Ish Tsuyoshi, Sootome Hiroshi, King Alastair J, Suda Mikiya, Noro Nobuhiro, Yamashita Keizo, Noumi Takato, Ishii Tsuyoshi
GlaxoSmithKline K.K., Tsukuba-shi Ibaraki, Japan.
J Biomol Screen. 2007 Sep;12(6):809-17. doi: 10.1177/1087057107303323. Epub 2007 May 21.
Checkpoint kinase 1 (Chk1), a serine/threonine kinase, plays an important role in DNA damage checkpoint control and is an attractive target for cancer treatment. To develop a Chk1-specific cell-based assay, stable clones were established in which Chk1 kinase domain fused at its N-terminus with p53 through 4 tandem repeats of Gly-Gly-Gly-Gly-Ser was expressed in an inducible manner. Chk1 kinase specificity of the phosphorylation of fused p53 was confirmed by the experiments with a kinase-inactive Chk1. Only in the presence of an inducer molecule was phosphorylation of p53 at Ser-15 in the stable clones induced. Furthermore, its assay performance proved acceptable for high-throughput screening applications, judging from the Z' factor values (> 0.77). Finally, the cell-based assay thus established yielded structure-activity relationship data for a small set of test inhibitors of Chk1 within cells. Collectively, these results demonstrate that the established cell-based assay provides a novel and highly sensitive cellular platform for Chk1 inhibitor discovery.
检验点激酶1(Chk1)是一种丝氨酸/苏氨酸激酶,在DNA损伤检验点控制中发挥重要作用,是癌症治疗的一个有吸引力的靶点。为了开发一种基于细胞的Chk1特异性检测方法,构建了稳定克隆,其中Chk1激酶结构域在其N端通过4个Gly-Gly-Gly-Gly-Ser串联重复序列与p53融合,并以可诱导的方式表达。通过对激酶失活的Chk1进行实验,证实了融合p53磷酸化的Chk1激酶特异性。仅在诱导分子存在的情况下,稳定克隆中p53的Ser-15位点才会被诱导磷酸化。此外,从Z'因子值(>0.77)判断,其检测性能对于高通量筛选应用来说是可接受的。最后,由此建立的基于细胞的检测方法为细胞内一小部分Chk1测试抑制剂生成了构效关系数据。总的来说,这些结果表明,所建立的基于细胞的检测方法为Chk1抑制剂的发现提供了一个新颖且高度灵敏的细胞平台。
