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在两个功能不同的结构域中,速激肽原-A前体近端启动子中的三个立即早期基因反应元件。

Three immediate early gene response elements in the proximal preprotachykinin-A promoter in two functionally distinct domains.

作者信息

Paterson J M, Mendelson S C, McAllister J, Morrison C F, Dobson S, Grace C, Quinn J P

机构信息

MRC Brain Metabolism Unit, Royal Edinburgh Hospital, Edinburgh, U.K.

出版信息

Neuroscience. 1995 Jun;66(4):921-32. doi: 10.1016/0306-4522(95)00041-g.

Abstract

The preprotachykinin-A promoter contains two blocks of DNA sequence, with a high degree of homology to one another, both containing activator protein 1/cAMP response element-like elements which constitute cis-acting regulatory domains. These two domains are differentially regulated in HeLa cells and primary cultures of dorsal root ganglion neurons when they are placed in the context of a reporter gene driven by the c-fos minimum promoter. One of the domains, corresponding to a region of the preprotachykinin promoter spanning nucleotides -345 to -308, contains two activator protein 1 elements adjacent to an E-box binding protein consensus sequence. Both of the activator protein 1 elements can bind a complex containing c-fos/c-fos related antigen proteins and the adjacent E-box element is specifically recognized by proteins present in HeLa nuclear extract. This domain requires the synergistic action of both activator protein 1 elements to drive expression of the reporter gene in both HeLa and dorsal root ganglion cells. The second or proximal domain spans nucleotides -198 to -155 and contains a previously characterized activator protein 1/cAMP response element/ATF enhancer element which, in contrast to the activator protein 1 elements in the distal domain, functions in both HeLa and dorsal root ganglion cells as one copy. This domain is differentially regulated in HeLa and dorsal root ganglia. The previously characterized enhancer activity is repressed in the context of the extended cis-acting domain in HeLa cells but remains active in dorsal root ganglion, although no further enhancement of activity supported by the single enhancer is observed when in the context of the extended sequence. This proximal domain, in addition to binding the enhancer complex, can be bound by at least two other complexes, one of which binds to an E-box consensus sequence. As the elements corresponding to the E-box consensus in both domains cross-compete for binding of specific complex(es) it would appear that repression of the activity of the proximal domain is correlated with a specific protein complex binding adjacent to the characterized enhancer in the region spanning nucleotides -198 to -155. The preprotachykinin-A proximal promoter is therefore bound by multiple activator protein I complexes, which in the context of the cis-acting domains in which they are present can be differentially regulated. In the proximal domain their function may also be regulated in a tissue-specific manner by other proteins which bind to adjacent regulatory elements.

摘要

前速激肽原A启动子包含两个DNA序列区域,它们彼此具有高度同源性,均含有激活蛋白1/cAMP反应元件样元件,这些元件构成顺式作用调节域。当将这两个区域置于由c-fos最小启动子驱动的报告基因的背景下时,它们在HeLa细胞和背根神经节神经元的原代培养物中受到不同的调节。其中一个区域对应于前速激肽原启动子中跨越核苷酸-345至-308的区域,包含两个与E盒结合蛋白共有序列相邻的激活蛋白1元件。这两个激活蛋白1元件都能结合一个包含c-fos/c-fos相关抗原蛋白的复合物,并且相邻的E盒元件能被HeLa细胞核提取物中的蛋白质特异性识别。该区域需要两个激活蛋白1元件的协同作用来驱动报告基因在HeLa细胞和背根神经节细胞中表达。第二个区域或近端区域跨越核苷酸-198至-155,包含一个先前已鉴定的激活蛋白1/cAMP反应元件/ATF增强子元件,与远端区域的激活蛋白1元件不同,该元件在HeLa细胞和背根神经节细胞中作为一个拷贝发挥作用。该区域在HeLa细胞和背根神经节中受到不同的调节。先前鉴定的增强子活性在HeLa细胞的扩展顺式作用域背景下受到抑制,但在背根神经节中仍保持活性,尽管在扩展序列背景下未观察到由单个增强子支持的活性进一步增强。这个近端区域除了能结合增强子复合物外,还能被至少另外两个复合物结合,其中一个复合物能结合E盒共有序列。由于两个区域中与E盒共有序列对应的元件相互竞争特定复合物的结合,因此近端区域活性的抑制似乎与在跨越核苷酸-198至-155的区域中与已鉴定的增强子相邻结合的特定蛋白复合物有关。因此,前速激肽原A近端启动子被多个激活蛋白I复合物结合,在它们所处的顺式作用域背景下,这些复合物可受到不同的调节。在近端区域,它们的功能也可能通过与相邻调节元件结合的其他蛋白质以组织特异性方式进行调节。

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