Singh Balraj, Berry Jacob A, Shoher Angela, Ramakrishnan Vijay, Lucci Anthony
Michael E. DeBakey Department of Surgery, Baylor College of Medicine, Houston, TX 77030, USA.
Int J Oncol. 2005 May;26(5):1393-9.
Cyclooxygenase-2 (COX-2), an inducible enzyme involved in prostaglandin (including PGE(2)) biosynthesis, is overexpressed in several epithelial malignancies including breast cancer. We tested the hypothesis that COX-2 overexpression in breast cancer cells results in increased cell motility and invasion. COX-2 overproducing cells were generated by stable transfection of several human breast cancer cells with pSG5-COX2 vector. We confirmed the overexpression of COX-2 protein by western blotting, and by measuring PGE(2) in the medium with an immunoassay. We measured cell motility by counting the number of cells crossing an 8-micron pore size PET membrane, and cell invasion by counting the number of cells invading through a Matrigel-coated membrane that simulates basement membrane. COX-2 transfected MDA-231 cells produced 30-43-fold more PGE2 as compared to parental cells. COX-2 overexpression increased cell migration approximately 2.2-fold and cell invasion through Matrigel approximately 5.1-fold. Addition of 50 microM NS-398, a COX-2 inhibitor, inhibited Matrigel invasion of MDA-231 cells by 54% as compared to solvent confirming the role of COX-2 in cell invasion. It is known that an increase in cell migration and invasion can be brought about by cytoskeletal alterations and basement membrane degradation due to increased expression of pro-urokinase plasminogen activator (pro-uPA). To investigate the mechanism of our observed increase in cell invasion by COX-2, we found by western blotting that the level of pro-uPA was significantly higher (approximately 5-fold) in COX-2 transfected MDA-231 cells than untransfected MDA-231 cells. Similar to our observations in cell culture, we found evidence that increased COX-2 activity correlates with uPA in a mouse model of breast cancer metastasis to bone. In this study, we conclude that COX-2 overexpression in human breast cancer cells enhances cell motility and invasiveness thus suggesting a mechanism of COX-2 mediated metastasis.
环氧化酶-2(COX-2)是一种参与前列腺素(包括PGE₂)生物合成的诱导酶,在包括乳腺癌在内的多种上皮恶性肿瘤中过度表达。我们验证了一个假说,即乳腺癌细胞中COX-2的过度表达会导致细胞运动性和侵袭性增加。通过用pSG5-COX2载体稳定转染几种人乳腺癌细胞,产生了COX-2过量产生的细胞。我们通过蛋白质印迹法以及用免疫测定法测量培养基中的PGE₂,证实了COX-2蛋白的过度表达。我们通过计算穿过8微米孔径PET膜的细胞数量来测量细胞运动性,并通过计算穿过模拟基底膜的基质胶包被膜的细胞数量来测量细胞侵袭性。与亲本细胞相比,COX-2转染的MDA-231细胞产生的PGE₂多30至43倍。COX-2的过度表达使细胞迁移增加约2.2倍,使穿过基质胶的细胞侵袭增加约5.1倍。加入50微摩尔的COX-2抑制剂NS-398,与溶剂相比,抑制了MDA-231细胞对基质胶的侵袭54%,证实了COX-2在细胞侵袭中的作用。已知细胞迁移和侵袭的增加可由前尿激酶型纤溶酶原激活剂(pro-uPA)表达增加导致的细胞骨架改变和基底膜降解引起。为了研究我们观察到的COX-2导致细胞侵袭增加的机制,我们通过蛋白质印迹法发现,COX-2转染的MDA-231细胞中pro-uPA的水平比未转染的MDA-231细胞显著更高(约5倍)。与我们在细胞培养中的观察结果相似,我们发现在乳腺癌转移至骨的小鼠模型中,COX-2活性增加与uPA相关的证据。在本研究中,我们得出结论,人乳腺癌细胞中COX-2的过度表达增强了细胞运动性和侵袭性,从而提示了COX-2介导转移的机制。
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