Department of Pharmacology, Case Western Reserve University, Cleveland, OH, USA.
Cell Cycle. 2011 Feb 1;10(3):500-6. doi: 10.4161/cc.10.3.14753.
In response to DNA damage, cells launch elegant networks of genome surveillance mechanisms, called cell cycle checkpoints, to detect and repair damaged DNA to maintain the genome stability. Key components of cell cycle checkpoints are two PI3K-related protein kinases (PIKK), ATR and ATM, which participate in both sensing the DNA damage and transducing the damage signal through phosphorylating two target protein kinases, Chk1 and Chk2, respectively. However, how exactly cell cycle checkpoints are activated, maintained, and terminated are not completely understood. Given the complexity of the cell cycle checkpoint signaling and the cellular environment, systems that can faithfully mimic the cell cycle checkpoint activation in vitro, such as the Xenopus egg extracts, are of extreme value in dissecting the precise molecular mechanisms underlying DNA damage response. Here we describe that the well-established in vitro transcription and translation (IVTNT) system has the capability to induce protein phosphorylation of substrates for ATR or ATM, including Chk1, Rad17, and ATM itself. These phosphorylation events highly mimic those occurring in cells when treated with DNA damaging agents. Our results demonstrate that the IVTNT system could be developed into a novel in vitro system to facilitating the dissecting of mechanisms leading to cell cycle checkpoint activation in vivo.
针对 DNA 损伤,细胞启动了一系列精巧的基因组监测机制,称为细胞周期检查点,以检测和修复受损的 DNA,从而维持基因组的稳定性。细胞周期检查点的关键组成部分是两种与 PI3K 相关的蛋白激酶(PIKK),ATR 和 ATM,它们分别参与了 DNA 损伤的感应和通过磷酸化两个靶蛋白激酶 Chk1 和 Chk2 来传递损伤信号。然而,细胞周期检查点如何被激活、维持和终止的机制还不完全清楚。鉴于细胞周期检查点信号传递的复杂性和细胞环境的复杂性,能够在体外真实模拟细胞周期检查点激活的系统,如非洲爪蟾卵提取物,对于解析 DNA 损伤反应的精确分子机制具有极高的价值。在这里,我们描述了成熟的体外转录和翻译(IVTNT)系统能够诱导 ATR 或 ATM 的底物蛋白磷酸化,包括 Chk1、Rad17 和 ATM 本身。这些磷酸化事件与用 DNA 损伤剂处理细胞时发生的事件高度相似。我们的结果表明,IVTNT 系统可以开发成一种新的体外系统,有助于解析导致体内细胞周期检查点激活的机制。
