Synthetic and genetic dimers as quantification ruler for single-molecule counting with PALM

被引:17
|
作者
Baldering, Tim N. [1 ]
Dietz, Marina S. [1 ]
Gatterdam, Karl [2 ]
Karathanasis, Christos [1 ]
Wieneke, Ralph [2 ]
Tampe, Robert [2 ]
Heilemann, Mike [1 ]
机构
[1] Goethe Univ Frankfurt, Inst Phys & Theoret Chem, Single Mol Biophys, D-60438 Frankfurt, Germany
[2] Goethe Univ Frankfurt, Inst Biochem, D-60438 Frankfurt, Germany
关键词
LOCALIZATION MICROSCOPY; PROTEINS; RESOLUTION; OLIGOMERIZATION; PAIR;
D O I
10.1091/mbc.E18-10-0661
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
How membrane proteins oligomerize determines their function. Superresolution microscopy can report on protein clustering and extract quantitative molecular information. Here, we evaluate the blinking kinetics of four photoactivatable fluorescent proteins for quantitative single-molecule microscopy. We identified mEos3.2 and mMaple3 to be suitable for molecular quantification through blinking histogram analysis. We designed synthetic and genetic dimers of mEos3.2 as well as fusion proteins of monomeric and dimeric membrane proteins as reference structures, and we demonstrate their versatile use for quantitative superresolution imaging in vitro and in situ. We further found that the blinking behavior of mEos3.2 and mMaple3 is modified by a reducing agent, offering the possibility to adjust blinking parameters according to experimental needs.
引用
收藏
页码:1369 / 1376
页数:8
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