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大鼠前脑啡肽原DNA结合蛋白:5'侧翼区

Preproenkephalin DNA-binding proteins in the rat: 5' flanking region.

作者信息

La Gamma E F, Goldstein N K, Snyder J B, Weisinger G

机构信息

Department of Pediatrics and Neurobiology, SUNY, Stony Brook 11794-8111.

出版信息

Brain Res Mol Brain Res. 1989 Mar;5(2):131-40. doi: 10.1016/0169-328x(89)90004-1.

Abstract

Various extracellular signals (i.e. transmitters, hormones, growth factors, etc.), together with their respective second-messenger pathways, regulate transmitter biosynthesis and neuronal function by altering gene expression. In this study we validated a protocol for isolating rat striatum and adrenal medullary nuclei for the purpose of extracting, identifying, and characterizing, nuclear regulatory factors which may serve a functional role in signal-transduction processes. Through gel retardation studies using a 299 base pair (bp) XmnI-SacI 32P-labeled probe (derived from the 5' untranslated region of the rat preproenkephalin gene), we show that different patterns of retained bands result from nuclear extracts derived from rat adrenal medulla and striatum (as well as from other tissue). These tissue differences may have biological significance since rat adrenal medullae have low basal enkephalin levels while the striatum has high levels of this peptide and its respective mRNA. Additionally, certain retained bands were common to both cytosolic and nuclear compartments, suggesting binding factors may be located in either cell space. An initial biochemical characterization of these factors was also undertaken. Generally, salt levels of 100 mM or more reduced factor binding while 10-50 mM sodium ion levels showed preferentially enhanced bands. Binding activity appeared optimal at pH 6.8. As all retained bands were abrogated by proteinase K treatment, these factors appear to have a significant protein component. Finally, of particular interest is that this 299 bp region contains many sequences showing over 80% sequence identity with several previously characterized transcriptional control elements (i.e. cAMP and phorbol ester inducible enhancers, GCN4, AP1, Sp1, CCAAT binding factor, ATF, and AP2). If binding is confirmed (footprint analysis) and function validated (transfection studies), the evolutionary significance of the apparent presence of gene regulatory sequences and functional element divergence of the DNA region between different species can be evaluated.

摘要

各种细胞外信号(即递质、激素、生长因子等)及其各自的第二信使途径,通过改变基因表达来调节递质生物合成和神经元功能。在本研究中,我们验证了一种用于分离大鼠纹状体和肾上腺髓质核的方案,目的是提取、鉴定和表征可能在信号转导过程中发挥功能作用的核调节因子。通过使用299碱基对(bp)的XmnI - SacI 32P标记探针(源自大鼠前脑啡肽原基因的5'非翻译区)进行凝胶阻滞研究,我们表明,来自大鼠肾上腺髓质和纹状体(以及其他组织)的核提取物产生了不同的保留带模式。这些组织差异可能具有生物学意义,因为大鼠肾上腺髓质的基础脑啡肽水平较低,而纹状体中这种肽及其相应mRNA的水平较高。此外,某些保留带在胞质和核区室中都很常见,这表明结合因子可能位于任何一个细胞空间中。我们还对这些因子进行了初步的生化表征。一般来说,100 mM或更高的盐浓度会降低因子结合,而10 - 50 mM的钠离子浓度则会优先增强条带。结合活性在pH 6.8时似乎最佳。由于所有保留带都被蛋白酶K处理消除,这些因子似乎具有重要的蛋白质成分。最后,特别值得关注的是,这个299 bp区域包含许多与几个先前表征的转录控制元件(即cAMP和佛波酯诱导增强子、GCN4、AP1、Sp1、CCAAT结合因子、ATF和AP2)显示出超过80%序列同一性的序列。如果结合得到证实(足迹分析)且功能得到验证(转染研究),就可以评估不同物种之间该DNA区域基因调控序列明显存在和功能元件差异的进化意义。

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