Abdul-Manan N, Hinton J F
Department of Chemistry and Biochemistry, University of Arkansas, Fayetteville 72701.
Biochemistry. 1994 Jun 7;33(22):6773-83. doi: 10.1021/bi00188a005.
Gramicidin A incorporated into SDS (sodium dodecyl sulfate) micelles exists as a right-handed, N-to-N-terminal beta 6.3 helical dimer [Lomize, A. L., Orechov, V. Yu., & Arseniev, A.S. (1992) Bioorg. Khim. 18, 182-189]. In the incorporation procedure to achieve the ion channel state of gramicidin A in SDS micelles, trifluoroethanol (TFE) is used to solubilize the hydrophobic peptide before addition to the aqueous/micelle solution. The conformational transition of gramicidin A to form ion channels in SDS micelles, i.e., in TFE and 10% TFE/water, has been investigated using 2D NMR and CD spectroscopy. In neat TFE, gramicidin A was found to be monomeric and may possibly exist in an equilibrium of rapidly interconverting conformers of at least three different forms believed to be left- and/or right-handed alpha and beta 4.4 helices. It was found that the interconversion between these conformers was slowed down in 55% TFE as evident by the observation of at least three different sets of d alpha N COSY peaks although CD gave a net spectrum similar to that in neat TFE. In 10% TFE gramicidin A spontaneously forms a precipitate. The precipitated species were isolated and solubilized in dioxane where gramicidin conformers undergo very slow interconversion and could be characterized by NMR. At least seven different gramicidin A conformations were found in 10% TFE. Four of thes are the same types of double helices as previously found in ethanol (i.e., a symmetric left-handed parallel beta 5.6 double helix, an unsymmetric left-handed parallel beta 5.6 double helix, a symmetric left-handed antiparallel beta 5.6 double helix, a symmetric right-handed parallel beta 5.6 double helix); the fifth is possibly a symmetric right-handed antiparallel beta 5.6 double helix. There is also evidence for the presence of at least one form of monomeric species. Previous observation on the solvent history dependence in the ease of channel incorporation may be explained by the presence of several different folding pathways to channel formation. To test this proposal, the conformation of gramicidin A in 10% DMSO and 10% methanol was studied. In the former environment, the major form was a random coil with a minor population of double-stranded helices, while in the latter, NMR spectra indicate the presence of the same double-helical conformers as found in neat methanol.
掺入十二烷基硫酸钠(SDS)胶束中的短杆菌肽A以右手的、从N端到N端的β6.3螺旋二聚体形式存在[洛米泽,A.L.,奥列霍夫,V.Yu.,& 阿尔谢尼耶夫,A.S.(1992年)《生物有机化学》18,182 - 189]。在使短杆菌肽A在SDS胶束中达到离子通道状态的掺入过程中,在添加到水/胶束溶液之前,使用三氟乙醇(TFE)来溶解疏水性肽。已使用二维核磁共振(2D NMR)和圆二色光谱(CD)研究了短杆菌肽A在SDS胶束中,即在TFE和10% TFE/水体系中形成离子通道的构象转变。在纯TFE中,发现短杆菌肽A是单体形式,并且可能以至少三种不同形式的快速相互转化构象的平衡状态存在,这些构象被认为是左手和/或右手的α螺旋和β4.4螺旋。结果发现,在55% TFE中这些构象之间的相互转化减缓,这通过观察到至少三组不同的δαN COSY峰得以证明,尽管CD给出的净光谱与纯TFE中的相似。在10% TFE中,短杆菌肽A自发形成沉淀。分离出沉淀物质并将其溶解在二氧六环中,在那里短杆菌肽构象的相互转化非常缓慢,并且可以通过核磁共振进行表征。在10% TFE中发现了至少七种不同的短杆菌肽A构象。其中四种是与先前在乙醇中发现的相同类型的双螺旋(即对称的左手平行β5.6双螺旋、不对称的左手平行β5.6双螺旋、对称的左手反平行β5.6双螺旋、对称的右手平行β5.6双螺旋);第五种可能是对称的右手反平行β5.6双螺旋。也有证据表明存在至少一种单体形式。先前关于通道掺入难易程度对溶剂历史的依赖性的观察结果,可能可以通过存在几种不同的形成通道的折叠途径来解释。为了验证这一推测,研究了短杆菌肽A在10%二甲基亚砜(DMSO)和10%甲醇中的构象。在前一种环境中,主要形式是无规卷曲,有少量双链螺旋,而在后一种环境中,核磁共振光谱表明存在与纯甲醇中发现的相同的双螺旋构象。
