首页> 美国卫生研究院文献>Biophysical Journal >Particle counting by fluorescence correlation spectroscopy. Simultaneous measurement of aggregation and diffusion of molecules in solutions and in membranes.
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Particle counting by fluorescence correlation spectroscopy. Simultaneous measurement of aggregation and diffusion of molecules in solutions and in membranes.

机译:通过荧光相关光谱法计数颗粒。同时测量溶液和膜中分子的聚集和扩散。

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摘要

A method for simultaneous determination of molar weights (M) and lateral diffusion constants (D) of particles in three- and two-dimensional systems is described. Spontaneous concentration fluctuations in space and time are analyzed, by monitoring fluctuations in the fluorescence from fluorescein-labeled molecules (1 dye/molecule is sufficient), excited by a rotating laser spot. For particles in solution, M values are determined over the range of 3 x 10(2) to 3 x 10(11) daltons, and D values can be determined from approximately 10(-7) to 10(-10) cm2/s. The time for a determination is approximately 1 min. Aggregation can be followed by changes of either M or D. This method is used to study the calcium dependence of vesicle aggregation or fusion, and the time course of aggregate formation of porin (an Escherichia Coli outer membrane protein) in lipid monolayers. Essential parameters for the development of the method are described. Equations to estimate the signal-to-noise ratios and to find the optimal free parameters for a specific application are derived. The theoretical predictions for the correlation function of the signal and for the signal-to-noise ratio are compared with observed values.
机译:描述了一种同时测定三维和二维系统中颗粒的摩尔质量(M)和横向扩散常数(D)的方法。通过监测荧光素标记的分子(1个染料/分子就足够了)受到旋转激光点激发的荧光的波动,分析了空间和时间的自发浓度波动。对于溶液中的颗粒,M值的确定范围是3 x 10(2)至3 x 10(11)道尔顿,D值可以确定为大约10(-7)至10(-10)cm2 / s 。测定时间约为1分钟。聚集之后可以是M或D的变化。此方法用于研究脂质单层中囊泡聚集或融合的钙依赖性,以及孔蛋白(大肠杆菌外膜蛋白)聚集形成的时间过程。描述了开发该方法的基本参数。得出了用于估算信噪比并找到针对特定应用的最佳自由参数的方程式。将信号的相关函数和信噪比的理论预测与观测值进行比较。

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