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The comparison of aggregation and folding of enhanced green fluorescent protein (EGFP) by spectroscopic studies

机译:光谱研究增强绿色荧光蛋白(EGFP)聚集和折叠的比较

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GFP (Green Fluorescent Protein) is well known for its unique chromophore which is formed by autocatalytic cyclization of a polypeptide backbone of Ser65, Tyr66 and Gly67, and is able to emit green visible light. Due to unusual chromophore responsible for the fluorescence GFP and its mutants (e.g., EGFP) have become widely used reporter proteins in molecular biology and biotechnology. GFP can easily be fused to any protein of interest and co-expressed in cells; the GFP fluorescence is then used to visualize the distribution, transport and aggregation of the protein in the cell. However, GFP has a tendency to aggregate itself, and also formation of its chromophore critically depends on the presence of reducing agents. Therefore we have undertaken spectroscopic kinetic studies of EGFP folding and aggregation as a function of pH, and in the presence of various reducing agents, to study the competition between these two processes. The best conditions for folding of EGFP provides BME as a reducing agent. Aggregation of EGFP depends strongly on pH, and on the concentration of the protein. The careful control experiments must therefore be performed during investigations of proteins fused with EGFP, especially at pH lower than 7.
机译:GFP(绿色荧光蛋白)以其独特的生色团而闻名,该生色团是通过Ser65,Tyr66和Gly67多肽骨架的自催化环化形成的,并能够发出绿色可见光。由于负责荧光GFP的不常见的生色团及其突变体(例如EGFP)已成为分子生物学和生物技术中广泛使用的报告蛋白。 GFP可以很容易地与任何目标蛋白融合,并在细胞中共表达。然后使用GFP荧光可视化蛋白质在细胞中的分布,转运和聚集。然而,GFP具有自身聚集的趋势,并且其生色团的形成也关键地取决于还原剂的存在。因此,我们进行了EGFP折叠和聚集作为pH的函数的光谱动力学研究,并在存在各种还原剂的情况下研究了这两个过程之间的竞争。折叠EGFP的最佳条件是BME作为还原剂。 EGFP的聚集在很大程度上取决于pH值和蛋白质的浓度。因此,在研究与EGFP融合的蛋白质时,尤其是在pH值低于7的蛋白质期间,必须进行仔细的对照实验。

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