An ultrasensitive GSH-specific fluorescent probe unveils celastrol-induced ccRCC ferroptosis

[Display omitted] •GSH-specific fluorescent probe for GSH detection in clinical samples and live cell and tumor imaging.•Celastrol induces ferroptosis in ccRCC.•GSH-specific fluorescent probe tracks celastrol-induced ccRCC ferroptosis. Glutathione (GSH) is closely related to the occurrence and devel...

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Published inBioorganic chemistry Vol. 134; p. 106454
Main Authors Li, Hongfang, Deng, Changfeng, Zhu, Neng, Zhang, Chanjuan, Zeng, Qing, Qin, Li
Format Journal Article
LanguageEnglish
Published SAN DIEGO Elsevier Inc 01.05.2023
Elsevier
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Abstract [Display omitted] •GSH-specific fluorescent probe for GSH detection in clinical samples and live cell and tumor imaging.•Celastrol induces ferroptosis in ccRCC.•GSH-specific fluorescent probe tracks celastrol-induced ccRCC ferroptosis. Glutathione (GSH) is closely related to the occurrence and development of tumors. The intracellular GSH levels are abnormally altered when tumor cells undergo programmed cell death. Therefore, real-time monitoring of the dynamic changes of intracellular GSH levels can better enable the early diagnosis of diseases and evaluate the effects of cell death-inducing drugs. In this study, a stable and highly selective fluorescent probe AR has been designed and synthesized for the fluorescence imaging and rapid detection of GSH in vitro and in vivo, as well as patient-derived tumor tissue. More importantly, the AR probe can be used to track changes in GSH levels and fluorescence imaging during the treatment of clear cell renal cell carcinoma (ccRCC) with celastrol (CeT) via inducing ferroptosis. These findings demonstrate that the developed fluorescent probe AR exhibits high selectivity and sensitivity, as well as good biocompatibility and long-term stability, which can be used to image endogenous GSH in living tumors and cells. Also, a significant decrease in GSH levels was observed by the fluorescent probe AR during the treatment of ccRCC with CeT-induced ferroptosis in vitro and in vivo. Overall, these findings will provide a novel strategy for celastrol targeting ferroptosis in the treatment of ccRCC and the application of fluorescent probes to help reveal the underlying mechanism of CeT in the treatment of ccRCC.
AbstractList [Display omitted] •GSH-specific fluorescent probe for GSH detection in clinical samples and live cell and tumor imaging.•Celastrol induces ferroptosis in ccRCC.•GSH-specific fluorescent probe tracks celastrol-induced ccRCC ferroptosis. Glutathione (GSH) is closely related to the occurrence and development of tumors. The intracellular GSH levels are abnormally altered when tumor cells undergo programmed cell death. Therefore, real-time monitoring of the dynamic changes of intracellular GSH levels can better enable the early diagnosis of diseases and evaluate the effects of cell death-inducing drugs. In this study, a stable and highly selective fluorescent probe AR has been designed and synthesized for the fluorescence imaging and rapid detection of GSH in vitro and in vivo, as well as patient-derived tumor tissue. More importantly, the AR probe can be used to track changes in GSH levels and fluorescence imaging during the treatment of clear cell renal cell carcinoma (ccRCC) with celastrol (CeT) via inducing ferroptosis. These findings demonstrate that the developed fluorescent probe AR exhibits high selectivity and sensitivity, as well as good biocompatibility and long-term stability, which can be used to image endogenous GSH in living tumors and cells. Also, a significant decrease in GSH levels was observed by the fluorescent probe AR during the treatment of ccRCC with CeT-induced ferroptosis in vitro and in vivo. Overall, these findings will provide a novel strategy for celastrol targeting ferroptosis in the treatment of ccRCC and the application of fluorescent probes to help reveal the underlying mechanism of CeT in the treatment of ccRCC.
