CEU-San Pablo University School of Medicine and Hospital of Madrid Scientific Foundation, Institute of Applied Molecular Medicine, IMMA, Madrid, Spain.
J Transl Med. 2011 Aug 25;9:142. doi: 10.1186/1479-5876-9-142.
Human melanoma frequently colonizes bone marrow (BM) since its earliest stage of systemic dissemination, prior to clinical metastasis occurrence. However, how melanoma cell adhesion and proliferation mechanisms are regulated within bone marrow stromal cell (BMSC) microenvironment remain unclear. Consistent with the prometastatic role of inflammatory and angiogenic factors, several studies have reported elevated levels of cyclooxygenase-2 (COX-2) in melanoma although its pathogenic role in bone marrow melanoma metastasis is unknown.
Herein we analyzed the effect of cyclooxygenase-2 (COX-2) inhibitor celecoxib in a model of generalized BM dissemination of left cardiac ventricle-injected B16 melanoma (B16M) cells into healthy and bacterial endotoxin lipopolysaccharide (LPS)-pretreated mice to induce inflammation. In addition, B16M and human A375 melanoma (A375M) cells were exposed to conditioned media from basal and LPS-treated primary cultured murine and human BMSCs, and the contribution of COX-2 to the adhesion and proliferation of melanoma cells was also studied.
Mice given one single intravenous injection of LPS 6 hour prior to cancer cells significantly increased B16M metastasis in BM compared to untreated mice; however, administration of oral celecoxib reduced BM metastasis incidence and volume in healthy mice, and almost completely abrogated LPS-dependent melanoma metastases. In vitro, untreated and LPS-treated murine and human BMSC-conditioned medium (CM) increased VCAM-1-dependent BMSC adherence and proliferation of B16M and A375M cells, respectively, as compared to basal medium-treated melanoma cells. Addition of celecoxib to both B16M and A375M cells abolished adhesion and proliferation increments induced by BMSC-CM. TNFα and VEGF secretion increased in the supernatant of LPS-treated BMSCs; however, anti-VEGF neutralizing antibodies added to B16M and A375M cells prior to LPS-treated BMSC-CM resulted in a complete abrogation of both adhesion- and proliferation-stimulating effect of BMSC on melanoma cells. Conversely, recombinant VEGF increased adherence to BMSC and proliferation of both B16M and A375M cells, compared to basal medium-treated cells, while addition of celecoxib neutralized VEGF effects on melanoma. Recombinant TNFα induced B16M production of VEGF via COX-2-dependent mechanism. Moreover, exogenous PGE2 also increased B16M cell adhesion to immobilized recombinant VCAM-1.
We demonstrate the contribution of VEGF-induced tumor COX-2 to the regulation of adhesion- and proliferation-stimulating effects of TNFα, from endotoxin-activated bone marrow stromal cells, on VLA-4-expressing melanoma cells. These data suggest COX-2 neutralization as a potential anti-metastatic therapy in melanoma patients at high risk of systemic and bone dissemination due to intercurrent infectious and inflammatory diseases.
人类黑色素瘤在其全身扩散的早期阶段(即在临床转移发生之前)经常在骨髓(BM)中定植。然而,在骨髓基质细胞(BMSC)微环境中,黑色素瘤细胞黏附和增殖的机制是如何调节的仍不清楚。与炎症和血管生成因子的促转移作用一致,尽管环氧化酶-2(COX-2)在黑色素瘤中的致病作用尚不清楚,但已有几项研究报道黑色素瘤中 COX-2 水平升高。
本文分析了 COX-2 抑制剂塞来昔布(celecoxib)在左心室注射 B16 黑色素瘤(B16M)细胞至健康和细菌内毒素脂多糖(LPS)预处理小鼠引发炎症的情况下,对广泛骨髓扩散模型的影响。此外,B16M 和人 A375 黑色素瘤(A375M)细胞暴露于基础和 LPS 处理的原代培养的鼠和人 BMSC 条件培养基中,并研究了 COX-2 对黑色素瘤细胞黏附和增殖的作用。
与未处理的小鼠相比,在癌细胞注射前 6 小时给予小鼠单次静脉注射 LPS 显著增加了 B16M 在 BM 中的转移;然而,口服塞来昔布降低了健康小鼠 BM 转移的发生率和体积,并几乎完全消除了 LPS 依赖性黑色素瘤转移。在体外,未处理和 LPS 处理的鼠和人 BMSC 条件培养基(CM)分别增加了 VCAM-1 依赖性 BMSC 对 B16M 和 A375M 细胞的黏附和增殖,与基础培养基处理的黑色素瘤细胞相比。在 B16M 和 A375M 细胞中加入塞来昔布可消除 BMSC-CM 诱导的黏附和增殖增加。LPS 处理的 BMSCs 的上清液中 TNFα 和 VEGF 分泌增加;然而,在 LPS 处理的 BMSC-CM 加入抗 VEGF 中和抗体可完全消除 BMSC 对黑色素瘤细胞的黏附和增殖刺激作用。相反,重组 VEGF 增加了与基础培养基处理的细胞相比,B16M 和 A375M 细胞对 BMSC 的黏附和增殖,而加入塞来昔布则中和了 VEGF 对黑色素瘤的作用。重组 TNFα 通过 COX-2 依赖性机制诱导 B16M 产生 VEGF。此外,外源性 PGE2 还增加了 B16M 细胞对固定化重组 VCAM-1 的黏附。
我们证明了 VEGF 诱导的肿瘤 COX-2 对 TNFα 从内毒素激活的骨髓基质细胞调节黏附和增殖刺激作用的贡献,在 VLA-4 表达的黑色素瘤细胞上。这些数据表明,COX-2 中和作为一种潜在的抗转移治疗方法,在黑色素瘤患者中具有高风险的全身和骨骼播散,由于并发的感染和炎症性疾病。
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