Lam E, Chua N H
Laboratory of Plant Molecular Biology, Rockefeller University, New York 10021-6399.
Plant Cell. 1989 Dec;1(12):1147-56. doi: 10.1105/tpc.1.12.1147.
We have used nuclear extracts prepared from tobacco leaf tissue to characterize a factor binding site, designated as-2 (activating sequence-2), at the -100 region of the cauliflower mosaic virus 35S promoter. The activity of this factor, called ASF-2 (activating sequence factor-2), is not detected in tobacco root extracts. as-2 includes two GT motifs with sequence homology to the SV40 enhancer core A element and the Box II element of pea rbcS. Nevertheless, oligomers of these sequence elements do not compete for ASF-2 binding in gel retardation assays, indicating that the GT motifs may not be involved. Methylation interference studies identify two guanines (G93 and G98) that are required for interaction with ASF-2. Sequences surrounding these two critical guanines display homologies to a GATA repeat conserved among several light-responsive promoters. One such sequence from a petunia Cab promoter is able to compete with as-2 for factor binding. In transgenic plants, a tetramer of as-2 is able to confer leaf expression when fused 5' to the -90 derivative of the 35S promoter. The expression is not dependent on light and, thus, the as-2 tetramer does not function as a light-responsive element in this context. Histochemical localization of the reporter gene product suggests that the as-2 tetramer directs expression in trichomes, vascular elements, and epidermal and mesophyll cells.
我们利用从烟草叶片组织制备的核提取物,对花椰菜花叶病毒35S启动子 -100区域的一个因子结合位点(命名为-2,即激活序列-2)进行了表征。这种名为ASF-2(激活序列因子-2)的因子活性,在烟草根提取物中未检测到。-2包含两个与SV40增强子核心A元件及豌豆rbcS的Box II元件具有序列同源性的GT基序。然而,这些序列元件的寡聚物在凝胶阻滞分析中并不竞争ASF-2的结合,这表明GT基序可能不参与其中。甲基化干扰研究确定了与ASF-2相互作用所需的两个鸟嘌呤(G93和G98)。这两个关键鸟嘌呤周围的序列与几个光响应启动子中保守的GATA重复序列具有同源性。矮牵牛Cab启动子的一个这样的序列能够与-2竞争因子结合。在转基因植物中,-2的四聚体与35S启动子的-90衍生物5'端融合时,能够赋予叶片表达。该表达不依赖于光,因此,在这种情况下,-2四聚体不作为光响应元件起作用。报告基因产物的组织化学定位表明,-2四聚体在毛状体、维管束、表皮和叶肉细胞中指导表达。