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A tryptophan-rich peptide acts as a transcription activation domain

机译:富含色氨酸的肽充当转录激活域

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Eukaryotic transcription activators normally consist of a sequence-specific DNA-binding domain (DBD) and a transcription activation domain (AD). While many sequence patterns and motifs have been defined for DBDs, ADs do not share easily recognizable motifs or structures. We report herein that the N-terminal domain of yeast valyl-tRNA synthetase can function as an AD when fused to a DNA-binding protein, LexA, and turn on reporter genes with distinct LexA-responsive promoters. The transcriptional activity was mainly attributed to a five-residue peptide, WYDWW, near the C-terminus of the N domain. Remarkably, the pentapeptide per se retained much of the transcriptional activity. Mutations which substituted tryptophan residues for both of the non-tryptophan residues in the pentapeptide (resulting in W5) significantly enhanced its activity (~1.8-fold), while mutations which substituted aromatic residues with alanine residues severely impaired its activity. Accordingly, a much more active peptide, pentatryptophan (W7), was produced, which elicited ~3-fold higher activity than that of the native pentapeptide and the N domain. Further study indicated that W7 mediates transcription activation through interacting with the general transcription factor, TFIIB. Since W7 shares no sequence homology or features with any known transcription activators, it may represent a novel class of AD.
机译:真核转录激活因子通常由序列特异性DNA结合域(DBD)和转录激活域(AD)组成。尽管已经为DBD定义了许多序列模式和基序,但AD并不共享易于识别的基序或结构。我们在此报告,当与DNA结合蛋白LexA融合时,酵母缬氨酰tRNA合成酶的N末端结构域可作为AD,并以不同的LexA反应性启动子开启报告基因。转录活性主要归因于N结构域C端附近的五残基肽WYDWW。值得注意的是,五肽本身保留了许多转录活性。用五肽中的两个非色氨酸残基取代色氨酸残基的突变(导致W5)显着增强了其活性(约1.8倍),而用丙氨酸残基取代芳族残基的突变则严重削弱了其活性。因此,产生了活性更高的肽五色氨酸(W7),其活性比天然五肽和N结构域高约3倍。进一步的研究表明W7通过与一般转录因子TFIIB相互作用来介导转录激活。由于W7与任何已知的转录激活因子均不具有序列同源性或特征,因此它可以代表一类新颖的AD。

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