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首页> 外文期刊>Neurobiology of Aging: Experimental and Clinical Research >Imaging and detecting molecular interactions of single transmembrane proteins.
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Imaging and detecting molecular interactions of single transmembrane proteins.

机译:成像和检测单个跨膜蛋白的分子相互作用。

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Single-molecule atomic force microscopy (AFM) provides novel ways to characterize structure-function relationships of native membrane proteins. High-resolution AFM-topographs allow observing substructures of single membrane proteins at sub-nanometer resolution as well as their conformational changes, oligomeric state, molecular dynamics and assembly. Complementary to AFM imaging, single-molecule force spectroscopy experiments allow detecting molecular interactions established within and between membrane proteins. The sensitivity of this method makes it possible to detect the interactions that stabilize secondary structures such as transmembrane alpha-helices, polypeptide loops and segments within. Changes in temperature or protein-protein assembly do not change the position of stable structural segments, but influence their stability established by collective molecular interactions. Such changes alter the probability of proteins to choose a certain unfolding pathway. Recent examples have elucidated unfolding and refolding pathways of membrane proteins as well as their energy landscapes. We review current and future potential of these approaches to reveal insights into membrane protein structure, function, and unfolding as we recognize that they could help answering key questions in the molecular basis of certain neuro-pathological dysfunctions.
机译:单分子原子力显微镜(AFM)提供了新颖的方法来表征天然膜蛋白的结构-功能关系。高分辨率的AFM形貌仪可在亚纳米分辨率下观察单个膜蛋白的亚结构,以及它们的构象变化,低聚状态,分子动力学和组装。作为AFM成像的补充,单分子力谱实验可以检测膜蛋白内部和之间建立的分子相互作用。该方法的灵敏性使得检测稳定二级结构(如跨膜α-螺旋,多肽环和其中的片段)的相互作用成为可能。温度或蛋白质-蛋白质装配的变化不会改变稳定结构片段的位置,但会影响通过集体分子相互作用建立的稳定性。这样的变化改变了蛋白质选择某种展开途径的可能性。最近的例子阐明了膜蛋白的展开和重折叠途径及其能量分布。我们回顾了这些方法的当前和未来潜力,以揭示对膜蛋白结构,功能和展开的见解,因为我们认识到它们可以帮助回答某些神经病理功能障碍的分子基础中的关键问题。

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