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稳定的、去酪氨酸化的微管在成纤维细胞中发挥作用,使波形蛋白中间丝定位。

Stable, detyrosinated microtubules function to localize vimentin intermediate filaments in fibroblasts.

作者信息

Gurland G, Gundersen G G

机构信息

Department of Pathology, Columbia University, College of Physicians and Surgeons, New York 10032, USA.

出版信息

J Cell Biol. 1995 Dec;131(5):1275-90. doi: 10.1083/jcb.131.5.1275.

Abstract

Separate populations of microtubules (MTs) distinguishable by their level of posttranslationally modified tubulin subunits and by their stability in vivo have been described. In polarized 3T3 cells at the edge of an in vitro wound, we have found a striking preferential coalignment of vimentin intermediate filaments (IFs) with detyrosinated MTs (Glu MTs) rather than with the bulk of the MTs, which were tyrosinated MTs (Tyr MTs). Vimentin IFs were not stabilizing the Glu MTs since collapse of the IF network to a perinuclear location, induced by microinjection of monoclonal anti-IF antibody, had no noticeable effect on the array of Glu MTs. To test whether Glu MTs may affect the organization of IFs we regrew MTs in cells that had been treated with nocodazole to depolymerize all the MTs and to collapse IFs; the reextension of IFs into the lamella lagged behind the rapid regrowth of Tyr MTs, but was correlated with the slower reformation of Glu MTs. Similar realignment of IFs with newly formed Glu MTs was observed in serum-starved cells treated with either serum or taxol to induce the formation of Glu MTs. Next, we microinjected affinity purified antibodies specific for Glu tubulin (polyclonal SG and monoclonal 4B8) and specific for Tyr tubulin (polyclonal W2 and monoclonal YL1/2) into 3T3 cells. Both injected SG and 4B8 antibodies labeled the subset of endogenous Glu MTs; W2 and YL1/2 antibodies labeled virtually all of the cytoplasmic MTs. Injection of SG or 4B8 resulted in the collapse of IFs to a perinuclear region. This collapse was comparable to that observed after complete MT depolymerization by nocodazole. Injection of W2, YL1/2, or nonspecific control IgGs did not result in collapse of the IFs. Taken together, these results show that Glu MTs localize IFs in migrating 3T3 fibroblasts and suggest that detyrosination of tubulin acts as a signal for the recruitment of vimentin IFs to MTs.

摘要

已描述了不同群体的微管(MTs),它们可通过翻译后修饰的微管蛋白亚基水平以及在体内的稳定性来区分。在体外伤口边缘的极化3T3细胞中,我们发现波形蛋白中间丝(IFs)与去酪氨酸化的MTs(Glu MTs)有显著的优先共排列,而不是与大部分酪氨酸化的MTs(Tyr MTs)共排列。波形蛋白IFs并没有稳定Glu MTs,因为通过显微注射单克隆抗IF抗体诱导IF网络向核周位置塌陷,对Glu MTs阵列没有明显影响。为了测试Glu MTs是否可能影响IFs的组织,我们在已用诺考达唑处理以解聚所有MTs并使IFs塌陷的细胞中重新生长MTs;IFs向片层的重新延伸落后于Tyr MTs的快速重新生长,但与Glu MTs的较慢重新形成相关。在用血清或紫杉醇处理以诱导Glu MTs形成的血清饥饿细胞中,观察到IFs与新形成的Glu MTs有类似的重新排列。接下来,我们将针对Glu微管蛋白的亲和纯化抗体(多克隆SG和单克隆4B8)以及针对Tyr微管蛋白的抗体(多克隆W2和单克隆YL1/2)显微注射到3T3细胞中。注射的SG和4B8抗体均标记内源性Glu MTs的子集;W2和YL1/2抗体几乎标记了所有细胞质MTs。注射SG或4B8导致IFs塌陷到核周区域。这种塌陷与诺考达唑完全解聚MTs后观察到的塌陷相当。注射W2、YL1/2或非特异性对照IgG不会导致IFs塌陷。综上所述,这些结果表明Glu MTs在迁移的3T3成纤维细胞中定位IFs,并表明微管蛋白去酪氨酸化作为波形蛋白IFs募集到MTs的信号。

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