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首页> 外文期刊>Scientific reports. >Specific modification at the C-terminal lysine residue of the green fluorescent protein variant, GFPuv, expressed in Escherichia coli
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Specific modification at the C-terminal lysine residue of the green fluorescent protein variant, GFPuv, expressed in Escherichia coli

机译:在大肠杆菌中表达的绿色荧光蛋白变体GFPuv的C端赖氨酸残基的特异性修饰

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Green fluorescent protein (GFP) is amenable to recombinant expression in various kinds of cells and is widely used in life science research. We found that the recombinant expression of GFPuv, a commonly-used mutant of GFP, in E. coli produced two distinct molecular species as judged by in-gel fluorescence SDS-PAGE. These molecular species, namely form I and II, could be separately purified by anion-exchange chromatography without any remarkable differences in the fluorescence spectra. Mass spectrometric analyses revealed that the molecular mass of form I is almost the same as the calculated value, while that of form II is approximately 1?Da larger than that of form I. Further mass spectrometric top-down sequencing pinpointed the modification in GFPuv form II, where the ε-amino group of the C-terminal Lys238 residue is converted into the hydroxyl group. No equivalent modification was observed in the native GFP in jellyfish Aequorea victoria, suggesting that this modification is not physiologically relevant. Crystal structure analysis of the two species verified the structural identity of the backbone and the vicinity of the chromophore. The modification found in this study may also be generated in other GFP variants as well as in other recombinant expression systems.
机译:绿色荧光蛋白(GFP)适于在各种细胞中进行重组表达,并广泛用于生命科学研究。我们发现,通过凝胶内荧光SDS-PAGE判断,GFPuv(GFP的常用突变体)在大肠杆菌中的重组表达产生了两个不同的分子种类。这些分子种类,即形式I和II,可以通过阴离子交换色谱法分别纯化,而荧光光谱没有任何显着差异。质谱分析显示,形式I的分子量几乎与计算值相同,而形式II的分子量比形式I大约大1?Da。进一步的质谱自上而下测序准确地指出了GFPuv形式的修饰II,其中C末端Lys238残基的ε-氨基被转化为羟基。在水母维多利亚水母中的天然GFP中未观察到等效修饰,表明该修饰在生理上不相关。两种物质的晶体结构分析证实了骨架和发色团附近的结构特征。在这项研究中发现的修饰也可能在其他GFP变体以及其他重组表达系统中产生。

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