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ATM 激酶活性的分子成像。

Molecular imaging of the ATM kinase activity.

机构信息

Department of Radiation Oncology, Ohio State University, Columbus, Ohio, USA.

出版信息

Int J Radiat Oncol Biol Phys. 2013 Aug 1;86(5):969-77. doi: 10.1016/j.ijrobp.2013.04.028. Epub 2013 May 29.

Abstract

PURPOSE

Ataxia telangiectasia mutated (ATM) is a serine/threonine kinase critical to the cellular DNA-damage response, including from DNA double-strand breaks. ATM activation results in the initiation of a complex cascade of events including DNA damage repair, cell cycle checkpoint control, and survival. We sought to create a bioluminescent reporter that dynamically and noninvasively measures ATM kinase activity in living cells and subjects.

METHODS AND MATERIALS

Using the split luciferase technology, we constructed a hybrid cDNA, ATM-reporter (ATMR), coding for a protein that quantitatively reports on changes in ATM kinase activity through changes in bioluminescence.

RESULTS

Treatment of ATMR-expressing cells with ATM inhibitors resulted in a dose-dependent increase in bioluminescence activity. In contrast, induction of ATM kinase activity upon irradiation resulted in a decrease in reporter activity that correlated with ATM and Chk2 activation by immunoblotting in a time-dependent fashion. Nuclear targeting improved ATMR sensitivity to both ATM inhibitors and radiation, whereas a mutant ATMR (lacking the target phosphorylation site) displayed a muted response. Treatment with ATM inhibitors and small interfering (si)RNA-targeted knockdown of ATM confirm the specificity of the reporter. Using reporter expressing xenografted tumors demonstrated the ability of ATMR to report in ATM activity in mouse models that correlated in a time-dependent fashion with changes in Chk2 activity.

CONCLUSIONS

We describe the development and validation of a novel, specific, noninvasive bioluminescent reporter that enables monitoring of ATM activity in real time, in vitro and in vivo. Potential applications of this reporter include the identification and development of novel ATM inhibitors or ATM-interacting partners through high-throughput screens and in vivo pharmacokinetic/pharmacodynamic studies of ATM inhibitors in preclinical models.

摘要

目的

共济失调毛细血管扩张突变基因(ATM)是丝氨酸/苏氨酸激酶,对细胞 DNA 损伤反应至关重要,包括 DNA 双链断裂。ATM 的激活导致一系列复杂事件的启动,包括 DNA 损伤修复、细胞周期检查点控制和存活。我们试图创建一种生物发光报告器,可动态且非侵入性地测量活细胞和活体中的 ATM 激酶活性。

方法和材料

使用分裂萤光素酶技术,我们构建了一个杂交 cDNA,即 ATM 报告器(ATMR),编码一种通过生物发光变化定量报告 ATM 激酶活性变化的蛋白质。

结果

用 ATM 抑制剂处理表达 ATMR 的细胞会导致生物发光活性呈剂量依赖性增加。相比之下,照射诱导 ATM 激酶活性会导致报告活性降低,这与免疫印迹显示 ATM 和 Chk2 激活呈时间依赖性相关。核靶向提高了 ATMR 对 ATM 抑制剂和辐射的敏感性,而缺乏靶磷酸化位点的突变 ATMR 则显示出反应迟钝。用 ATM 抑制剂和靶向 ATM 的小干扰 RNA(siRNA)处理证实了报告器的特异性。用表达报告器的异种移植肿瘤证明了该报告器能够报告在小鼠模型中的 ATM 活性,该活性与 Chk2 活性的变化呈时间依赖性相关。

结论

我们描述了一种新型、特异、非侵入性生物发光报告器的开发和验证,该报告器可实时监测体外和体内的 ATM 活性。该报告器的潜在应用包括通过高通量筛选鉴定和开发新型 ATM 抑制剂或与 ATM 相互作用的伙伴,以及在临床前模型中对 ATM 抑制剂进行药代动力学/药效学的体内研究。

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