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开发一种新型可扩增系统,用于定量检测活细胞中的过氧化氢。

Development of a Novel Amplifiable System to Quantify Hydrogen Peroxide in Living Cells.

机构信息

Verna and Marrs McLean Department of Biochemistry and Molecular Pharmacology, Baylor College of Medicine, Houston, Texas 77030, United States.

Center for NextGen Therapeutics, Baylor College of Medicine, Houston, Texas 77030, United States.

出版信息

J Am Chem Soc. 2024 Aug 14;146(32):22396-22404. doi: 10.1021/jacs.4c05366. Epub 2024 Jul 30.

Abstract

Although many redox signaling molecules are present at low concentrations, typically ranging from micromolar to submicromolar levels, they often play essential roles in a wide range of biological pathways and disease mechanisms. However, accurately measuring low-abundant analytes has been a significant challenge due to the lack of sensitivity and quantitative capability of existing measurement methods. In this study, we introduced a novel chemically induced amplifiable system for quantifying low-abundance redox signaling molecules in living cells. We utilized HO as a proof-of-concept analyte and developed a probe that quantifies cellular peroxide levels by combining the NanoBiT system with androgen receptor dimerization as a reporting mechanism. Our system demonstrated a highly sensitive response to cellular peroxide changes induced both endogenously and exogenously. Furthermore, the system can be adapted for the quantification of other signaling molecules if provided with suitable probing chemistry.

摘要

虽然许多氧化还原信号分子的浓度很低,通常在微摩尔到亚微摩尔的范围内,但它们在广泛的生物途径和疾病机制中起着至关重要的作用。然而,由于现有测量方法的灵敏度和定量能力有限,准确测量低丰度分析物一直是一个重大挑战。在本研究中,我们引入了一种新的化学诱导可扩增系统,用于定量活细胞中低丰度氧化还原信号分子。我们利用 HO 作为概念验证分析物,并开发了一种探针,通过将 NanoBiT 系统与雄激素受体二聚化结合作为报告机制,来定量细胞内过氧化物水平。我们的系统对细胞内过氧化物变化的响应具有高度的敏感性,无论是内源诱导还是外源诱导。此外,如果提供合适的探测化学物质,该系统可以适应其他信号分子的定量。

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