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Revealing Protein Aggregates under Thapsigargin-Induced ER Stress Using an ER-Targeted Thioflavin

Authors
Verwilst, PeterKim, KyutaeSunwoo, KyoungKim, Hye-RiKang, ChulhunKim, Jong Seung
Issue Date
11월-2019
Publisher
AMER CHEMICAL SOC
Keywords
protein aggregation; ER stress; fluorescence; thioflavin; chemical chaperones
Citation
ACS SENSORS, v.4, no.11, pp.2858 - 2863
Indexed
SCIE
SCOPUS
Journal Title
ACS SENSORS
Volume
4
Number
11
Start Page
2858
End Page
2863
URI
https://scholar.korea.ac.kr/handle/2021.sw.korea/61985
DOI
10.1021/acssensors.9b00568
ISSN
2379-3694
Abstract
Endoplasmic reticulum-thioflavin T (ER-ThT), a thioflavin T-based fluorescent chemosensor, was developed to detect protein aggregates in the endoplasmic reticulum (ER) and was applied to live cells under various forms of ER stress. Upon dithiothreitol (DTT)-induced reductive denaturation of lysozyme and albumin, the intensity was increased in a protein concentration-dependent way, following a nonfluorescent lag phase. ER-ThT detects protein aggregates rather than unfolded proteins in solution, and the protein aggregation can be visualized in the presence of lipid membranes or native proteins. Within live HeLa cells, ER-ThT is localized in the ER and its fluorescence was dramatically increased upon ER stress induction by DTT, Thapsigargin, or Brefeldin A. Moreover, in the presence of ER stress modulators (tauroursodeoxycholic acid, trimethylamine N-oxide, or 4-phenylbutyric acid), also known as chemical chaperones, the fluorescence under Thapsigargin treatment was suppressed to the level of the control group. Thus, ER-ThT is capable of detecting the accumulation of protein aggregates under ER stress in living cells and acts as an in vitro screening tool for ER stress modulators, putative prodrugs against ER-related proteopathy. Overall, the results strongly suggest that protein aggregation is intricately involved in the activation of the unfolded protein response following ER stress.
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