Targeting renal cell carcinoma with a HIF-2 antagonist

舒尼替尼 癌症研究 肾透明细胞癌 癌变 血管生成 缺氧诱导因子 肾细胞癌 生物 转录因子 HIF1A型 基因签名 酪氨酸激酶抑制剂 基因 癌症 基因表达 医学 内科学 遗传学
作者
Wenfang Chen,Haley Hill,Alana Christie,Min Soo Kim,Eboni Holloman,Andrea Pavía-Jiménez,Farrah Homayoun,Yuanqing Ma,Nirav Patel,Paul C. Yell,Guiyang Hao,Qurratulain Yousuf,Allison Joyce,Iván Pedrosa,Heather Geiger,He Zhang,Jenny H. Chang,Kevin H. Gardner,Richard K. Bruick,Catherine Reeves,Tae Hyun Hwang,Kevin D. Courtney,Eugene P. Frenkel,Xiankai Sun,Naseem J. Zojwalla,Tai W. Wong,James P. Rizzi,Eli M. Wallace,John A. Josey,Yang Xie,Xian‐Jin Xie,Payal Kapur,Renée M. McKay,James Brugarolas
出处
期刊:Nature [Nature Portfolio]
卷期号:539 (7627): 112-117 被引量:535
标识
DOI:10.1038/nature19796
摘要

Clear cell renal cell carcinoma (ccRCC) is characterized by inactivation of the von Hippel-Lindau tumour suppressor gene (VHL). Because no other gene is mutated as frequently in ccRCC and VHL mutations are truncal, VHL inactivation is regarded as the governing event. VHL loss activates the HIF-2 transcription factor, and constitutive HIF-2 activity restores tumorigenesis in VHL-reconstituted ccRCC cells. HIF-2 has been implicated in angiogenesis and multiple other processes, but angiogenesis is the main target of drugs such as the tyrosine kinase inhibitor sunitinib. HIF-2 has been regarded as undruggable. Here we use a tumourgraft/patient-derived xenograft platform to evaluate PT2399, a selective HIF-2 antagonist that was identified using a structure-based design approach. PT2399 dissociated HIF-2 (an obligatory heterodimer of HIF-2α-HIF-1β) in human ccRCC cells and suppressed tumorigenesis in 56% (10 out of 18) of such lines. PT2399 had greater activity than sunitinib, was active in sunitinib-progressing tumours, and was better tolerated. Unexpectedly, some VHL-mutant ccRCCs were resistant to PT2399. Resistance occurred despite HIF-2 dissociation in tumours and evidence of Hif-2 inhibition in the mouse, as determined by suppression of circulating erythropoietin, a HIF-2 target and possible pharmacodynamic marker. We identified a HIF-2-dependent gene signature in sensitive tumours. Gene expression was largely unaffected by PT2399 in resistant tumours, illustrating the specificity of the drug. Sensitive tumours exhibited a distinguishing gene expression signature and generally higher levels of HIF-2α. Prolonged PT2399 treatment led to resistance. We identified binding site and second site suppressor mutations in HIF-2α and HIF-1β, respectively. Both mutations preserved HIF-2 dimers despite treatment with PT2399. Finally, an extensively pretreated patient whose tumour had given rise to a sensitive tumourgraft showed disease control for more than 11 months when treated with a close analogue of PT2399, PT2385. We validate HIF-2 as a target in ccRCC, show that some ccRCCs are HIF-2 independent, and set the stage for biomarker-driven clinical trials.

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