Department of Biochemistry and Molecular Biology, University of Kansas Medical Center, Kansas City, KS 66160-7421, USA.
J Mol Biol. 2010 Sep 10;402(1):1-7. doi: 10.1016/j.jmb.2010.07.024. Epub 2010 Jul 21.
The diphtheria toxin T domain translocates the catalytic C domain across the endosomal membrane in response to acidification. To elucidate the role of histidine protonation in modulating pH-dependent membrane action of the T domain, we have used site-directed mutagenesis coupled with spectroscopic and physiological assays. Replacement of H257 with an arginine (but not with a glutamine) resulted in dramatic unfolding of the protein at neutral pH, accompanied by a substantial loss of helical structure and greatly increased exposure of the buried residues W206 and W281. This unfolding and spectral shift could be reversed by the interaction of the H257R mutant with model lipid membranes. Remarkably, this greatly unfolded mutant exhibited wild-type-like activity in channel formation, N-terminus translocation, and cytotoxicity assays. Moreover, membrane permeabilization caused by the H257R mutant occurs already at pH 6, where wild type protein is inactive. We conclude that protonation of H257 acts as a major component of the pH-dependent conformational switch, resulting in destabilization of the folded structure in solution and thereby promoting the initial membrane interactions necessary for translocation.
白喉毒素 T 结构域在酸性环境下响应酸化,将催化 C 结构域穿过内体膜。为了阐明组氨酸质子化在调节 T 结构域 pH 依赖性膜作用中的作用,我们使用定点突变与光谱和生理测定相结合的方法。用精氨酸(而不是谷氨酰胺)取代 H257 会导致蛋白质在中性 pH 下剧烈展开,同时螺旋结构大量丢失,并且埋藏的残基 W206 和 W281 大大暴露。这种展开和光谱位移可以通过 H257R 突变体与模型脂质膜的相互作用来逆转。值得注意的是,这种严重展开的突变体在通道形成、N 端易位和细胞毒性测定中表现出野生型样的活性。此外,H257R 突变体引起的膜通透性在 pH 6 时就已经发生,而野生型蛋白在此 pH 值下无活性。我们得出结论,H257 的质子化作用是 pH 依赖性构象开关的主要组成部分,导致溶液中折叠结构的不稳定性,从而促进了易位所需的初始膜相互作用。