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用冈田酸处理的活细胞中微管动态周转的刺激作用。

Stimulation of microtubule dynamic turnover in living cells treated with okadaic acid.

作者信息

Shelden E, Wadsworth P

机构信息

Department of Anatomy and Cell Biology, University of Michigan Medical School, Ann Arbor, USA.

出版信息

Cell Motil Cytoskeleton. 1996;35(1):24-34. doi: 10.1002/(SICI)1097-0169(1996)35:1<24::AID-CM2>3.0.CO;2-I.

Abstract

We have examined the effects of okadaic acid, an inhibitor of protein phosphatases type 1 and 2A, on the dynamic instability behavior of individual microtubules in living cells. Addition of 1 microM okadaic acid to PtK1 epithelial cells induced ruffling of lamellar regions; after 50 min in okadaic acid, many cells were observed to round up. Confocal microscopy of okadaic acid-treated cells stained with an antibody to tubulin showed that microtubules were more densely packed near the periphery of the rounded cells, and in many cells, a reduction in the density of microtubules near the microtubule-organizing center was observed. The dynamic behavior of individual microtubules in cells previously injected with rhodamine-labeled tubulin was quantified by tracking individual microtubules from image sequences. Microtubule dynamic turnover was markedly stimulated in cells treated with 1 microM okadaic acid for 50-60 min: The average rates of both microtubule growing and shortening increased, and the average duration of pause, or attenuation, a phase in which neither growth nor shortening could be detected, was significantly decreased. Further, okadaic acid induced an approximately twofold increase in the frequency of catastrophe transitions and a threefold decrease in the frequency of rescue transitions. Dynamicity, a measure of the net gain and loss of polymer at microtubule plus ends, increased nearly threefold in okadaic acid-treated cells. These results demonstrate that microtubule turnover is stimulated in okadaic acid-treated cells and suggest that phosphorylation of molecules which interact with microtubules may result in increased microtubule dynamic turnover in vivo.

摘要

我们研究了冈田酸(一种1型和2A型蛋白磷酸酶抑制剂)对活细胞中单个微管动态不稳定性行为的影响。向PtK1上皮细胞中添加1微摩尔的冈田酸会诱导片状区域出现褶皱;在冈田酸中处理50分钟后,观察到许多细胞变圆。用抗微管蛋白抗体对经冈田酸处理的细胞进行共聚焦显微镜观察显示,在变圆细胞的周边附近微管堆积更为密集,并且在许多细胞中,观察到微管组织中心附近微管密度降低。通过跟踪图像序列中的单个微管,对先前注射了罗丹明标记微管蛋白的细胞中单个微管的动态行为进行了量化。在用1微摩尔冈田酸处理50 - 60分钟的细胞中,微管动态周转明显受到刺激:微管生长和缩短的平均速率均增加,并且暂停或衰减阶段(在此阶段既检测不到生长也检测不到缩短)的平均持续时间显著缩短。此外,冈田酸使灾难转换频率增加约两倍,救援转换频率降低三倍。动态性(一种衡量微管正端聚合物净增减的指标)在经冈田酸处理的细胞中增加了近三倍。这些结果表明,在经冈田酸处理的细胞中微管周转受到刺激,并表明与微管相互作用的分子的磷酸化可能导致体内微管动态周转增加。

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