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FRET study of membrane proteins: determination of the tilt and orientation of the N-terminal domain of M13 major coat protein.

机译:膜蛋白的FRET研究:测定M13主要外壳蛋白N末端结构域的倾斜和方向。

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摘要

A formalism for membrane protein structure determination was developed. This method is based on steady-state FRET data and information about the position of the fluorescence maxima on site-directed fluorescent labeled proteins in combination with global data analysis utilizing simulation-based fitting. The methodology was applied to determine the structural properties of the N-terminal domain of the major coat protein from bacteriophage M13 reconstituted into unilamellar DOPC/DOPG (4:1 mol/mol) vesicles. For our purpose, the cysteine mutants A7C, A9C, N12C, S13C, Q15C, A16C, S17C, and A18C in the N-terminal domain of this protein were produced and specifically labeled with the fluorescence probe AEDANS. The energy transfer data from the natural Trp-26 to AEDANS were analyzed assuming a two-helix protein model. Furthermore, the polarity Stokes shift of the AEDANS fluorescence maxima is taken into account. As a result the orientation and tilt of the N-terminal protein domain with respect to the bilayer interface were obtained, showing for the first time, to our knowledge, an overall alpha-helical protein conformation from amino acid residues 12-46, close to the protein conformation in the intact phage.
机译:建立了膜蛋白结构测定的形式学。该方法基于稳态FRET数据和有关定点荧光标记蛋白上荧光最大值位置的信息,并结合基于模拟的全局数据分析。应用该方法来确定重组为单层DOPC / DOPG(4:1 mol / mol)囊泡的噬菌体M13的主要外壳蛋白N末端结构域的结构特性。为了我们的目的,产生了在该蛋白质的N末端结构域中的半胱氨酸突变体A7C,A9C,N12C,S13C,Q15C,A16C,S17C和A18C,并用荧光探针AEDANS进行了特异性标记。假设两螺旋蛋白质模型,分析了从天然Trp-26到AEDANS的能量转移数据。此外,还考虑了AEDANS荧光最大值的极性斯托克斯位移。结果,获得了N末端蛋白结构域相对于双层界面的取向和倾斜,据我们所知,这首次显示出氨基酸残基12-46的总体α-螺旋蛋白构象,接近完整噬菌体中的蛋白质构象。

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