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使用光致发光探针测量细胞内钙水平的高通量筛选

High-Throughput Screening Using Photoluminescence Probe to Measure Intracellular Calcium Levels.

作者信息

Feno Simona, Di Marco Giulia, De Mario Agnese, Monticelli Halenya, Reane Denis Vecellio

机构信息

Department of Biomedical Sciences, University of Padua, Padua, Italy.

Department of Surgery, Oncology and Gastroenterology, University of Padua, Padua, Italy.

出版信息

Methods Mol Biol. 2019;1925:1-14. doi: 10.1007/978-1-4939-9018-4_1.

Abstract

Aequorin, a 22 kDa protein produced by the jellyfish Aequorea victoria, was the first probe used to measure Ca concentrations ([Ca]) of specific intracellular organelles in intact cells. After the binding of Ca to three high-affinity binding sites, an irreversible reaction occurs leading to the emission of photons that is proportional to [Ca]. While native aequorin is suitable for measuring cytosolic [Ca] after cell stimulation in a range from 0.5 to 10 μM, it cannot be used in organelles where [Ca] is much higher, such as in the lumen of endoplasmic/sarcoplasmic reticulum (ER/SR) and mitochondria. However, some modifications made on aequorin itself or on coelenterazine, its lipophilic prosthetic luminophore, and the addition of targeting sequences or the fusion with resident proteins allowed the specific organelle localization and the measurements of intra-organelle Ca levels. In the last years, the development of multiwell plate readers has opened the possibility to perform aequorin-based high-throughput screenings and has overcome some limitation of the standard method. Here we present the procedure for expressing, targeting, and reconstituting aequorin in intact cells and for measuring Ca in the bulk cytosol, mitochondria, and ER by a high-throughput screening system.

摘要

水母发光蛋白是由维多利亚多管发光水母产生的一种22千道尔顿的蛋白质,是首个用于测量完整细胞中特定细胞内细胞器钙浓度([Ca])的探针。钙与三个高亲和力结合位点结合后,会发生不可逆反应,导致发射与[Ca]成正比的光子。虽然天然水母发光蛋白适用于在0.5至10微摩尔范围内测量细胞刺激后胞质溶胶中的[Ca],但它不能用于[Ca]高得多的细胞器,如内质网/肌浆网(ER/SR)和线粒体的内腔。然而,对水母发光蛋白本身或其亲脂性辅基发光团腔肠素进行的一些修饰,以及添加靶向序列或与驻留蛋白融合,使得能够实现特定细胞器定位并测量细胞器内的钙水平。在过去几年中,微孔板读数器的发展为基于水母发光蛋白的高通量筛选提供了可能,并克服了标准方法的一些局限性。在此,我们介绍在完整细胞中表达、靶向和重组水母发光蛋白,以及通过高通量筛选系统测量胞质溶胶、线粒体和内质网中钙的方法。

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