一种内源性血管生成抑制剂与人肺癌细胞中的侧群表型和功能呈负相关。
An endogenous inhibitor of angiogenesis inversely correlates with side population phenotype and function in human lung cancer cells.
机构信息
Radiation Oncology Branch, Center for Cancer Research, National Cancer Institute, the National Institutes of Health, Advanced Technology Center, Bethesda, MD, USA.
出版信息
Oncogene. 2014 Feb 27;33(9):1198-206. doi: 10.1038/onc.2013.61. Epub 2013 Mar 11.
The side population (SP) in human lung cancer cell lines and tumors is enriched with cancer stem cells. An endogenous inhibitor of angiogenesis known as tissue inhibitor of matrix metalloproteinase-2 (TIMP-2), characterized for its ability to inhibit matrix metalloproteinases (MMPs), has been shown by several laboratories to impede tumor progression through MMP-dependent or -independent mechanisms. We recently reported that forced expression of TIMP-2, as well as the modified form Ala+TIMP-2 (that lacks MMP inhibitory activity) significantly blocks growth of A549 human lung cancer cells in vivo. However, the mechanisms underlying TIMP-2 antitumor effects are not fully characterized. Here, we examine the hypothesis that the TIMP-2 antitumor activity may involve regulation of the SP in human lung cancer cells. Indeed, using Hoechst dye efflux assay and flow cytometry, as well as quantitative reverse transcriptase-PCR analysis, we found that endogenous TIMP-2 mRNA levels showed a significant inverse correlation with SP fraction size in six non-small cell lung cancer cell lines. In A549 cells expressing increased levels of TIMP-2, a significant decrease in SP was observed, and this decrease was associated with lowered gene expression of ABCG2, ABCB1 and AKR1C1. Functional analysis of A549 cells showed that TIMP-2 overexpression increased chemosensitivity to cytotoxic drugs. The SP isolated from TIMP-2-overexpressing A549 cells also demonstrated impaired migratory capacity compared with the SP from empty vector control. More importantly, our data provide strong evidence that these TIMP-2 functions occur independent of MMP inhibition, as A549 cells overexpressing Ala+TIMP-2 exhibited identical behavior to those overexpressing TIMP-2 alone. Our findings provide the first indication that TIMP-2 modulates SP phenotype and function, and suggests that TIMP-2 may act as an endogenous suppressor of the SP in human lung cancer cells.
人肺癌细胞系和肿瘤中的侧群(SP)富含癌症干细胞。基质金属蛋白酶抑制剂-2(TIMP-2)是一种内源性血管生成抑制剂,其特征是能够抑制基质金属蛋白酶(MMPs),已经有几个实验室表明,它通过 MMP 依赖性或非依赖性机制阻碍肿瘤进展。我们最近报道,强制表达 TIMP-2 以及缺乏 MMP 抑制活性的修饰形式 Ala+TIMP-2 显著阻止了 A549 人肺癌细胞在体内的生长。然而,TIMP-2 抗肿瘤作用的机制尚未完全阐明。在这里,我们检验了这样一种假设,即 TIMP-2 的抗肿瘤活性可能涉及到对人肺癌细胞 SP 的调节。事实上,我们使用 Hoechst 染料外排实验和流式细胞术以及定量逆转录-PCR 分析,发现 6 种非小细胞肺癌细胞系中内源性 TIMP-2 mRNA 水平与 SP 分数大小呈显著负相关。在表达高水平 TIMP-2 的 A549 细胞中,观察到 SP 显著减少,并且这种减少与 ABCG2、ABCB1 和 AKR1C1 基因表达降低有关。A549 细胞的功能分析表明,TIMP-2 过表达增加了对细胞毒药物的敏感性。与空载体对照相比,从 TIMP-2 过表达的 A549 细胞中分离出的 SP 也表现出迁移能力受损。更重要的是,我们的数据提供了强有力的证据,表明这些 TIMP-2 功能的发生独立于 MMP 抑制,因为过表达 Ala+TIMP-2 的 A549 细胞表现出与单独过表达 TIMP-2 的细胞相同的行为。我们的发现首次表明 TIMP-2 调节 SP 表型和功能,并表明 TIMP-2 可能作为人肺癌细胞中 SP 的内源性抑制物发挥作用。
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