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An instrument for fast acquisition of fluorescence decay curves at picosecond resolution designed for “double kinetics” experiments: Application to fluorescence resonance excitation energy transfer study of protein folding

机译:一种用于皮秒分辨率的快速获取荧光衰减曲线的仪器,专为“双重动力学”实验而设计:在蛋白质折叠的荧光共振激发能转移研究中的应用

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摘要

The information obtained by studying fluorescence decay of labeled biopolymers is a major resource for understanding the dynamics of their conformations and interactions. The lifetime of the excited states of probes attached to macromolecules is in the nanosecond time regime, and hence, a series of snapshot decay curves of such probes might - in principle - yield details of fast changes of ensembles of labeled molecules down to sub-microsecond time resolution. Hence, a major current challenge is the development of instruments for the low noise detection of fluorescence decay curves within the shortest possible time intervals. Here, we report the development of an instrument, picosecond double kinetics apparatus, that enables recording of multiple fluorescence decay curves with picosecond excitation pulses over wide spectral range during microsecond data collection for each curve. The design is based on recording and averaging multiphoton pulses of fluorescence decay using a fast 13 GHz oscilloscope during microsecond time intervals at selected time points over the course of a chemical reaction or conformational transition. We tested this instrument in a double kinetics experiment using reference probes (N-acetyl-tryptophanamide). Very low stochastic noise level was attained, and reliable multi-parameter analysis such as derivation of distance distributions from time resolved FRET (fluorescence resonance excitation energy transfer) measurements was achieved. The advantage of the pulse recording and averaging approach used here relative to double kinetics methods based on the established time correlated single photon counting method, is that in the pulse recording approach, averaging of substantially fewer kinetic experiments is sufficient for obtaining the data. This results in a major reduction in the consumption of labeled samples, which in many cases, enables the performance of important experiments that were not previously feasible.
机译:通过研究标记生物聚合物的荧光衰减获得的信息是了解其构象和相互作用动力学的主要资源。附着在大分子上的探针的激发态的寿命处于纳秒级的时间范围内,因此,这类探针的一系列快照衰减曲线原则上可能会产生标记分子团簇快速变化至亚微秒的细节。时间分辨率。因此,当前的主要挑战是开发用于在尽可能短的时间间隔内低噪声检测荧光衰减曲线的仪器。在这里,我们报告了皮秒双动力学仪器的发展,该仪器能够在微秒数据收集过程中的每条曲线的较宽光谱范围内记录具有皮秒激发脉冲的多个荧光衰减曲线。该设计基于在化学反应或构象转变过程中的选定时间点,使用微弱的时间间隔(在选定的时间点),使用快速13 GHz示波器记录并平均荧光衰减的多光子脉冲。我们使用参考探针(N-乙酰基-色氨酸酰胺)在双重动力学实验中测试了该仪器。获得了非常低的随机噪声水平,并且实现了可靠的多参数分析,例如从时间分辨FRET(荧光共振激发能量转移)测量值推导距离分布。相对于基于已建立的时间相关的单光子计数方法的双重动力学方法,此处使用的脉冲记录和平均方法的优势在于,在脉冲记录方法中,平均少得多的动力学实验足以获得数据。这样可以大大减少标记样品的消耗,在许多情况下,可以执行以前不可行的重要实验。

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