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首页> 外文期刊>Biophysical Journal >Ultrafast photoconversion of the green fluorescent protein studied by accumulative femtosecond spectroscopy.
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Ultrafast photoconversion of the green fluorescent protein studied by accumulative femtosecond spectroscopy.

机译:飞秒累积光谱法研究绿色荧光蛋白的超快光转换。

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The irreversible photoconversion of T203V green fluorescent protein (GFP) via decarboxylation is studied under femtosecond excitation using an accumulative product detection method that allows us to measure small conversion efficiencies of down to DeltaOD = 10(-7) absorbance change per pulse. Power studies with 800- and 400-nm pulse excitation reveal that excitation to higher states of the neutral form of the GFP chromophore induces photoconversion very efficiently. The singly excited neutral chromophore is a resonant intermediate of the two-step excitation process that leads to efficient photoconversion. We determine the dynamics of this two-step process by separating the excitation step of the neutral chromophore from the further excitation step to the reactive state in a time-resolved two-color experiment. The dynamics show that a further excitation to the very reactive higher excited state is only possible from the initially excited neutral chromophore and not from the fluorescent intermediate state. For applications of GFP in two-photon fluorescence microscopy, the found photochemical behavior implies that the high intensity conditions used in microscopy can lead to photoconversion easily and care has to be taken to avoid unwanted photoconversion.
机译:在飞秒激发下使用累积产物检测方法研究了通过脱羧作用的T203V绿色荧光蛋白(GFP)不可逆的光转换,该累积产品检测方法使我们能够测量小转换效率,低至DeltaOD = 10(-7)每个脉冲吸光度变化。用800和400 nm脉冲激发进行的功率研究表明,激发到GFP生色团的中性形式的较高状态非常有效地诱导了光转化。单激发的中性生色团是两步激发过程的共振中​​间产物,可导致有效的光转换。我们通过在时间分辨的双色实验中将中性发色团的激发步骤与进一步的激发步骤分离为反应态来确定此两步过程的动力学。动力学表明,只有从最初被激发的中性发色团而不是从荧光中间态,才可能进一步激发到反应性更高的激发态。对于GFP在双光子荧光显微镜中的应用,发现的光化学行为表明,在显微镜中使用的高强度条件很容易导致光转换,因此必须小心避免不必要的光转换。

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