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使用多重生物传感器条形码对基于荧光共振能量转移(FRET)的生物传感器进行校准。

Calibration of FRET-based biosensors using multiplexed biosensor barcoding.

作者信息

Wu Jhen-Wei, Yang Jr-Ming, Chen Chao-Cheng, Au Gabriel, Wang Suyang, Chern Gia-Wei, Huang Chuan-Hsiang

出版信息

bioRxiv. 2024 Sep 8:2024.09.04.610346. doi: 10.1101/2024.09.04.610346.

DOI:10.1101/2024.09.04.610346
PMID:39282286
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC11398328/
Abstract

Förster resonance energy transfer (FRET) between fluorescent proteins (FPs) is widely used in the design of genetically encoded fluorescent biosensors, which are powerful tools for monitoring the dynamics of biochemical activities in live cells. FRET ratio, defined as the ratio between acceptor and donor signals, is often used as a proxy for the actual FRET efficiency, which must be corrected for signal crosstalk using donor-only and acceptor-only samples. However, the FRET ratio is highly sensitive to imaging conditions, making direct comparisons across different experiments and over time challenging. Inspired by a method for multiplexed biosensor imaging using barcoded cells, we reasoned that calibration standards with fixed FRET efficiency can be introduced into a subset of cells for normalization of biosensor signals. Our theoretical analysis indicated that the FRET ratio of high-FRET species relative to non-FRET species slightly decreases at high excitation intensity, suggesting the need for calibration using both high and low FRET standards. To test these predictions, we created FRET donor-acceptor pairs locked in "FRET-ON" and "FRET-OFF" conformations and introduced them into a subset of barcoded cells. Our results confirmed the theoretical predictions and showed that the calibrated FRET ratio is independent of imaging settings. We also provided a strategy for calculating the FRET efficiency. Together, our study presents a simple strategy for calibrated and highly multiplexed imaging of FRET biosensors, facilitating reliable comparisons across experiments and supporting long-term imaging applications.

摘要

荧光蛋白(FPs)之间的Förster共振能量转移(FRET)在基因编码荧光生物传感器的设计中被广泛应用,这些生物传感器是监测活细胞中生化活动动态的强大工具。FRET比率定义为受体与供体信号之间的比率,常被用作实际FRET效率的替代指标,而实际FRET效率必须使用仅含供体和仅含受体的样本对信号串扰进行校正。然而,FRET比率对成像条件高度敏感,使得跨不同实验和随时间进行直接比较具有挑战性。受一种使用条形码细胞进行多重生物传感器成像方法的启发,我们推断可以将具有固定FRET效率的校准标准引入细胞亚群中,以对生物传感器信号进行归一化。我们的理论分析表明,在高激发强度下,高FRET物种相对于非FRET物种的FRET比率略有下降,这表明需要使用高FRET和低FRET标准进行校准。为了验证这些预测,我们创建了锁定在“FRET开启”和“FRET关闭”构象的FRET供体-受体对,并将它们引入条形码细胞的一个亚群中。我们的结果证实了理论预测,并表明校准后的FRET比率与成像设置无关。我们还提供了一种计算FRET效率的策略。总之,我们的研究提出了一种用于FRET生物传感器校准和高度多重成像的简单策略,便于跨实验进行可靠比较,并支持长期成像应用。

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