Androutsopoulos Vasilis, Arroo Randolph R J, Hall John F, Surichan Somchaiya, Potter Gerry A
Leicester School of Pharmacy, De Montfort University, The Gateway, Leicester, UK.
Breast Cancer Res. 2008;10(3):R39. doi: 10.1186/bcr2090. Epub 2008 May 2.
The natural product eupatorin has been reported to have antiproliferative activity in tumour cell lines, but the exact mechanism is unclear. The cytochromes P450 CYP1B1, CYP1A1, and CYP1A2 have been shown to participate in the activation of various xenobiotics, compounds derived from the diet as well as chemotherapeutic drugs. CYP1B1 and CYP1A1 have also been proposed as targets for cancer chemotherapy for their differential and selective overexpression in tumour cells. In this study, we aimed to identify a possible mechanism of action for the antiproliferative effect of eupatorin, which can be attributed to CYP1 family-mediated metabolism.
The study focuses on the antiproliferative action of eupatorin on the human breast carcinoma cell line MDA-MB-468 and on a cell line derived from normal mammary tissue, MCF-10A. The cytotoxicity of the flavone, its effect on the cell cycle of the abovementioned cell lines, and its metabolism by CYP1 family enzymes were examined.
Eupatorin showed a dose-dependent inhibitory effect of cell growth on MDA-MB-468 cells with a submicromolar median inhibition concentration (IC50) whereas the IC50 of this compound in MCF-10A cells was considerably higher. The antiproliferative effect, as measured by EROD (ethoxyresorufin-O-deethylase) assay and Western immunoblotting, was attributed mainly to CYP1A1 expression in MDA-MB-468 cells but not in MCF-10A cells. Moreover, CYP1 family enzymes were shown to metabolise eupatorin in vitro to the flavone cirsiliol and two other unidentified metabolites. Metabolism of eupatorin was also detected in MDA-MB-468 cell cultures, whereas metabolism by MCF-10A cells was negligible. Eupatorin was further shown to arrest the cell cycle of the CYP1-expressing cell line MDA-MB-468 in G2/M phase, whereas no effect was observed in MCF-10A cells, which do not express CYP1 enzymes. The effect of eupatorin on the MDA-MB-468 cell cycle could be reversed by co-application of the CYP1 inhibitor acacetin.
The flavone eupatorin is selectively activated in breast cancer cells, but not in normal breast cells, due to CYP1 family metabolism. This provides a basis for selectivity which is desired against breast tumour cells. In this sense, eupatorin is shown by this study to be a very promising chemopreventative candidate that should be examined further in an in vivo study.
据报道,天然产物灯盏乙素在肿瘤细胞系中具有抗增殖活性,但其确切机制尚不清楚。细胞色素P450 CYP1B1、CYP1A1和CYP1A2已被证明参与各种外源性物质、饮食来源的化合物以及化疗药物的激活过程。CYP1B1和CYP1A1也因其在肿瘤细胞中的差异和选择性过表达而被提议作为癌症化疗的靶点。在本研究中,我们旨在确定灯盏乙素抗增殖作用的一种可能作用机制,该机制可归因于CYP1家族介导的代谢。
本研究聚焦于灯盏乙素对人乳腺癌细胞系MDA-MB-468和源自正常乳腺组织的细胞系MCF-10A的抗增殖作用。检测了黄酮类化合物的细胞毒性、其对上述细胞系细胞周期的影响以及其被CYP1家族酶的代谢情况。
灯盏乙素对MDA-MB-468细胞的生长具有剂量依赖性抑制作用,中位抑制浓度(IC50)为亚微摩尔级别,而该化合物在MCF-10A细胞中的IC50则高得多。通过EROD(乙氧基异吩恶唑酮-O-脱乙基酶)测定和Western免疫印迹法测定的抗增殖作用主要归因于MDA-MB-468细胞中CYP1A1的表达,而在MCF-10A细胞中则不然。此外,CYP1家族酶在体外可将灯盏乙素代谢为黄酮类化合物刺槐素和另外两种未鉴定的代谢产物。在MDA-MB-468细胞培养物中也检测到了灯盏乙素的代谢,而MCF-10A细胞的代谢可忽略不计。进一步研究表明,灯盏乙素可使表达CYP1的细胞系MDA-MB-468的细胞周期停滞在G2/M期,而在不表达CYP1酶的MCF-10A细胞中未观察到这种作用。灯盏乙素对MDA-MB-468细胞周期的影响可通过共同应用CYP1抑制剂金合欢素而逆转。
由于CYP1家族的代谢作用,黄酮类化合物灯盏乙素在乳腺癌细胞中被选择性激活,而在正常乳腺细胞中则不然。这为针对乳腺肿瘤细胞的选择性提供了基础。从这个意义上讲,本研究表明灯盏乙素是一种非常有前景的化学预防候选药物,应在体内研究中进一步考察。
Zotero 插件
