Przybylski M, Glocker M O, Nestel U, Schnaible V, Blüggel M, Diederichs K, Weckesser J, Schad M, Schmid A, Welte W, Benz R
Universitat Konstanz, Fakultat fur Chemie, Germany.
Protein Sci. 1996 Aug;5(8):1477-89. doi: 10.1002/pro.5560050804.
The role of charges near the pore mouth has been discussed in theoretical work about ion channels. To introduce new negative charges in a channel protein, amino groups of porin from Rhodobacter capsulatus 37b4 were succinylated with succinic anhydride, and the precise extent and sites of succinylations and structures of the succinylporins determined by mass spectrometry and X-ray crystallography. Molecular weight and peptide mapping analyses using matrix-assisted laser desorption-ionization mass spectrometry identified selective succinylation of three lysine-epsilon-amino groups (Lys-46, Lys-298, Lys-300) and the N-terminal alpha-amino group. The structure of a tetra-succinylated porin (TS-porin) was determined to 2.4 A and was generally found unchanged in comparison to native porin to form a trimeric complex. All succinylated amino groups found in a mono/di-succinylated porin (MS-porin) and a TS-porin are localized at the inner channel surface and are solvent-accessible: Lys-46 is located at the channel constriction site, whereas Lys-298, Lys-300, and the N-terminus are all near the periplasmic entrance of the channel. The Lys-46 residue at the central constriction loop was modeled as succinyl-lysine from the electron density data and shown to bend toward the periplasmic pore mouth. The electrical properties of the MS-and TS-porins were determined by reconstitution into black lipid membranes, and showed a negative charge effect on ion transport and an increased cation selectivity through the porin channel. The properties of a typical general diffusion porin changed to those of a channel that contains point charges near the pore mouth. The single-channel conductance was no longer a linear function of the bulk aqueous salt concentration. The substantially higher cation selectivity of the succinylated porins compared with the native protein is consistent with the increase of negatively charged groups introduced. These results show tertiary structure-selective modification of charged residues as an efficient approach in the structure-function evaluation of ion channels, and X-ray crystallography and mass spectrometry as complementary analytical tools for defining precisely the chemically modified structures.
离子通道的理论研究中探讨了孔口附近电荷的作用。为了在通道蛋白中引入新的负电荷,用琥珀酸酐对来自荚膜红细菌37b4的孔蛋白的氨基进行琥珀酰化,并通过质谱和X射线晶体学确定琥珀酰化的精确程度和位点以及琥珀酰孔蛋白的结构。使用基质辅助激光解吸电离质谱进行的分子量和肽图谱分析确定了三个赖氨酸ε-氨基(Lys-46、Lys-298、Lys-300)和N端α-氨基的选择性琥珀酰化。确定了四琥珀酰化孔蛋白(TS-孔蛋白)的结构,分辨率为2.4 Å,与天然孔蛋白相比,其三聚体复合物结构总体上未发生变化。在单/二琥珀酰化孔蛋白(MS-孔蛋白)和TS-孔蛋白中发现的所有琥珀酰化氨基都位于通道内表面且可与溶剂接触:Lys-46位于通道收缩位点,而Lys-298、Lys-300和N端都靠近通道的周质入口。根据电子密度数据,中心收缩环处的Lys-46残基被模拟为琥珀酰赖氨酸,并显示其向周质孔口弯曲。通过将MS-孔蛋白和TS-孔蛋白重构到黑色脂质膜中,测定了它们的电学性质,结果表明其对离子转运有负电荷效应,并且通过孔蛋白通道的阳离子选择性增加。典型的一般扩散孔蛋白的性质转变为孔口附近含有点电荷的通道的性质。单通道电导不再是本体盐水浓度的线性函数。与天然蛋白相比,琥珀酰化孔蛋白显著更高的阳离子选择性与引入的负电荷基团的增加一致。这些结果表明,对带电残基进行三级结构选择性修饰是离子通道结构-功能评估的有效方法,而X射线晶体学和质谱是精确确定化学修饰结构的互补分析工具。
