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Quantification of Cellular Poly(ADP-ribosyl)ation by Stable Isotope Dilution Mass Spectrometry Reveals Tissue- and Drug-Dependent Stress Response Dynamics

机译:通过稳定同位素稀释质谱法定量细胞多聚(aDp-核糖基),揭示组织和药物依赖性应激反应动力学

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Poly(ADP-ribosyl)ation is an essential post-translational modification with the biopolymer poly(ADP-ribose) (PAR). The reaction is catalyzed by poly(ADP-ribose) polymerases (PARPs) and plays key roles in cellular physiology and stress response. PARP inhibitors are currently being tested in clinical cancer treatment, in combination therapy, or as monotherapeutic agents by inducing synthetic lethality. We have developed an accurate and sensitive bioanalytical platform based on isotope dilution mass spectrometry in order to quantify steady-state and stress-induced PAR levels in cells and tissues and to characterize pharmacological properties of PARP inhibitors. In contrast to existing PAR-detection techniques, the LC–MS/MS method uses authentic isotope-labeled standards, which provide unequivocal chemical specificity to quantify cellular PAR in absolute terms with femtomol sensitivity. Using this platform we analyzed steady-state levels as well as stress-induced dynamics of poly(ADP-ribosyl)ation in a series of biological systems including cancer cell lines, mouse tissues, and primary human lymphocytes. Our results demonstrate a rapid and transient stress-induced increase in PAR levels by >100-fold in a dose- and time-dependent manner with significant differences between cell types and individual human lymphocyte donors. Furthermore, ex vivo pharmacodynamic studies in human lymphocytes provide new insight into pharmacological properties of clinically relevant PARP inhibitors. Finally, we adapted the LC–MS/MS method to quantify poly(ADP-ribosyl)ation in solid tissues and identified tissue-dependent associations between PARP1 expression and PAR levels in a series of different mouse organs. In conclusion, this study demonstrates that mass spectrometric quantification of cellular poly(ADP-ribosyl)ation has a wide range of applications in basic research as well as in drug development.
机译:聚(ADP-核糖)化是生物聚合物聚(ADP-核糖)(PAR)的重要翻译后修饰。该反应由聚(ADP-核糖)聚合酶(PARP)催化,在细胞生理学和应激反应中起关键作用。 PARP抑制剂目前正在临床癌症治疗中,联合治疗中或通过诱导合成致死性作为单一治疗剂进行测试。我们已经开发了一种基于同位素稀释质谱的准确而灵敏的生物分析平台,以便量化细胞和组织中的稳态和应激诱导的PAR水平,并表征PARP抑制剂的药理特性。与现有的PAR检测技术相比,LC-MS / MS方法使用可靠的同位素标记的标准品,该标准品具有毫不含糊的化学特异性,可以以毫微微摩尔灵敏度对绝对量的细胞PAR进行定量。使用该平台,我们分析了一系列生物系统(包括癌细胞系,小鼠组织和原代人淋巴细胞)中的稳态水平以及聚(ADP-核糖基)化的应力诱导动力学。我们的结果表明,剂量和时间依赖的方式使瞬时和短暂的应激诱导的PAR水平升高> 100倍,并且细胞类型与单个人类淋巴细胞供体之间存在显着差异。此外,人淋巴细胞的体外药效学研究为临床相关的PARP抑制剂的药理特性提供了新的见识。最后,我们采用LC-MS / MS方法对实体组织中的聚(ADP-核糖基)进行定量,并鉴定了一系列不同小鼠器官中PARP1表达与PAR水平之间的组织依赖性关联。总之,这项研究表明,细胞多聚(ADP-核糖基)的质谱定量分析在基础研究和药物开发中具有广泛的应用。

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