Lee Jinwoo, Glover Kerney Jebrell
Department of Chemistry, Lehigh University, Bethlehem, PA 18015, USA.
Biochim Biophys Acta. 2012 May;1818(5):1158-64. doi: 10.1016/j.bbamem.2011.12.033. Epub 2012 Jan 4.
Caveolin is an integral membrane protein that is found in high abundance in caveolae. Both the N- and C- termini lie on the same side of the membrane, and the transmembrane domain has been postulated to form an unusual intra-membrane horseshoe configuration. To probe the structure of the transmembrane domain, we have prepared a construct of caveolin-1 that encompasses residues 96-136 (the entire intact transmembrane domain). Caveolin-1(96-136) was over-expressed and isotopically labeled in E. coli, purified to homogeneity, and incorporated into lyso-myristoylphosphatidylglycerol micelles. Circular dichroism and NMR spectroscopy reveal that the transmembrane domain of caveolin-1 is primarily α-helical (57-65%). Furthermore, chemical shift indexing reveals that the transmembrane domain has a helix-break-helix structure which could be critical for the formation of the intra-membrane horseshoe conformation predicted for caveolin-1. The break in the helix spans residues 108 to 110, and alanine scanning mutagenesis was carried out to probe the structural significance of these residues. Our results indicate that mutation of glycine 108 to alanine does not disrupt the structure, but mutation of isoleucine 109 and proline 110 to alanine dramatically alters the helix-break-helix structure. To explore the structural determinants further, additional mutagenesis was performed. Glycine 108 can be substituted with other small side chain amino acids (i.e. alanine), leucine 109 can be substituted with other β-branched amino acids (i.e. valine), and proline 110 cannot be substituted without disrupting the helix-break-helix structure.
小窝蛋白是一种整合膜蛋白,在小窝中大量存在。其N端和C端位于膜的同一侧,跨膜结构域被推测形成一种不寻常的膜内马蹄形结构。为了探究跨膜结构域的结构,我们制备了包含96 - 136位残基(完整的跨膜结构域)的小窝蛋白-1构建体。小窝蛋白-1(96 - 136)在大肠杆菌中过表达并进行同位素标记,纯化至同质,然后整合到溶血肉豆蔻酰磷脂酰甘油胶束中。圆二色性和核磁共振光谱表明,小窝蛋白-1的跨膜结构域主要是α螺旋结构(57 - 65%)。此外,化学位移指数分析表明,跨膜结构域具有螺旋-断裂-螺旋结构,这可能对小窝蛋白-1预测的膜内马蹄形构象的形成至关重要。螺旋的断裂跨越108至110位残基,进行丙氨酸扫描诱变以探究这些残基的结构意义。我们的结果表明,将甘氨酸108突变为丙氨酸不会破坏结构,但将异亮氨酸109和脯氨酸110突变为丙氨酸会显著改变螺旋-断裂-螺旋结构。为了进一步探究结构决定因素,进行了额外的诱变。甘氨酸108可以被其他小侧链氨基酸(如丙氨酸)取代,亮氨酸109可以被其他β分支氨基酸(如缬氨酸)取代,而脯氨酸110在不破坏螺旋-断裂-螺旋结构的情况下不能被取代。