作者
Gleb Shtengel, James A Galbraith, Catherine G Galbraith, Jennifer Lippincott-Schwartz, Jennifer M Gillette, Suliana Manley, Rachid Sougrat, Clare M Waterman, Pakorn Kanchanawong, Michael W Davidson, Richard D Fetter, Harald F Hess
发表日期
2009/3/3
期刊
Proceedings of the National Academy of Sciences
卷号
106
期号
9
页码范围
3125-3130
出版商
National Academy of Sciences
简介
Understanding molecular-scale architecture of cells requires determination of 3D locations of specific proteins with accuracy matching their nanometer-length scale. Existing electron and light microscopy techniques are limited either in molecular specificity or resolution. Here, we introduce interferometric photoactivated localization microscopy (iPALM), the combination of photoactivated localization microscopy with single-photon, simultaneous multiphase interferometry that provides sub-20-nm 3D protein localization with optimal molecular specificity. We demonstrate measurement of the 25-nm microtubule diameter, resolve the dorsal and ventral plasma membranes, and visualize the arrangement of integrin receptors within endoplasmic reticulum and adhesion complexes, 3D protein organization previously resolved only by electron microscopy. iPALM thus closes the gap between electron tomography and light …
引用总数
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学术搜索中的文章
G Shtengel, JA Galbraith, CG Galbraith… - Proceedings of the National Academy of Sciences, 2009