Analyzing proteome topology and function by automated multidimensional fluorescence microscopy

被引:370
作者
Schubert, Walter [1 ]
Bonnekoh, Bernd
Pommer, Ansgar J.
Philipsen, Lars
Boeckelmann, Raik
Malykh, Yanina
Gollnick, Harald
Friedenberger, Manuela
Bode, Marcus
Dress, Andreas W. M.
机构
[1] Univ Magdeburg, Inst Med Neurobiol, MPRR Grp, D-39120 Magdeburg, Germany
[2] Univ Magdeburg, Clin Dermatol & Venereol, D-39120 Magdeburg, Germany
[3] SIBS, CAS MPG Partner Inst Computat Biol, PICB, CN-200031 Shanghai, Peoples R China
[4] MPI Math Sci, D-04103 Leipzig, Germany
关键词
D O I
10.1038/nbt1250
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 [微生物学]; 0836 [生物工程]; 090102 [作物遗传育种]; 100705 [微生物与生化药学];
摘要
Temporal and spatial regulation of proteins contributes to function. We describe a multidimensional microscopic robot technology for high-throughput protein colocalization studies that runs cycles of fluorescence tagging, imaging and bleaching in situ. This technology combines three advances: a fluorescence technique capable of mapping hundreds of different proteins in one tissue section or cell sample; a method selecting the most prominent combinatorial molecular patterns by representing the data as binary vectors; and a system for imaging the distribution of these protein clusters in a so-called toponome map. By analyzing many cell and tissue types, we show that this approach reveals rules of hierarchical protein network organization, in which the frequency distribution of different protein clusters obeys Zipf's law, and state-specific lead proteins appear to control protein network topology and function. The technology may facilitate the development of diagnostics and targeted therapies.
引用
收藏
页码:1270 / 1278
页数:9
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