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A quantitative method to monitor STING degradation with dual-luciferase reporters

降级(电信) 荧光素酶 对偶(语法数字) 化学 细胞生物学 色谱法 生物物理学 生物 计算机科学 生物化学 工程类 电信 航空航天工程 艺术 转染 文学类 基因
作者
Tsumugi Shoji,Kanako Sato,Ayumi Shinojima,Shogo Koide,Ruri Shindo,Kazuhiro Hongo,Kojiro Mukai,Yoshihiko Kuchitsu,Tomohiko Taguchi
出处
期刊:Cell Structure and Function [Japan Society of Cell Biology]
标识
DOI:10.1247/csf.25011
摘要

Stimulator of interferon genes (STING) triggers the type I interferon and inflammatory responses against a variety of DNA pathogens, which is essential to limiting viral infection and replication. STING activates the downstream kinase TBK1 at the trans-Golgi network (TGN) and is degraded at lysosomes through a process called lysosomal microautophagy. Impaired STING targeting to lysosomes results in the prolonged inflammatory signal, which may be associated with a variety of neurodegenerative and autoinflammatory diseases. Thus, development of methods to quantify STING degradation helps understand the mechanism of lysosomal microautophagy and its related diseases. Here we report a quantitative method to monitor STING degradation with two luciferases, firefly luciferase (FLuc) and Nanoluciferase (NLuc). The expression plasmid is composed of FLuc, a P2A self-cleavage site, and NLuc-tagged STING. FLuc intensity reflects the total amount of translated protein, serving as an internal control, while NLuc intensity corresponds to the amount of STING. Comparison of the NLuc/FLuc ratio after STING stimulation reported the kinetics of decay of STING levels in live cells. This method should provide a useful complement to western blotting and fluorescence- activated cell sorter (FACS) analysis presently used to monitor STING degradation.Key words: Innate immunity, STING, membrane traffic, lysosomal degradation, luciferase.

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