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对中央螺旋连接区有缺失的钙调蛋白突变体进行的小角X射线散射研究表明,连接区主要保持α螺旋构象。

Small-angle X-ray scattering studies of calmodulin mutants with deletions in the linker region of the central helix indicate that the linker region retains a predominantly alpha-helical conformation.

作者信息

Kataoka M, Head J F, Persechini A, Kretsinger R H, Engelman D M

机构信息

Department of Molecular Biophysics and Biochemistry, Yale University, New Haven, Connecticut 06511.

出版信息

Biochemistry. 1991 Feb 5;30(5):1188-92. doi: 10.1021/bi00219a004.

DOI:10.1021/bi00219a004
PMID:1991098
Abstract

Two mutant forms of calmodulin were examined by small-angle X-ray scattering in solution and compared with the wild-type protein. Each mutant has deletions in the linker region of the central helix: one lacks residues Glu-83 and Glu-84 (Des2) and the other lacks residues Ser-81 through Glu-84 (Des4). The deletions change both the radii of gyration and the maximum dimensions of the molecules. In the presence of Ca2+, the observed radii of gyration are 22.4 A for wild-type bacterially expressed calmodulin, 19.5 A for Des2 calmodulin, and 20.3 A for Des4 calmodulin. A reduction in the radius of gyration by 1-2 A on removal of calcium, previously observed in the native protein, was also found in the wild type and the Des4 mutant; however, no significant size change was observed in the Des2 mutant. The large calcium-dependent conformational change in calmodulin induced by the binding of melittin [Kataoka, M., Head, J.F., Seaton, B.A., & Engelman, D.M. (1989) Proc. Natl. Acad. Sci. U.S.A. 86, 6944-6948] was observed in all the bacterially expressed proteins. Each protein appears to undergo a transition from a dumbbell shape to a more globular conformation on binding melittin in the presence of calcium, although quantitatively the changes in the wild-type and Des4 proteins greatly exceed those in Des2. Modeling shows the central linker region of the molecule. Thus, the structure of the linker region is stable enough to maintain the average orientation and separation of the lobes yet flexible enough to permit the lobes to approach each other upon binding a peptide.

摘要

通过溶液中的小角X射线散射对两种钙调蛋白突变体形式进行了检测,并与野生型蛋白进行了比较。每个突变体在中央螺旋的连接区都有缺失:一个缺失了Glu-83和Glu-84残基(Des2),另一个缺失了Ser-81至Glu-84残基(Des4)。这些缺失改变了分子的回转半径和最大尺寸。在Ca2+存在的情况下,野生型细菌表达的钙调蛋白的回转半径为22.4 Å,Des2钙调蛋白为19.5 Å,Des4钙调蛋白为20.3 Å。在野生型和Des4突变体中也发现,去除钙后回转半径减小1-2 Å,这在天然蛋白中也曾观察到;然而,Des2突变体中未观察到明显的尺寸变化。在所有细菌表达的蛋白中都观察到了蜂毒肽结合诱导的钙调蛋白中依赖钙的大的构象变化[片冈,M.,黑德,J.F.,西顿,B.A.,& 恩格尔曼,D.M.(1989年)《美国国家科学院院刊》86,6944 - 6948]。在钙存在的情况下,每种蛋白在结合蜂毒肽时似乎都从哑铃状转变为更球状的构象,尽管从数量上看,野生型和Des4蛋白的变化远远超过Des2蛋白。建模展示了分子的中央连接区。因此,连接区的结构足够稳定,能够维持叶的平均取向和间距,但又足够灵活,能够在结合肽时允许叶相互靠近。

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