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开发和验证高通量分析筛选 HDAC6 选择性抑制剂。

Development and Validation of High-Content Analysis for Screening HDAC6-Selective Inhibitors.

机构信息

Discovery Project Unit, HitGen, Chengdu, Sichuan, China.

出版信息

SLAS Discov. 2021 Jun;26(5):628-641. doi: 10.1177/24725552211002463. Epub 2021 Mar 30.

Abstract

Throughout recent decades, histone deacetylase (HDAC) inhibitors have shown encouraging potential in cancer treatment, and several pan-HDAC inhibitors have been approved for treating malignant cancers. Numerous adverse effects of pan-HDAC inhibitors have been reported, however, during preclinical and clinical evaluations. To avoid undesirable responses, an increasing number of investigations are focusing on the development of isotype-selective HDAC inhibitors. In this study, we present an effective and quantitative cellular assay using high-content analysis (HCA) to determine compounds' inhibition of the activity of HDAC6 and Class I HDAC isoforms, by detecting the acetylation of their corresponding substrates (i.e., α-tubulin and histone H3). Several conditions that are critical for HCA assays, such as cell seeding number, fixation and permeabilization reagent, and antibody dilution, have been fully validated in this study. We used selective HDAC6 inhibitors and inhibitors targeting different HDAC isoforms to optimize and validate the capability of the HCA assay. The results indicated that the HCA assay is a robust assay for quantifying compounds' selectivity of HDAC6 and Class I HDAC isoforms in cells. Moreover, we screened a panel of compounds for HDAC6 selectivity using this HCA assay, which provided valuable information for the structure-activity relationship (SAR). In summary, our results suggest that the HCA assay is a powerful tool for screening selective HDAC6 inhibitors.

摘要

在过去几十年中,组蛋白去乙酰化酶(HDAC)抑制剂在癌症治疗中显示出了令人鼓舞的潜力,并且已经有几种泛 HDAC 抑制剂被批准用于治疗恶性癌症。然而,在临床前和临床评估中,已经报道了许多泛 HDAC 抑制剂的不良反应。为了避免不良反应,越来越多的研究致力于开发同工型选择性 HDAC 抑制剂。在这项研究中,我们提出了一种有效的、基于高通量分析(HCA)的定量细胞测定方法,用于通过检测其相应底物(即α-微管蛋白和组蛋白 H3)的乙酰化来确定化合物对 HDAC6 和 I 类 HDAC 同工型活性的抑制作用。在这项研究中,我们充分验证了 HCA 测定中几个关键条件,如细胞接种数量、固定和透化试剂以及抗体稀释度。我们使用选择性 HDAC6 抑制剂和针对不同 HDAC 同工型的抑制剂来优化和验证 HCA 测定的能力。结果表明,HCA 测定是一种用于定量测定细胞中化合物对 HDAC6 和 I 类 HDAC 同工型选择性的强大测定方法。此外,我们使用该 HCA 测定法筛选了一组化合物对 HDAC6 的选择性,这为结构-活性关系(SAR)提供了有价值的信息。总之,我们的结果表明,HCA 测定法是筛选选择性 HDAC6 抑制剂的有力工具。

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