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流式细胞术全细胞微管分析。

Whole cell microtubule analysis by flow cytometry.

机构信息

Roger Adams Laboratory, Department of Chemistry, University of Illinois at Urbana-Champaign, Urbana, IL 61801, USA.

出版信息

Anal Biochem. 2012 Jan 1;420(1):26-32. doi: 10.1016/j.ab.2011.08.020. Epub 2011 Aug 18.

Abstract

Perturbation of the tubulin/microtubule dynamic in cells is perhaps the single most important mode of action of anticancer drugs. Standard methods for identifying and evaluating compounds for their ability to alter tubulin polymerization are low throughput, labor intensive, expensive, or make their assessment in vitro. Here we report a method to rapidly quantify the extent of tubulin polymerization in whole cells using flow cytometry, and we use this technique to evaluate compounds that stabilize and destabilize microtubule formation. This facile method is useful for conveniently, quantitatively, and cost-effectively comparing small molecules that perturb tubulin polymerization.

摘要

扰乱细胞中的微管蛋白/微管动态可能是抗癌药物的唯一最重要的作用模式。用于识别和评估化合物改变微管聚合能力的标准方法存在通量低、劳动强度大、昂贵或无法在体外进行评估等问题。在这里,我们报告了一种使用流式细胞术快速定量测定全细胞中微管蛋白聚合程度的方法,并使用该技术评估了稳定和破坏微管形成的化合物。这种简单的方法可用于方便、定量和具有成本效益地比较扰乱微管蛋白聚合的小分子。

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