Glutathione (GSH) is closely related to the occurrence and development of tumors. The intracellular GSH levels are abnormally altered when tumor cells undergo programmed cell death. Therefore, real-time monitoring of the dynamic changes of intracellular GSH levels can better enable the early diagnosis of diseases and evaluate the effects of cell death-inducing drugs. In this study, a stable and highly selective fluorescent probe AR has been designed and synthesized for the fluorescence imaging and rapid detection of GSH in vitro and in vivo, as well as patient-derived tumor tissue. More importantly, the AR probe can be used to track changes in GSH levels and fluorescence imaging during the treatment of clear cell renal cell carcinoma (ccRCC) with celastrol (CeT) via inducing ferroptosis. These findings demonstrate that the developed fluorescent probe AR exhibits high selectivity and sensitivity, as well as good biocompatibility and long-term stability, which can be used to image endogenous GSH in living tumors and cells. Also, a significant decrease in GSH levels was observed by the fluorescent probe AR during the treatment of ccRCC with CeT-induced ferroptosis in vitro and in vivo. Overall, these findings will provide a novel strategy for celastrol targeting ferroptosis in the treatment of ccRCC and the application of fluorescent probes to help reveal the underlying mechanism of CeT in the treatment of ccRCC.
Glutathione (GSH) is closely related to the occurrence and development of tumors. The intracellular GSH levels are abnormally altered when tumor cells undergo programmed cell death. Therefore, real-time monitoring of the dynamic changes of intracellular GSH levels can better enable the early diagnosis of diseases and evaluate the effects of cell death-inducing drugs. In this study, a stable and highly selective fluorescent probe AR has been designed and synthesized for the fluorescence imaging and rapid detection of GSH in vitro and in vivo, as well as patient-derived tumor tissue. More importantly, the AR probe can be used to track changes in GSH levels and fluorescence imaging during the treatment of clear cell renal cell carcinoma (ccRCC) with celastrol (CeT) via inducing ferroptosis. These findings demonstrate that the developed fluorescent probe AR exhibits high selec-tivity and sensitivity, as well as good biocompatibility and long-term stability, which can be used to image endogenous GSH in living tumors and cells. Also, a significant decrease in GSH levels was observed by the fluorescent probe AR during the treatment of ccRCC with CeT-induced ferroptosis in vitro and in vivo. Overall, these findings will provide a novel strategy for celastrol targeting ferroptosis in the treatment of ccRCC and the application of fluorescent probes to help reveal the underlying mechanism of CeT in the treatment of ccRCC.
ArticleNumber 106454
Author Zeng, Qing
Deng, Changfeng
Zhu, Neng
Li, Hongfang
Zhang, Chanjuan
Qin, Li
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Keywords Ferroptosis
Fluorescence probe
Clear cell renal cell carcinoma
Celastrol
Glutathione
METABOLISM
DIRECT ELECTRON-TRANSFER
Language English
License This is an open access article under the CC BY-NC-ND license.
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– volume: 12
  year: 2021
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Snippet [Display omitted] •GSH-specific fluorescent probe for GSH detection in clinical samples and live cell and tumor imaging.•Celastrol induces ferroptosis in...
Glutathione (GSH) is closely related to the occurrence and development of tumors. The intracellular GSH levels are abnormally altered when tumor cells undergo...
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SubjectTerms Biochemistry & Molecular Biology
Carcinoma
Carcinoma, Renal Cell
Celastrol
Chemistry
Chemistry, Organic
Clear cell renal cell carcinoma
Ferroptosis
Fluorescence probe
Fluorescent Dyes - pharmacology
Glutathione
Glutathione - metabolism
Humans
Kidney Neoplasms
Life Sciences & Biomedicine
Physical Sciences
Science & Technology
Title An ultrasensitive GSH-specific fluorescent probe unveils celastrol-induced ccRCC ferroptosis
URI https://dx.doi.org/10.1016/j.bioorg.2023.106454
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https://www.ncbi.nlm.nih.gov/pubmed/36889199
https://search.proquest.com/docview/2785197422
Volume 134
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