In vitro toxicological assessment of PhSeZnCl in human liver cells

被引:7
|
作者
di Vito, Raffaella [1 ,3 ]
Levorato, Sara [1 ,4 ]
Fatigoni, Cristina [1 ]
Acito, Mattia [1 ]
Sancineto, Luca [2 ]
Traina, Giovanna [3 ]
Villarini, Milena [1 ]
Santi, Claudio [2 ]
Moretti, Massimo [1 ]
机构
[1] Univ Perugia, Dept Pharmaceut Sci, Unit Publ Hlth, Via Giochetto, I-06122 Perugia, Italy
[2] Univ Perugia, Dept Pharmaceut Sci, Grp Catalysis Synth & Organ Green Chem, I-06123 Perugia, Italy
[3] Univ Perugia, Dept Pharmaceut Sci, Unit Physiol, Via San Costanzo, I-06126 Perugia, Italy
[4] European Food Safety Author, Via Carlo Magno 1A, I-43126 Parma, Italy
关键词
Phenylselenenylzinc chloride; HepG2; HepaRG; Comet assay; Apoptosis; Cell cycle; METABOLICALLY COMPETENT; GLUTATHIONE-PEROXIDASE; HEPARG CELLS; COMET ASSAY; SELENIUM; APOPTOSIS; CANCER; LINE; CHEMOPREVENTION; CULTURE;
D O I
10.1007/s43188-022-00148-y
中图分类号
R99 [毒物学(毒理学)];
学科分类号
100405 ;
摘要
Phenylselenenylzinc chloride (PhSeZnCl) is an air-stable selenolate, easily synthesizable through oxidative insertion of elemental zinc into the Se-halogen bond of the commercially available phenylselenyl chloride. PhSeZnCl was shown to possess a marked GPx-like activity both in NMR and in vitro tests, and to effectively react with cellular thiols, and was supposed for a potential use in the chemotherapy of drug-resistant cancers. However, activity of PhSeZnCl in hepatic cells has never been tested before now. In this in vitro approach, we evaluated the cytotoxic, genotoxic, and apoptotic activities, as well as the effects on cell cycle of PhSeZnCl in two preclinical hepatic models, namely HepG2 and HepaRG cells. Results showed that cell viability of HepG2 and HepaRG cells decreased in a dose-dependent manner, with a more marked effect in HepG2 tumour cells. Moreover, treatment with 50 mu g/mL PhSeZnCl caused an increase of primary DNA damage (4 h) and a statistically significant increase of HepG2 cells arrested in G(2)/M phase. In addition, it altered mitochondrial membrane potential and induced chromosomal DNA fragmentation (24 h). In HepaRG cells, PhSeZnCl was able to determine a cell cycle-independent induction of apoptosis. Particularly, 50 mu g/mL induced mitochondrial membrane depolarization after 24 h and apoptosis after 4 h treatment. Futhermore, all PhSeZnCl concentrations tested determined a significant increase of apoptotic cells after 24 h. Apoptosis was also highlighted by the detection of active Caspase-3 by Western Blot analysis after 24 h exposure. In conclusion, this first toxicological assessment provides new insights into the biological activity of PhSeZnCl in preclinical hepatic models that will be useful in future safety assessment investigation of this compound as a potential pharmaceutical.
引用
收藏
页码:105 / 114
页数:10
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