Cummings Jeffrey, Hodgkinson Cassandra, Odedra Rajesh, Sini Patrizia, Heaton Simon P, Mundt Kirsten E, Ward Tim H, Wilkinson Robert W, Growcott Jim, Hughes Andrew, Dive Caroline
Clinical and Experimental Pharmacology, Paterson Institute for Cancer Research, University of Manchester, Manchester, UK.
Mol Cancer Ther. 2008 Mar;7(3):455-63. doi: 10.1158/1535-7163.MCT-07-2136.
M30 and M65 are ELISAs that detect different circulating forms of cytokeratin 18. Using the aurora kinase inhibitor AZD1152 and the SW620 human colon cancer xenograft, experiments were conducted to qualify preclinically both assays as serologic biomarkers of cell death. Using two different apoptotic markers, the kinetics of cell death induced by AZD1152 was first characterized in vitro in three different cell lines and shown to peak 5 to 7 days after drug addition. Treatment of non-tumor-bearing rats with AZD1152 (25 mg/kg) produced no alterations in circulating baseline values of M30 and M65 antigens. In treated, tumor-bearing animals, M30 detected a 2- to 3-fold (P < 0.05) increase in plasma antigen levels by day 5 compared with controls. This correlated to a 3-fold increase in the number of apoptotic cells detected on day 5 in SW620 xenografts using immunohistochemistry. By contrast, M65 did not detect a drug-induced increase in circulating antigen levels at day 5. However, M65 plasma levels correlated to changes in tumor growth in control animals (r(2) = 0.93; P < 0.01) and also followed the magnitude of the temporal effect of AZD1152 on tumor growth. An intermediate but active dose of AZD1152 (12.5 mg/kg) produced a less significant increase in M30 plasma levels at day 5. It was also confirmed that the plasma profiles of M30 and M65 mirrored closely those measured in whole tumor lysates. We conclude that M30 is a pharmacodynamic biomarker of AZD1152-induced apoptosis in the SW620 xenograft model, whereas M65 is a biomarker of therapeutic response.
M30和M65是用于检测细胞角蛋白18不同循环形式的酶联免疫吸附测定(ELISA)。使用极光激酶抑制剂AZD1152和SW620人结肠癌异种移植模型,进行实验以在临床前将这两种测定鉴定为细胞死亡的血清生物标志物。使用两种不同的凋亡标志物,首先在三种不同的细胞系中体外表征AZD1152诱导的细胞死亡动力学,结果显示在添加药物后5至7天达到峰值。用AZD1152(25mg/kg)处理无肿瘤大鼠,未导致M30和M65抗原的循环基线值发生改变。在接受治疗的荷瘤动物中,与对照组相比,M30在第5天时检测到血浆抗原水平增加了2至3倍(P<0.05)。这与使用免疫组织化学在第5天检测到的SW620异种移植瘤中凋亡细胞数量增加3倍相关。相比之下,M65在第5天时未检测到药物诱导的循环抗原水平增加。然而,M65血浆水平与对照动物肿瘤生长的变化相关(r²=0.93;P<0.01),并且也遵循AZD1152对肿瘤生长的时间效应幅度。中等但有效的剂量AZD1152(12.5mg/kg)在第5天时使M30血浆水平的增加不太显著。还证实了M30和M65的血浆谱与在整个肿瘤裂解物中测得的谱密切反映。我们得出结论,在SW620异种移植模型中,M30是AZD1152诱导凋亡的药效学生物标志物,而M65是治疗反应的生物标志物。
