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利用原子力显微镜对蛋白质复合物内部化学基团进行成像和三维重建。

Imaging and three-dimensional reconstruction of chemical groups inside a protein complex using atomic force microscopy.

作者信息

Kim Duckhoe, Sahin Ozgur

机构信息

Departments of Biological Sciences and Physics, Columbia University, New York, New York 10027, USA.

出版信息

Nat Nanotechnol. 2015 Mar;10(3):264-9. doi: 10.1038/nnano.2014.335. Epub 2015 Feb 9.

DOI:10.1038/nnano.2014.335
PMID:25664622
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4429059/
Abstract

Scanning probe microscopes can be used to image and chemically characterize surfaces down to the atomic scale. However, the localized tip-sample interactions in scanning probe microscopes limit high-resolution images to the topmost atomic layer of surfaces, and characterizing the inner structures of materials and biomolecules is a challenge for such instruments. Here, we show that an atomic force microscope can be used to image and three-dimensionally reconstruct chemical groups inside a protein complex. We use short single-stranded DNAs as imaging labels that are linked to target regions inside a protein complex, and T-shaped atomic force microscope cantilevers functionalized with complementary probe DNAs allow the labels to be located with sequence specificity and subnanometre resolution. After measuring pairwise distances between labels, we reconstruct the three-dimensional structure formed by the target chemical groups within the protein complex using simple geometric calculations. Experiments with the biotin-streptavidin complex show that the predicted three-dimensional loci of the carboxylic acid groups of biotins are within 2 Å of their respective loci in the corresponding crystal structure, suggesting that scanning probe microscopes could complement existing structural biological techniques in solving structures that are difficult to study due to their size and complexity.

摘要

扫描探针显微镜可用于对表面进行成像,并在原子尺度上对其进行化学表征。然而,扫描探针显微镜中局部的针尖-样品相互作用将高分辨率图像限制在表面的最顶层原子层,对于此类仪器而言,表征材料和生物分子的内部结构是一项挑战。在此,我们展示了原子力显微镜可用于对蛋白质复合物内部的化学基团进行成像并三维重建。我们使用短单链DNA作为成像标签,将其连接到蛋白质复合物内部的目标区域,并用互补探针DNA功能化的T形原子力显微镜悬臂可使标签以序列特异性和亚纳米分辨率定位。在测量标签之间的成对距离后,我们使用简单的几何计算重建蛋白质复合物内目标化学基团形成的三维结构。对生物素-链霉亲和素复合物的实验表明,生物素羧酸基团的预测三维位点与其在相应晶体结构中的各自位点相差在2 Å以内,这表明扫描探针显微镜可补充现有的结构生物学技术,以解决因尺寸和复杂性而难以研究的结构问题。

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