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使用荧光探针分析组织中的蛋白酶体活性。

Profiling proteasome activity in tissue with fluorescent probes.

作者信息

Berkers Celia R, van Leeuwen Fijs W B, Groothuis Tom A, Peperzak Victor, van Tilburg Erica W, Borst Jannie, Neefjes Jacques J, Ovaa Huib

机构信息

Division of Cellular Biochemistry, Tumor Biology, and Immunology, Netherlands Cancer Institute, Plesmanlaan 121, 1066 CX Amsterdam, The Netherlands.

出版信息

Mol Pharm. 2007 Sep-Oct;4(5):739-48. doi: 10.1021/mp0700256. Epub 2007 Aug 21.

Abstract

With proteasome inhibitors in use in the clinic for the treatment of multiple myeloma and with clinical trials in progress investigating the treatment of a variety of hematologic and solid malignancies, accurate methods that allow profiling of proteasome inhibitor specificity and efficacy in patients are in demand. Here, we describe the development, full biochemical validation, and comparison of fluorescent proteasome activity reporters that can be used to profile proteasome activities in living cells with high sensitivity. Seven of the synthesized probes tested label proteasomes in lysates, although the fluorescent dye used affects their specificity. Two differentially labeled probes tested are suitable for studying proteasome activity in living cells by gel-based assays, by confocal laser scanning microscopy, and by flow cytometry. We established methods using these fluorescent reporters to profile proteasome activity in different mouse tissues, carefully avoiding postlysis artifacts, and we show that proteasome subunit activity is regulated in an organ-specific manner. The techniques described here could be used to study in vivo pharmacological properties of proteasome inhibitors.

摘要

随着蛋白酶体抑制剂在临床上用于治疗多发性骨髓瘤,并且针对多种血液系统恶性肿瘤和实体恶性肿瘤的治疗正在进行临床试验,因此需要准确的方法来分析蛋白酶体抑制剂在患者中的特异性和疗效。在此,我们描述了荧光蛋白酶体活性报告分子的开发、全面的生化验证及其比较,这些报告分子可用于高灵敏度地分析活细胞中的蛋白酶体活性。所测试的七种合成探针可标记裂解物中的蛋白酶体,尽管所使用的荧光染料会影响它们的特异性。所测试的两种差异标记探针适用于通过基于凝胶的分析、共聚焦激光扫描显微镜和流式细胞术研究活细胞中的蛋白酶体活性。我们建立了使用这些荧光报告分子分析不同小鼠组织中蛋白酶体活性的方法,小心避免裂解后假象,并且我们表明蛋白酶体亚基活性以器官特异性方式受到调节。本文所述技术可用于研究蛋白酶体抑制剂的体内药理学特性。

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