Desai D S, Niles R M
Department of Biochemistry and Molecular Biology, Marshall University School of Medicine, Huntington, West Virginia 25755-9310, USA.
J Cell Physiol. 1995 Nov;165(2):349-57. doi: 10.1002/jcp.1041650216.
Recently, a new subfamily of nuclear retinoid receptors that is distinct from that of RARs has been identified and named Retinoid X receptors (RXRs). These receptors specifically bind 9-cis-retinoic acid (9cisRA), but not all-trans-retinoic acid (ATRA). We determined which RXR subtypes were expressed in B16 mouse melanoma cells and then studied the effect of ATRA, 8-bromo-cyclic AMP (8BrcA), and phorbol dibutyrate (PDB) on RXR mRNA levels. ATRA induces differentiation in these cells while 8BrcA and PDB antagonize the RA-induced differentiation of B16 melanoma cells. Northern analysis demonstrated the expression of RXR alpha and RXR beta mRNA in B16 cells, but RXR gamma was not detectable. Further analysis using RT-PCR also failed to detect RXR gamma in these cells. Long-term RA treatment decreased the expression of RXR alpha, but not RXR beta mRNAs. PDB did not alter the expression of either RXR mRNAs, however, 8BrcA treatment resulted in a time dependent decrease in the amount of RXR beta, but not RXR alpha mRNA. Inhibition of protein synthesis by cycloheximide resulted in a large increase in RXR alpha and RXR beta mRNA levels. This effect of cycloheximide was time and concentration dependent with maximal stimulation of RXR alpha and RXR beta mRNAs occurring at 4 h of treatment. Inhibition of transcription with actinomycin D completely abolished the cycloheximide-induced increase of RXR beta. In contrast to its effect on other genes, such as immediate response genes, cycloheximide treatment did not increase the half-life of RXR beta mRNA. Nuclear run-on assays showed that cycloheximide treatment of intact B16 melanoma cells stimulated the transcription rate of RXR beta, but not RXR alpha. These results suggest the presence of an unstable transcription factor that negatively regulates the expression of RXR beta in B16 melanoma cells. In addition, since RXR beta is the predominant isotype in B16 cells, 8BrcA may, at least partially, inhibit RA-induced differentiation through down-regulation of this RXR.
最近,已鉴定出一个与视黄酸受体(RARs)不同的新型核类视黄醇受体亚家族,并将其命名为视黄酸X受体(RXRs)。这些受体特异性结合9-顺式视黄酸(9cisRA),而非全反式视黄酸(ATRA)。我们确定了哪些RXR亚型在B16小鼠黑色素瘤细胞中表达,然后研究了ATRA、8-溴环磷酸腺苷(8BrcA)和佛波醇二丁酸酯(PDB)对RXR mRNA水平的影响。ATRA可诱导这些细胞分化,而8BrcA和PDB则拮抗RA诱导的B16黑色素瘤细胞分化。Northern分析表明B16细胞中存在RXRα和RXRβ mRNA表达,但未检测到RXRγ。使用逆转录聚合酶链反应(RT-PCR)进一步分析也未能在这些细胞中检测到RXRγ。长期RA处理可降低RXRα的表达,但不影响RXRβ mRNA的表达。PDB未改变任何一种RXR mRNA的表达,然而,8BrcA处理导致RXRβ的量随时间依赖性减少,但不影响RXRα mRNA的表达。用放线菌酮抑制蛋白质合成可导致RXRα和RXRβ mRNA水平大幅增加。放线菌酮的这种作用具有时间和浓度依赖性,在处理4小时时对RXRα和RXRβ mRNA的刺激最大。用放线菌素D抑制转录可完全消除放线菌酮诱导的RXRβ增加。与它对其他基因(如即时反应基因)的作用相反,放线菌酮处理并未增加RXRβ mRNA的半衰期。细胞核连续转录分析表明,用放线菌酮处理完整的B16黑色素瘤细胞可刺激RXRβ的转录速率,但不影响RXRα。这些结果表明存在一种不稳定的转录因子,它对B16黑色素瘤细胞中RXRβ的表达起负调节作用。此外,由于RXRβ是B16细胞中的主要同种型,8BrcA可能至少部分通过下调这种RXR来抑制RA诱导的分化。
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