嘌呤能受体
细胞内
三磷酸腺苷
细胞生物学
先天免疫系统
效应器
化学
腺苷
鸟苷三磷酸
免疫系统
生物
受体
生物化学
GTP'
免疫学
酶
作者
Sabrina Forveille,Juliette Humeau,Allan Sauvat,Lucillia Bezu,Guido Kroemer,Oliver Kepp
标识
DOI:10.1016/bs.mie.2019.05.050
摘要
Several antineoplastic agents are endowed with the ability to induce immunogenic cell death (ICD), a modality of cellular demise that is accompanied by the release of danger associated molecular patterns such as adenosine triphosphate (ATP) into the tumor microenvironment. ATP-mediated ligation of purinergic P2R receptors then facilitates the chemotactic recruitment and activation of innate immune effectors, thus favoring the induction of anticancer immunity. Here, we provide a protocol for the fluorescence microscopy-based quantification of ICD-associated ATP secretion that is amenable to high-throughput screening. As compared to the traditional luciferase-based detection of ATP in cell culture supernatants, the analysis presented here is cost-efficient and can be combined with the parallel assessment of cellular morphology.
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