Faculty of Life Sciences, The Michael Smith Building, University of Manchester, Oxford Road, Manchester M13 9PT, UK.
Mol Cell. 2010 Jan 29;37(2):159-71. doi: 10.1016/j.molcel.2009.12.023.
The Wilms' tumor suppressor protein WT1 functions as a transcriptional regulator of genes controlling growth, apoptosis, and differentiation. It has become clear that WT1 can act as an oncogene in many tumors, primarily through the inhibition of apoptosis. Here, we identify the serine protease HtrA2 as a WT1 binding partner and find that it cleaves WT1 at multiple sites following the treatment of cells with cytotoxic drugs. Ablation of HtrA2 activity either by chemical inhibitor or by siRNA prevents the proteolysis of WT1 under apoptotic conditions. Moreover, the apoptosis-dependent cleavage of WT1 is defective in HtrA2 knockout cells. Proteolysis of WT1 by HtrA2 causes the removal of WT1 from its binding sites at gene promoters, leading to alterations in gene regulation that enhance apoptosis. Our findings provide insights into the function of HtrA2 in the regulation of apoptosis and the oncogenic activities of WT1.
Wilms 肿瘤抑制蛋白 WT1 作为控制生长、凋亡和分化的基因的转录调节剂发挥作用。现已清楚,WT1 可在许多肿瘤中作为致癌基因发挥作用,主要是通过抑制细胞凋亡。在这里,我们鉴定出丝氨酸蛋白酶 HtrA2 是 WT1 的结合伴侣,并发现它在细胞用细胞毒性药物处理后可在多个位点切割 WT1。通过化学抑制剂或 siRNA 消除 HtrA2 的活性可防止在凋亡条件下 WT1 的蛋白水解。此外,在 HtrA2 敲除细胞中,凋亡依赖性 WT1 的切割是有缺陷的。HtrA2 对 WT1 的蛋白水解导致 WT1 从基因启动子上的结合位点被去除,导致增强凋亡的基因调控改变。我们的研究结果为 HtrA2 在凋亡调控和 WT1 的致癌活性中的功能提供了新的认识。
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