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Electrophoretic mobility shift assay reveals a novel recognition sequence for Setaria italica NAC protein

机译:电泳迁移率变化分析揭示了一种新的识别方法即Setaria italica NAC蛋白

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摘要

The NAC (NAM/ATAF1,2/CUC2) proteins are among the largest family of plant transcription factors. Its members have been associated with diverse plant processes and intricately regulate the expression of several genes. Inspite of this immense progress, knowledge of their DNA-binding properties are still limited. In our recent publication, we reported isolation of a membrane-associated NAC domain protein from Setaria italica (SiNAC). Transactivation analysis revealed that it was a functionally active transcription factor as it could stimulate expression of reporter genes in vivo. Truncation of the transmembrane region of the protein lead to its nuclear localization. Here we describe expression and purification of SiNAC DNA-binding domain. We further report identification of a novel DNA-binding site, [C/G][A/T] [T/A][G/C]TC[C/G][A/T][C/G][G/C] for SiNAC by electrophoretic mobility shift assay. The SiNAC-GST protein could bind to the NAC recognition sequence in vitro as well as to sequences where some bases had been reshuffled. The results presented here contribute to our understanding of the DNA-binding specificity of SiNAC protein.
机译:NAC(NAM / ATAF1,2 / CUC2)蛋白是植物转录因子的最大家族。其成员已与多种植物过程相关联,并复杂地调节了几种基因的表达。尽管取得了如此巨大的进展,但对其DNA结合特性的了解仍然有限。在我们最近的出版物中, 我们报道了从Setaria italica(SiNAC)中分离出一种膜相关的NAC域蛋白。反式激活分析显示它是一种功能活跃的转录因子,因为它可以刺激体内报道基因的表达。蛋白质跨膜区域的截短导致其核定位。在这里,我们描述了SiNAC DNA结合域的表达和纯化。我们进一步报告鉴定了一种新型的DNA结合位点[C / G] [A / T] [T / A] [G / C] TC [C / G] [A / T] [C / G] [G / C],通过电泳迁移率变动分析。 SiNAC-GST蛋白可以在体外与NAC识别序列以及某些碱基已改组的序列结合。这里介绍的结果有助于我们对SiNAC蛋白的DNA结合特异性的理解。

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