用成纤维细胞激活蛋白激活前药靶向肿瘤基质中的癌相关成纤维细胞。
Targeting carcinoma-associated fibroblasts within the tumor stroma with a fibroblast activation protein-activated prodrug.
机构信息
Department of Pharmacology and Molecular Sciences, The Johns Hopkins University, Baltimore, MD, USA.
出版信息
J Natl Cancer Inst. 2012 Sep 5;104(17):1320-34. doi: 10.1093/jnci/djs336. Epub 2012 Aug 21.
BACKGROUND
Fibroblasts undergo a morphological transformation to a reactive phenotype in the tumor microenvironment characterized by the expression of proteins such as fibroblast activation protein (FAP), a post-prolyl endopeptidase with expression largely restricted to carcinoma-associated fibroblasts. Thapsigargin (TG) is a highly toxic natural plant product that triggers a rise in intracellular calcium levels and apoptosis. FAP is therefore a provocative target for the activation of prodrugs consisting of a FAP-specific peptide coupled to a potent cytotoxic analog of TG.
METHODS
The efficacy of FAP-activated peptidyl-TG prodrugs was tested in vitro in cell proliferation assays and effects on intracellular calcium in human cancer cell lines. The effects of FAP-activated prodrugs on tumor growth and host toxicity were tested in Balb-C nude MCF-7 and LNCaP xenograft mice (n = 9-11 per group). P values were calculated using permutation tests based on 50 000 permutations. Mixed effects models were used to account for correlations among replicate measures. All statistical tests were two-sided.
RESULTS
FAP-activated prodrugs killed human cancer cells at low nanomolar concentrations (MCF-7 cells: IC(50) = 3.5 nM). Amino acid-12ADT analogs from FAP-cleaved prodrugs, but not uncleaved prodrugs, produced a rapid rise in intracellular calcium within minutes of exposure. Immunohistochemical analysis of xenografts exposed to FAP-prodrugs documented stromal-selective cell death of fibroblasts, pericytes, and endothelial cells of sufficient magnitude to inhibit growth of MCF-7 and LNCaP xenografts with minimal systemic toxicity, whereas non-FAP cleavable prodrugs were inactive. MCF-7 and LNCaP xenografts treated with a FAP-activated prodrug had maximal treated-to-control tumor volume ratios of 0.36 (treated: mean = 0.206 mm(3), 95% CI = 0.068 to 0.344 mm(3); control: mean = 0.580 mm(3), 95% CI = 0.267 to 0.893 mm(3)) and 0.24 (treated: mean = 0.131 mm(3), 95% CI = 0.09 to 0.180 mm(3); control: mean = 0.543 mm(3), 95% CI = 0.173 to 0.913 mm(3)), respectively, on day 21 after therapy.
CONCLUSIONS
This study validates the proteolytic activity of FAP as a target for the activation of a systemically delivered cytotoxic prodrug and demonstrates that targeted killing of cells within the stromal compartment of the tumor microenvironment can produce a therapeutic response.
背景
成纤维细胞在肿瘤微环境中经历形态转化为反应性表型,其特征是表达成纤维细胞激活蛋白(FAP)等蛋白,FAP 是一种脯氨酰内肽酶,其表达主要局限于癌相关成纤维细胞。他普西加汀(TG)是一种高度毒性的天然植物产物,可引发细胞内钙水平升高和细胞凋亡。因此,FAP 是激活包含 FAP 特异性肽与 TG 有效细胞毒性类似物的前药的有吸引力的靶标。
方法
在细胞增殖测定中测试 FAP 激活的肽-TG 前药在体外的功效,并测试其对人癌细胞系细胞内钙的影响。在 Balb-C 裸鼠 MCF-7 和 LNCaP 异种移植小鼠中测试 FAP 激活的前药对肿瘤生长和宿主毒性的影响(每组 n = 9-11)。使用基于 50000 次置换的置换检验计算 P 值。使用混合效应模型来解释重复测量之间的相关性。所有统计检验均为双侧。
结果
FAP 激活的前药以低纳摩尔浓度(MCF-7 细胞:IC50 = 3.5 nM)杀死人癌细胞。FAP 切割前药的氨基酸 12ADT 类似物,但不是未切割的前药,在暴露后几分钟内迅速引起细胞内钙升高。暴露于 FAP 前药的异种移植物的免疫组织化学分析记录了成纤维细胞、周细胞和内皮细胞的基质选择性细胞死亡,其程度足以抑制 MCF-7 和 LNCaP 异种移植物的生长,而最小的全身毒性,而非 FAP 可切割的前药无活性。用 FAP 激活的前药治疗的 MCF-7 和 LNCaP 异种移植物的最大治疗与对照肿瘤体积比分别为 0.36(治疗:平均值 = 0.206mm3,95%CI = 0.068 至 0.344mm3;对照:平均值 = 0.580mm3,95%CI = 0.267 至 0.893mm3)和 0.24(治疗:平均值 = 0.131mm3,95%CI = 0.09 至 0.180mm3;对照:平均值 = 0.543mm3,95%CI = 0.173 至 0.913mm3),分别在治疗后 21 天。
结论
本研究验证了 FAP 的蛋白水解活性作为一种激活系统递送细胞毒性前药的靶标,并证明靶向杀伤肿瘤微环境基质区室中的细胞可以产生治疗反应。
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