Holzmeister Phil, Pibiri Enrico, Schmied Jürgen J, Sen Tapasi, Acuna Guillermo P, Tinnefeld Philip
NanoBioSciences Group, Institute for Physical and Theoretical Chemistry and Braunschweig Integrated Centre of Systems Biology (BRICS), and Laboratory for Emerging Nanometrology (LENA), Braunschweig University of Technology, Hans-Sommer-Strasse 10, Braunschweig 38106, Germany.
1] NanoBioSciences Group, Institute for Physical and Theoretical Chemistry and Braunschweig Integrated Centre of Systems Biology (BRICS), and Laboratory for Emerging Nanometrology (LENA), Braunschweig University of Technology, Hans-Sommer-Strasse 10, Braunschweig 38106, Germany [2].
Nat Commun. 2014 Nov 5;5:5356. doi: 10.1038/ncomms6356.
The interaction of dyes and metallic nanostructures strongly affects the fluorescence and can lead to significant fluorescence enhancement at plasmonic hot spots, but also to quenching. Here we present a method to distinguish the individual contributions to the changes of the excitation, radiative and non-radiative rate and use this information to determine the quantum yields for single molecules. The method is validated by precisely placing single fluorescent dyes with respect to gold nanoparticles as well as with respect to the excitation polarization using DNA origami nanostructures. Following validation, measurements in zeromode waveguides reveal that suppression of the radiative rate and enhancement of the non-radiative rate lead to a reduced quantum yield. Because the method exploits the intrinsic blinking of dyes, it can generally be applied to fluorescence measurements in arbitrary nanophotonic environments.
染料与金属纳米结构的相互作用会强烈影响荧光,在等离子体热点处可导致显著的荧光增强,但也会导致荧光猝灭。在此,我们提出一种方法,以区分对激发、辐射和非辐射速率变化的各自贡献,并利用此信息确定单分子的量子产率。通过使用DNA折纸纳米结构,相对于金纳米颗粒以及激发偏振精确放置单个荧光染料,对该方法进行了验证。验证之后,在零模波导中的测量表明,辐射速率的抑制和非辐射速率的增强会导致量子产率降低。由于该方法利用了染料固有的闪烁特性,它通常可应用于任意纳米光子环境中的荧光测量。
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