Hurst R E, Waliszewski P, Waliszewska M, Bonner R B, Benbrook D M, Dar A, Hemstreet G P
Department of Urology, University of Oklahoma Health Sciences Center, Oklahoma City 73190, USA.
Adv Exp Med Biol. 1999;462:449-67. doi: 10.1007/978-1-4615-4737-2_35.
Carcinogenesis involves inactivation or subversion of the normal controls of proliferation, differentiation, and apoptosis. However, these controls are robust, redundant, and interlinked at the gene expression levels, regulation of mRNA lifetimes, transcription, and recycling of proteins. One of the central systems of control of proliferation, differentiation and apoptosis is retinoid signaling. The hRAR alpha nuclear receptor occupies a central position with respect to induction of gene transcription in that when bound to appropriate retinoid ligands, its homodimers and heterodimers with hRXR alpha regulate the transcription of a number of retinoid-responsive genes. These include genes in other signaling pathways, so that the whole forms a complex network. In this study we showed that simple, cause-effect interpretations in terms of hRAR alpha gene transcription being the central regulatory event would not describe the retinoid-responsive gene network. A set of cultured bladder-derived cells representing different stages of bladder tumorigenesis formed a model system. It consisted of 2 immortalized bladder cell lines (HUC-BC and HUC-PC), one squamous cell carcinoma cell line (SCaBER), one papilloma line (RT4), and 4 transitional cell carcinomas (TCC-Sup, 5637, T24, J82) of varying stages and grades. This set of cells were used to model the range of behaviors of bladder cancers. Relative gene expression before (constitutive) and after treatment with 10 microM all-trans-retinoic acid (aTRA) was measured for androgen and estrogen receptor; a set of genes involved with retinoid metabolism and action, hRAR alpha nd beta, hRXR alpha and beta CRBP, CRABP I and II; and for signaling genes that are known to be sensitive to retinoic acid, EGFR, cytokine MK, ICAM I and transglutaminase. The phenotype for inhibition of proliferation and for apoptotic response to both aTRA and the synthetic retinoid 4-HPR was determined. Transfection with a CAT-containing plasmid containing an aTRA-sensitive promoter was used to determine if the common retinoic acid responsive element (RARE)-dependent pathway for retinoid regulation of gene expression was active. Each of the genes selected is known from previous studies to react to aTRA in a certain way, either by up- or down-regulation of the message and protein. A complex data set not readily interpretable by simple cause and effect was observed. While all cell lines expressed high levels of the mRNAs for hRXR alpha and beta that were not altered by treatment with exogenous aTRA, constitutive and stimulated responses of the other genes varied widely among the cell lines. For example, CRABP I was not expressed by J82, T24, 5637 and RT4, but was expressed at low levels that did not change in SCaBER and at moderate levels that decreased, increased, or decreased sharply in HUC-BC, TCC-Sup and HUC-PC, respectively. The expression of hRAR alpha, which governs the expression of many retinoid-sensitive genes, was expressed at moderate to high levels in all cell lines, but in some it was sharply upregulated (TCC-Sup, HUC-PC and J82), remained constant (5637 and HUC-BC), or was down-regulated (SCaBER, T24 and RT4). The phenotypes for inhibition of proliferation showed no obvious relationship to the expression of any single gene, but cell lines that were inhibited by aTRA (HUC-BC and TCC-Sup) were not sensitive to 4-HPR, and vice versa. One line (RT4) was insensitive to either retinoid. Transfection showed very little retinoid-stimulated transfection of the CAT reporter gene with RT4 or HUC-PC. About 2-fold enhancement transactivation was observed with SCaBER, HUC-BC, J82 and T24 cells and 3-8 fold with 5637, TCC-Sup cells. In HUC-BC, a G to T point mutation was found at position 606 of the hRAR alpha gene. This mutation would substitute tyrosine for asparagine in a highly conserved domain. These data indicate that retinoid signaling is probably a frequent target of inactivation in bladder carcinogenesis. (ABSTRAC
致癌作用涉及增殖、分化和凋亡的正常调控机制的失活或颠覆。然而,这些调控机制在基因表达水平、mRNA寿命调控、转录以及蛋白质循环利用方面是强大、冗余且相互关联的。增殖、分化和凋亡调控的核心系统之一是类视黄醇信号传导。hRARα核受体在基因转录诱导方面占据中心地位,因为当与合适的类视黄醇配体结合时,它与hRXRα形成的同源二聚体和异源二聚体可调节许多类视黄醇反应性基因的转录。这些基因包括其他信号通路中的基因,从而形成一个复杂的网络。在本研究中,我们表明,简单地将hRARα基因转录视为核心调控事件的因果解释并不能描述类视黄醇反应性基因网络。一组代表膀胱肿瘤发生不同阶段的培养膀胱来源细胞构成了一个模型系统。它由2个永生化膀胱细胞系(HUC - BC和HUC - PC)、1个鳞状细胞癌细胞系(SCaBER)、1个乳头状瘤细胞系(RT4)以及4个不同阶段和分级的移行细胞癌(TCC - Sup、5637、T24、J82)组成。这组细胞用于模拟膀胱癌的一系列行为。测定了雄激素和雌激素受体在使用10 microM全反式维甲酸(aTRA)处理前后(组成型)的相对基因表达;一组与类视黄醇代谢和作用相关的基因,hRARα和β、hRXRα和β、CRBP、CRABP I和II;以及已知对维甲酸敏感的信号基因,EGFR、细胞因子MK、ICAM I和转谷氨酰胺酶。确定了对增殖抑制以及对aTRA和合成类视黄醇4 - HPR的凋亡反应的表型。用含有aTRA敏感启动子的含CAT质粒进行转染,以确定类视黄醇调节基因表达的常见维甲酸反应元件(RARE)依赖性途径是否活跃。从先前的研究可知,所选的每个基因都会以某种方式对aTRA作出反应,要么通过上调或下调信息和蛋白质。观察到一个不易用简单因果关系解释的复杂数据集。虽然所有细胞系都高水平表达hRXRα和β的mRNA,且外源性aTRA处理未改变其表达,但其他基因的组成型和刺激反应在细胞系之间差异很大。例如,CRABP I在J82、T24、5637和RT4中不表达,但在SCaBER中低水平表达且无变化,在HUC - BC、TCC - Sup和HUC - PC中分别以中等水平表达,且表达水平下降、上升或急剧下降。控制许多类视黄醇敏感基因表达的hRARα在所有细胞系中以中等至高水平表达,但在某些细胞系中它急剧上调(TCC - Sup、HUC - PC和J82),保持恒定(5637和HUC - BC),或下调(SCaBER、T24和RT4)。增殖抑制表型与任何单个基因的表达均无明显关系,但被aTRA抑制的细胞系(HUC - BC和TCC - Sup)对4 - HPR不敏感,反之亦然。一个细胞系(RT4)对任何一种类视黄醇均不敏感。转染显示RT4或HUC - PC对类视黄醇刺激的CAT报告基因转染很少。在SCaBER、HUC - BC、J82和T24细胞中观察到约2倍的增强反式激活,在5637、TCC - Sup细胞中为3 - 8倍。在HUC - BC中,在hRARα基因的606位发现了一个G到T的点突变。该突变会在一个高度保守的结构域中用酪氨酸替代天冬酰胺。这些数据表明,类视黄醇信号传导可能是膀胱致癌过程中失活的常见靶点。(摘要)
