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1
Microtubule dynamics in vivo: a test of mechanisms of turnover.体内微管动力学:周转机制的检验
J Cell Biol. 1987 Mar;104(3):395-405. doi: 10.1083/jcb.104.3.395.
2
Direct observation of microtubule dynamics in living cells.活细胞中微管动力学的直接观察。
Nature. 1988 Apr 21;332(6166):724-6. doi: 10.1038/332724a0.
3
Dynamics of microtubules bundled by microtubule associated protein 2C (MAP2C).由微管相关蛋白2C(MAP2C)捆绑的微管动力学
J Cell Biol. 1993 Jan;120(2):451-65. doi: 10.1083/jcb.120.2.451.
4
Polymerization of tubulin in vivo: direct evidence for assembly onto microtubule ends and from centrosomes.微管蛋白在体内的聚合:组装到微管末端及从中心体组装的直接证据。
J Cell Biol. 1985 May;100(5):1682-9. doi: 10.1083/jcb.100.5.1682.
5
Spindle microtubule dynamics in sea urchin embryos: analysis using a fluorescein-labeled tubulin and measurements of fluorescence redistribution after laser photobleaching.海胆胚胎中的纺锤体微管动力学:使用荧光素标记微管蛋白进行分析及激光光漂白后荧光重新分布的测量
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6
Analysis of the treadmilling model during metaphase of mitosis using fluorescence redistribution after photobleaching.利用光漂白后的荧光重新分布分析有丝分裂中期的踏车模型。
J Cell Biol. 1986 Mar;102(3):1032-8. doi: 10.1083/jcb.102.3.1032.
7
Monte Carlo simulations of microtubule arrays: The critical roles of rescue transitions, the cell boundary, and tubulin concentration in shaping microtubule distributions.微管阵列的蒙特卡罗模拟:救援跃迁、细胞边界和微管蛋白浓度在塑造微管分布中的关键作用。
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Microtubule dynamics investigated by microinjection of Paramecium axonemal tubulin: lack of nucleation but proximal assembly of microtubules at the kinetochore during prometaphase.通过微注射草履虫轴丝微管蛋白研究微管动力学:前中期动粒处微管缺乏成核但近端组装
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A simple formulation of microtubule dynamics: quantitative implications of the dynamic instability of microtubule populations in vivo and in vitro.
J Cell Sci. 1989 Jun;93 ( Pt 2):241-54. doi: 10.1242/jcs.93.2.241.

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Synergistic suppression of noscapine and conventional chemotherapeutics on human glioblastoma cell growth.纳库啡与常规化疗药物协同抑制人脑胶质瘤细胞生长。
Acta Pharmacol Sin. 2013 Jul;34(7):930-8. doi: 10.1038/aps.2013.40. Epub 2013 May 27.
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Paracrine and epigenetic control of trophectoderm differentiation from human embryonic stem cells: the role of bone morphogenic protein 4 and histone deacetylases.旁分泌和表观遗传控制人类胚胎干细胞滋养外胚层分化:骨形态发生蛋白 4 和组蛋白去乙酰化酶的作用。
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Cytoplasmic linker proteins promote microtubule rescue in vivo.细胞质连接蛋白在体内促进微管挽救。
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Antagonistic forces generated by myosin II and cytoplasmic dynein regulate microtubule turnover, movement, and organization in interphase cells.肌球蛋白II和胞质动力蛋白产生的拮抗力量调节间期细胞中微管的周转、运动和组织。
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Stepwise reconstitution of interphase microtubule dynamics in permeabilized cells and comparison to dynamic mechanisms in intact cells.通透细胞中间期微管动力学的逐步重建及与完整细胞中动力学机制的比较。
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Actomyosin-based retrograde flow of microtubules in the lamella of migrating epithelial cells influences microtubule dynamic instability and turnover and is associated with microtubule breakage and treadmilling.迁移上皮细胞片层中基于肌动球蛋白的微管逆行流动影响微管动态不稳定性和周转,并与微管断裂和踏车行为相关。
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9
Microtubule release from the centrosome.微管从中心体释放。
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10
Microtubule dynamics at the G2/M transition: abrupt breakdown of cytoplasmic microtubules at nuclear envelope breakdown and implications for spindle morphogenesis.G2/M转换期的微管动力学:核膜破裂时胞质微管的突然崩解及其对纺锤体形态发生的影响
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Immunofluorescence and immunocytochemical procedures with affinity purified antibodies: tubulin-containing structures.使用亲和纯化抗体的免疫荧光和免疫细胞化学方法:含微管蛋白的结构
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体内微管动力学:周转机制的检验

Microtubule dynamics in vivo: a test of mechanisms of turnover.

作者信息

Sammak P J, Gorbsky G J, Borisy G G

出版信息

J Cell Biol. 1987 Mar;104(3):395-405. doi: 10.1083/jcb.104.3.395.

DOI:10.1083/jcb.104.3.395
PMID:3546333
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2114545/
Abstract

Clarification of the mechanism of microtubule dynamics requires an analysis of the microtubule pattern at two time points in the same cell with single fiber resolution. Single microtubule resolution was obtained by microinjection of haptenized tubulin (fluorescein-tubulin) and subsequent indirect immunofluorescence with an antifluorescein antibody. The two time points in a single cell were, first, the time of photobleaching fluorescein-tubulin, and second, the time of fixation. The pattern of fluorescence replacement in the bleached zone during this time interval revealed the relevant mechanisms. In fibroblasts, microtubule domains in the bleached zone are replaced microtubule by microtubule and not by mechanisms that affect all microtubules simultaneously. Of the models we consider, treadmilling and subunit exchange along the length do not account for this observation, but dynamic instability can since it suggests that growing and shrinking microtubules coexist. In addition, we show that the half-time for microtubule replacement is shortest at the leading edge. Dynamic instability accounts for this observation if in general microtubules do not catastrophically disassemble from the plus end, but instead have a significant probability of undergoing a transition to the growing phase before they depolymerize completely. This type of instability we call tempered rather than catastrophic because, through limited disassembly followed by regrowth, it will preferentially replace polymer domains at the ends of microtubules, thus accounting for the observation that the half-time of microtubule domain replacement is shorter with proximity to the leading edge.

摘要

阐明微管动力学机制需要在同一细胞内的两个时间点,以单纤维分辨率分析微管模式。通过显微注射半抗原化微管蛋白(荧光素 - 微管蛋白)并随后用抗荧光素抗体进行间接免疫荧光,获得了单微管分辨率。单个细胞内的两个时间点,首先是荧光素 - 微管蛋白光漂白的时间,其次是固定的时间。在此时间间隔内漂白区域荧光替代的模式揭示了相关机制。在成纤维细胞中,漂白区域的微管结构域是微管逐个替代的,而不是通过同时影响所有微管的机制。在我们考虑的模型中,踏车行为和沿长度的亚基交换无法解释这一观察结果,但动态不稳定性可以,因为它表明生长和收缩的微管共存。此外,我们表明微管替代的半衰期在前沿最短。如果一般来说微管不是从正端灾难性地解聚,而是在完全解聚之前有很大概率转变为生长阶段,那么动态不稳定性就能解释这一观察结果。我们将这种类型的不稳定性称为缓和而非灾难性的,因为通过有限的解聚随后再生长,它将优先替代微管末端的聚合物结构域,从而解释了微管结构域替代半衰期随着靠近前沿而缩短的观察结果。