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Engineering REST-Specific Synthetic PUF Proteins to Control Neuronal Gene Expression: A Combined Experimental and Computational Study

机译:工程休息特异性合成PUF蛋白,用于控制神经元基因表达:综合实验和计算研究

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摘要

Regulation of gene transcription is an essential mechanism for differentiation and adaptation of organisms. A key actor in this regulation process is the repressor element 1 (RE1)-silencing transcription factor (REST), a transcriptional repressor that controls more than 2000 putative target genes, most of which are neuron-specific. With the purpose of modulating REST expression, we exploited synthetic, ad hoc designed, RNA binding proteins (RBPs) able to specifically target and dock to REST mRNA. Among the various families of RBPs, we focused on the Pumilio and FBF (PUF) proteins, present in all eukaryotic organisms and controlling a variety of cellular functions. Here, a combined experimental and computational approach was used to design and test 8- and 16-repeat PUF proteins specific for REST mRNA. We explored the conformational properties and atomic features of the PUF-RNA recognition code by Molecular Dynamics simulations. Biochemical assays revealed that the 8- and 16-repeat PUF-based variants specifically bind the endogenous REST mRNA without affecting its translational regulation. The data also indicate a key role of stacking residues in determining the binding specificity. The newly characterized REST-specific PUF-based constructs act as excellent RNA-binding modules and represent a versatile and functional platform to specifically target REST mRNA and modulate its endogenous expression.
机译:基因转录的调节是有机体分化和适应的重要机制。在该调节过程中的关键actor是阻遏物元素1(Re1)-silcing转录因子(静止),其对超过2000个推定的靶基因的转录压缩机,其中大部分是神经元特异性的。目的是调制休息表达的目的,我们利用合成,临时设计,RNA结合蛋白(RBPS)能够特异地靶向和诊断静止mRNA。在rbps的各种家庭中,我们专注于Pumilio和FBF(PUF)蛋白,其在所有真核生物中存在并控制各种细胞功能。这里,使用组合的实验和计算方法来设计和测试特异的静态mRNA的8-重复PUF蛋白。我们通过分子动力学模拟探索了PUF-RNA识别码的构象性质和原子特征。生物化学测定显示出现8-和16-重复的PUF基变体特异性结合内源性静止mRNA而不影响其平移调节。数据还表明堆叠残留在确定结合特异性时的关键作用。新特征的休息特异性PUF的构建体用作优异的RNA结合模块,并且代表多功能和功能平台,以特异性靶向静态mRNA并调节其内源性表达。

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