首页> 美国卫生研究院文献>The Journal of Biological Chemistry >An Ion-insensitive cAMP Biosensor for Long Term Quantitative Ratiometric Fluorescence Resonance Energy Transfer (FRET) Measurements under Variable Physiological Conditions
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An Ion-insensitive cAMP Biosensor for Long Term Quantitative Ratiometric Fluorescence Resonance Energy Transfer (FRET) Measurements under Variable Physiological Conditions

机译:离子不敏感的cAMP生物传感器用于在可变生理条件下进行长期定量比率荧光共振能量转移(FRET)测量

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摘要

Ratiometric measurements with FRET-based biosensors in living cells using a single fluorescence excitation wavelength are often affected by a significant ion sensitivity and the aggregation behavior of the FRET pair. This is an important problem for quantitative approaches. Here we report on the influence of physiological ion concentration changes on quantitative ratiometric measurements by comparing different FRET pairs for a cAMP-detecting biosensor. We exchanged the enhanced CFP/enhanced YFP FRET pair of an established Epac1-based biosensor by the fluorophores mCerulean/mCitrine. In the case of enhanced CFP/enhanced YFP, we showed that changes in proton, and (to a lesser extent) chloride ion concentrations result in incorrect ratiometric FRET signals, which may exceed the dynamic range of the biosensor. Calcium ions have no direct, but an indirect pH-driven effect by mobilizing protons. These ion dependences were greatly eliminated when mCerulean/mCitrine fluorophores were used. For such advanced FRET pairs the biosensor is less sensitive to changes in ion concentration and allows consistent cAMP concentration measurements under different physiological conditions, as occur in metabolically active cells. In addition, we verified that the described FRET pair exchange increased the dynamic range of the FRET efficiency response. The time window for stable experimental conditions was also prolonged by a faster biosensor expression rate in transfected cells and a greatly reduced tendency to aggregate, which reduces cytotoxicity. These properties were verified in functional tests in single cells co-expressing the biosensor and the 5-HT1A receptor.
机译:使用单个荧光激发波长在活细胞中使用基于FRET的生物传感器进行比例测量通常会受到显着的离子敏感性和FRET对的聚集行为的影响。对于定量方法而言,这是一个重要的问题。在这里,我们通过比较cAMP检测生物传感器的不同FRET对,来报告生理离子浓度变化对定量比率测量的影响。我们通过荧光团mCerulean / mCitrine交换了已建立的基于Epac1的生物传感器的增强CFP / YFP FRET增强对。在CFP / YFP增强的情况下,我们表明质子的变化和(较小程度的)氯离子浓度会导致不正确的比例FRET信号,这可能会超出生物传感器的动态范围。钙离子没有直接的影响,而是通过动员质子的间接pH驱动作用。使用mCerulean / mCitrine荧光团可大大消除这些离子依赖性。对于此类高级FRET对,生物传感器对离子浓度的变化较不敏感,并允许在不同的生理条件下(如在代谢活性细胞中发生)进行一致的cAMP浓度测量。此外,我们验证了所描述的FRET对交换增加了FRET效率响应的动态范围。稳定的实验条件的时间窗口也因转染细胞中更快的生物传感器表达速率和大大降低的聚集趋势而延长,从而降低了细胞毒性。这些特性在共表达生物传感器和5-HT1A受体的单细胞中的功能测试中得到验证。

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