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利用荧光寿命成像监测细胞内纳摩尔级钙离子。

Monitoring intracellular nanomolar calcium using fluorescence lifetime imaging.

机构信息

UCL Institute of Neurology, University College London, London, UK.

出版信息

Nat Protoc. 2018 Mar;13(3):581-597. doi: 10.1038/nprot.2017.154. Epub 2018 Feb 22.

Abstract

Nanomolar-range fluctuations of intracellular [Ca] are critical for brain cell function but remain difficult to measure. We have advanced a microscopy technique to monitor intracellular [Ca] in individual cells in acute brain slices (also applicable in vivo) using fluorescence lifetime imaging (FLIM) of the Ca-sensitive fluorescent indicator Oregon Green BAPTA1 (OGB-1). The OGB-1 fluorescence lifetime is sensitive to [Ca] within the 10-500 nM range but not to other factors such as viscosity, temperature, or pH. This protocol describes the requirements, setup, and calibration of the FLIM system required for OGB-1 imaging. We provide a step-by-step procedure for whole-cell OGB-1 loading and two-photon FLIM. We also describe how to analyze the obtained FLIM data using total photon count and gated-intensity record, a ratiometric photon-counting approach that provides a highly improved signal-to-noise ratio and greater sensitivity of absolute [Ca] readout. We demonstrate our technique in nerve cells in situ, and it is adaptable to other cell types and fluorescent indicators. This protocol requires a basic understanding of FLIM and experience in single-cell electrophysiology and cell imaging. Setting up the FLIM system takes ∼2 d, and OGB-1 loading, imaging, and data analysis take 2 d.

摘要

细胞内 [Ca] 的纳摩尔级波动对脑细胞功能至关重要,但仍难以测量。我们已经开发出一种显微镜技术,使用钙敏感荧光指示剂 Oregon Green BAPTA1(OGB-1)的荧光寿命成像(FLIM),在急性脑切片中(也适用于体内)监测单个细胞内的细胞内 [Ca]。OGB-1 的荧光寿命对 10-500 nM 范围内的 [Ca] 敏感,但对其他因素如粘度、温度或 pH 不敏感。本协议描述了用于 OGB-1 成像的 FLIM 系统的要求、设置和校准。我们提供了全细胞 OGB-1 加载和双光子 FLIM 的分步程序。我们还描述了如何使用总光子计数和门控强度记录分析获得的 FLIM 数据,这是一种比率光子计数方法,可提供更高的信噪比和更高的绝对 [Ca] 读出灵敏度。我们在原位神经细胞中展示了我们的技术,并且它适用于其他细胞类型和荧光指示剂。该协议需要对 FLIM 有基本的了解,并具有单细胞电生理学和细胞成像方面的经验。FLIM 系统的设置需要 2 天,OGB-1 加载、成像和数据分析需要 2 天。

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