Zunich Samantha M, Douglas Taneka, Valdovinos Maria, Chang Tiffany, Bushman Wade, Walterhouse David, Iannaccone Philip, Lamm Marilyn L G
Department of Pediatrics, Northwestern University Feinberg School of Medicine, Children's Memorial Research Center, Chicago, IL 60614, USA.
Mol Cancer. 2009 Mar 2;8:12. doi: 10.1186/1476-4598-8-12.
Sonic hedgehog (Shh) and components of its signalling pathway have been identified in human prostate carcinoma and increased levels of their expression appear to correlate with disease progression and metastasis. The mechanism through which Shh signalling could promote metastasis in bone, the most common site for prostate carcinoma metastasis, has not yet been investigated. The present study determined the effect of Shh signalling between prostate cancer cells and pre-osteoblasts on osteoblast differentiation, a requisite process for new bone formation that characterizes prostate carcinoma metastasis.
LNCaP human prostate cancer cells modified to overexpress Shh (designated LNShh cells) and MC3T3 mouse pre-osteoblasts were maintained as mixed populations within the same culture chamber. In this non-conventional mixed culture system, LNShh cells upregulated the expression of Shh target genes Gli1 and Patched 1 (Ptc1) in MC3T3 cells and this was inhibited by cyclopamine, a specific chemical inhibitor of hedgehog signalling. Concomitantly, MC3T3 cells exhibited time-dependent decreased cell proliferation, upregulated alkaline phosphatase Akp2 gene expression, and increased alkaline phosphatase activity indicative of early phase osteoblast differentiation. LNShh cell-induced differentiation was inhibited in MC3T3 cells stably transfected with a dominant negative form of Gli1, a transcription factor that mediates Shh signalling. Interestingly, LNShh cells did not significantly increase the endogenous expression of the osteoblast differentiation transcription factor Runx2 and its target genes osteocalcin and osteopontin. Consistent with these results, exogenous Shh peptide did not upregulate Runx2 expression in MC3T3 cells. However, Runx2 levels were increased in MC3T3 cells by ascorbic acid, a known stimulator of osteoblast differentiation.
Altogether, these data demonstrate that Shh-expressing prostate cancer cells can directly and specifically induce differentiation in pre-osteoblasts via a Gli1-dependent mechanism that does not require transcriptional upregulation of Runx2. Paracrine activation of the Shh pathway in osteoblast progenitors and subsequent induction of osteoblast differentiation could be a mechanism through which high levels of Shh expression in prostate carcinoma contribute to bone metastasis. Targeting of paracrine Shh signalling may provide an effective therapeutic strategy against prostate carcinoma metastasis in bone.
在人类前列腺癌中已鉴定出音猬因子(Shh)及其信号通路的组成部分,其表达水平的升高似乎与疾病进展和转移相关。Shh信号通路促进前列腺癌最常见转移部位——骨转移的机制尚未得到研究。本研究确定了前列腺癌细胞与前成骨细胞之间的Shh信号对成骨细胞分化的影响,成骨细胞分化是新骨形成的一个必要过程,也是前列腺癌转移的特征。
将经修饰过表达Shh的LNCaP人前列腺癌细胞(命名为LNShh细胞)与MC3T3小鼠前成骨细胞作为混合群体维持在同一培养室中。在这种非传统的混合培养系统中,LNShh细胞上调了MC3T3细胞中Shh靶基因Gli1和patched 1(Ptc1)的表达,而这被环杷明(一种刺猬信号通路的特异性化学抑制剂)所抑制。与此同时,MC3T3细胞表现出细胞增殖随时间下降、碱性磷酸酶Akp2基因表达上调以及碱性磷酸酶活性增加,这表明处于成骨细胞分化的早期阶段。在用介导Shh信号的转录因子Gli1的显性负性形式稳定转染的MC3T3细胞中,LNShh细胞诱导的分化受到抑制。有趣的是,LNShh细胞并未显著增加成骨细胞分化转录因子Runx2及其靶基因骨钙素和骨桥蛋白的内源性表达。与这些结果一致,外源性Shh肽并未上调MC3T3细胞中Runx2的表达。然而,已知的成骨细胞分化刺激剂抗坏血酸可使MC3T3细胞中的Runx2水平升高。
总之,这些数据表明,表达Shh的前列腺癌细胞可通过一种不依赖Runx2转录上调的Gli1依赖性机制直接且特异性地诱导前成骨细胞分化。成骨细胞祖细胞中Shh通路的旁分泌激活以及随后的成骨细胞分化诱导可能是前列腺癌中高水平Shh表达导致骨转移的一种机制。靶向旁分泌Shh信号可能为抗前列腺癌骨转移提供一种有效的治疗策略。
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