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测量活细胞内荧光标记靶标物的浓度。

Measurement of intracellular concentration of fluorescently-labeled targets in living cells.

机构信息

Department of Molecular Biophysics, Bogomoletz Institute of Physiology, Kiev, Ukraine.

Department of Sensory Signaling, Bogomoletz Institute of Physiology, Kiev, Ukraine.

出版信息

PLoS One. 2018 Apr 25;13(4):e0194031. doi: 10.1371/journal.pone.0194031. eCollection 2018.

Abstract

Estimations of intracellular concentrations of fluorescently-labeled molecules within living cells are very important for guidance of biological experiments and interpretation of their results. Here we propose a simple and universal approach for such estimations. The approach is based upon common knowledge that the dye fluorescence is directly proportional to its quantum yield and the number of its molecules and that a coefficient of proportionality is determined by spectral properties of the dye and optical equipment used to record fluorescent signals. If two fluorescent dyes are present in the same volume, then a ratio of their concentrations is equal to a ratio of their fluorescence multiplied by some dye- and equipment-dependent coefficient. Thus, if the coefficient and concentration of one dye is known then the concentration of another dye can be determined. Here we have demonstrated how to calculate this coefficient (called a ratio factor) and how to use it for concentration measurements of fluorescently tagged molecules. As an example of how this approach can be used, we estimated a concentration of exogenously expressed neuronal Ca2+ sensor protein, hippocalcin, tagged by a fluorescent protein in a dendritic tree of rat hippocampal neurons loaded via a patch pipette with Alexa Fluor dye of known concentration. The new approach should allow performing a fast, inexpensive and reliable quantitative analysis of fluorescently-labeled targets in different parts of living cells.

摘要

在活细胞内对荧光标记分子的细胞内浓度进行估计对于指导生物实验和解释其结果非常重要。在这里,我们提出了一种简单而通用的估计方法。该方法基于一个常识,即染料荧光与其量子产率和分子数量成正比,而比例系数由染料的光谱特性和用于记录荧光信号的光学设备决定。如果在同一体积中存在两种荧光染料,则它们浓度的比值等于其荧光乘以某些与染料和设备相关的系数的比值。因此,如果已知一种染料的系数和浓度,则可以确定另一种染料的浓度。在这里,我们展示了如何计算这个系数(称为比率因子)以及如何使用它来测量荧光标记分子的浓度。作为这种方法如何使用的一个例子,我们估计了通过贴壁式吸管加载到大鼠海马神经元树突中的已知浓度的 Alexa Fluor 染料标记的外源性表达的神经元 Ca2+传感器蛋白 hippocalcin 的浓度。这种新方法应该允许对活细胞不同部位的荧光标记靶标进行快速、廉价和可靠的定量分析。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b72b/5918622/3879bc587b28/pone.0194031.g001.jpg

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