Targeted Mass Spectrometry Enables Quantification of Novel Pharmacodynamic Biomarkers of ATM Kinase Inhibition

Author:

Whiteaker Jeffrey R.ORCID,Wang Tao,Zhao Lei,Schoenherr Regine M.,Kennedy Jacob J.,Voytovich Ulianna,Ivey Richard G.,Huang Dongqing,Lin Chenwei,Colantonio Simona,Caceres Tessa W.,Roberts Rhonda R.,Knotts Joseph G.,Kaczmarczyk Jan A.,Blonder Josip,Reading Joshua J.,Richardson Christopher W.,Hewitt Stephen M.,Garcia-Buntley Sandra S.,Bocik William,Hiltke Tara,Rodriguez Henry,Harrington Elizabeth A.,Barrett J. Carl,Lombardi Benedetta,Marco-Casanova Paola,Pierce Andrew J.ORCID,Paulovich Amanda G.

Abstract

The ATM serine/threonine kinase (HGNC: ATM) is involved in initiation of repair of DNA double-stranded breaks, and ATM inhibitors are currently being tested as anti-cancer agents in clinical trials, where pharmacodynamic (PD) assays are crucial to help guide dose and scheduling and support mechanism of action studies. To identify and quantify PD biomarkers of ATM inhibition, we developed and analytically validated a 51-plex assay (DDR-2) quantifying protein expression and DNA damage-responsive phosphorylation. The median lower limit of quantification was 1.28 fmol, the linear range was over 3 orders of magnitude, the median inter-assay variability was 11% CV, and 86% of peptides were stable for storage prior to analysis. Use of the assay was demonstrated to quantify signaling following ionizing radiation-induced DNA damage in both immortalized lymphoblast cell lines and primary human peripheral blood mononuclear cells, identifying PD biomarkers for ATM inhibition to support preclinical and clinical studies.

Funder

National Cancer Institute

Office of Research Infrastructure Programs, National Institutes of Health

Publisher

MDPI AG

Subject

Cancer Research,Oncology

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