 Feb 20.
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