Ogata Y, Niisato N, Furuyama S, Cheifetz S, Kim R H, Sugiya H, Sodek J
Department of Periodontology, Nihon University School of Dentistry at Matsudo, Chiba, Japan.
J Cell Biochem. 1997 Jun 15;65(4):501-12. doi: 10.1002/(sici)1097-4644(19970615)65:4<501::aid-jcb6>3.0.co;2-s.
Transforming growth factor-beta (TGF-beta) increases steady-state mRNA levels of several extracellular matrix proteins in mineralized connective tissues. Bone sialoprotein (BSP) is a major constituent of the bone matrix, thought to initiate and regulate the formation of mineral crystals. To determine the molecular pathways of TGF-beta 1 regulation of bone proteins, we have analyzed the effects of the TGF-beta 1 on the expression of the BSP in the rat osteosarcoma cell line (ROS 17/2.8). TGF-beta 1 at 1 ng/ml, increased BSP mRNA levels in ROS 17/2.8 cells approximately 8-fold: the stimulation was first evident at 3 hr, reached maximal levels at 12 hr and slowly declined thereafter. Since the stability of the BSP mRNA was not significantly affected by TGF-beta 1, and nuclear "run-on" transcription analyses revealed only a approximately 2-fold increase in the transcription of the BSP gene, most of the increase in BSP mRNA appeared to involve a nuclear post-transcriptional mechanism. Moreover, the effects of TGF-beta 1 were indirect, since the increase in BSP mRNA was abrogated by cycloheximide (28 micrograms/ml). To identify the site of transcriptional regulation by TGF-beta 1, transient transfection analyses were performed using BSP gene promoter constructs linked to a luciferase reporter gene. Constructs that included nt -801 to -426 of the promoter sequence were found to enhance transcriptional activity approximately 1.8-fold in cells treated with TGF-beta 1. Within this sequence, approximately 500 nt upstream of the transcription start site, a putative TGF-beta activation element (TAE) was identified that contained the 5'-portion of the nuclear factor-1 (NF-1) canonical sequence (TTGGC) overlapping a consensus sequence for activator protein-2 (AP-2). The functionality of the TAE was shown by an increased binding of a nuclear protein from TGF-beta 1 stimulated cells in gel mobility shift assays and from the attenuation of TGF-beta 1-induced luciferase activity when cells were co-transfected with a double-stranded TAE oligonucleotide. Competition gel mobility shift analyses revealed that the nuclear protein that binds to the TAE has similar properties to, but is distinct from, NF-1 nuclear protein. These studies have therefore identified a TGF-beta activation element (TAE) in the rat BSP gene promoter that mediates the stimulatory effects of TGF-beta 1 on BSP gene transcription.
转化生长因子-β(TGF-β)可增加矿化结缔组织中几种细胞外基质蛋白的稳态mRNA水平。骨唾液蛋白(BSP)是骨基质的主要成分,被认为可启动和调节矿物晶体的形成。为了确定TGF-β1调节骨蛋白的分子途径,我们分析了TGF-β1对大鼠骨肉瘤细胞系(ROS 17/2.8)中BSP表达的影响。1 ng/ml的TGF-β1可使ROS 17/2.8细胞中的BSP mRNA水平增加约8倍:这种刺激在3小时时首次明显,在12小时时达到最高水平,此后缓慢下降。由于TGF-β1对BSP mRNA的稳定性没有显著影响,并且核“连续”转录分析显示BSP基因的转录仅增加约2倍,因此BSP mRNA的大部分增加似乎涉及核转录后机制。此外,TGF-β1的作用是间接的,因为放线菌酮(28微克/毫升)可消除BSP mRNA的增加。为了确定TGF-β1的转录调控位点,使用与荧光素酶报告基因相连的BSP基因启动子构建体进行了瞬时转染分析。发现在用TGF-β1处理的细胞中,包含启动子序列nt -801至-426的构建体可使转录活性增强约1.8倍。在该序列内,转录起始位点上游约500 nt处,鉴定出一个假定的TGF-β激活元件(TAE),其包含核因子-1(NF-1)规范序列(TTGGC)的5'部分,与激活蛋白-2(AP-2)的共有序列重叠。通过凝胶迁移率变动分析中TGF-β1刺激细胞的核蛋白结合增加以及当细胞与双链TAE寡核苷酸共转染时TGF-β1诱导的荧光素酶活性减弱,证明了TAE的功能。竞争凝胶迁移率变动分析表明,与TAE结合的核蛋白具有与NF-1核蛋白相似但不同的特性。因此,这些研究在大鼠BSP基因启动子中鉴定出一个TGF-β激活元件(TAE),其介导TGF-β1对BSP基因转录的刺激作用。
