Thallium Induces Antiproliferative and Cytotoxic Activity in Glioblastoma C6 and U373 Cell Cultures via Apoptosis and Changes in Cell Cycle

Edgar Rangel-López; Benjamín Robles-Bañuelos; Natalia Guadiana-Ramírez; Valeria Alvarez-Garduño; Sonia Galván-Arzate; Cecilia Zazueta; Cimen Karasu; Isaac Túnez; Alexey Tinkov; Michael Aschner; Abel Santamaría

doi:10.1007/s12640-022-00514-6

Thallium Induces Antiproliferative and Cytotoxic Activity in Glioblastoma C6 and U373 Cell Cultures via Apoptosis and Changes in Cell Cycle

Edgar Rangel-López, Benjamín Robles-Bañuelos, Natalia Guadiana-Ramírez, Valeria Alvarez-Garduño, Sonia Galván-Arzate, Cecilia Zazueta, Cimen Karasu, Isaac Túnez, Alexey Tinkov, Michael Aschner, Abel Santamaría

Molecular Pharmacology

Research output: Contribution to journal › Article › peer-review

6 Scopus citations

Abstract

Thallium (Tl⁺) is a heavy metal that causes toxicity in several organs, including the brain. Its cytotoxic profile, combined with its affinity for tumor cells when used as a radioligand for labeling these cells, suggests its potential use as antitumor therapy. In this study, glioblastoma cell lines C6 (from rat) and U373 (from human) were exposed to increased concentrations of thallium(I) acetate (5, 10, 50, 100, or 200 µM) and several toxic endpoints were evaluated, including loss of confluence and morphological changes, loss of cell viability, changes in cell cycle, and apoptosis. Tl⁺ was detected in cells exposed to thallium(I) acetate, demonstrating efficient uptake mechanism. Confluence in both cell lines decreased in a concentration-dependent manner (50–200 µM), while morphological changes (cell shrinkage and decreased cell volume) were more evident at exposures to higher Tl⁺ concentrations. For both parameters, the effects of Tl⁺ were more prominent in C6 cells compared to U373 cells. The same trend was observed for cell viability, with Tl⁺ affecting this parameter in C6 cells at low concentrations, whereas U373 cells showed greater resistance, with significant changes observed only at the higher concentrations. C6 and U373 cells treated with Tl⁺ also showed morphological characteristics corresponding to apoptosis. The cytotoxic effects of Tl⁺ were also assessed in neural and astrocytic primary cultures from the whole rat brain. Primary neural and astrocytic cultures were less sensitive than C6 and U373 cells, showing changes in cell viability at 50 and 100 µM concentrations, respectively. Cell cycle in both brain tumor cell lines was altered by Tl⁺ in G1/G2 and S phases. In addition, when combined with temozolamide (500 µM), Tl⁺ elicited cell cycle alterations, increasing SubG1 population. Combined, our novel results characterize and validate the cytotoxic and antiproliferative effects of Tl⁺ in glioblastoma cells.

Original language	English (US)
Pages (from-to)	814-824
Number of pages	11
Journal	Neurotoxicity Research
Volume	40
Issue number	3
DOIs	https://doi.org/10.1007/s12640-022-00514-6
State	Published - Jun 2022

Keywords

Apoptosis
C6
Cell cycle
Cell viability
Glioblastoma
Thallium cytoxicity
U373

ASJC Scopus subject areas

General Neuroscience
Toxicology

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Rangel-López, E., Robles-Bañuelos, B., Guadiana-Ramírez, N., Alvarez-Garduño, V., Galván-Arzate, S., Zazueta, C., Karasu, C., Túnez, I., Tinkov, A., Aschner, M., & Santamaría, A. (2022). Thallium Induces Antiproliferative and Cytotoxic Activity in Glioblastoma C6 and U373 Cell Cultures via Apoptosis and Changes in Cell Cycle. Neurotoxicity Research, 40(3), 814-824. https://doi.org/10.1007/s12640-022-00514-6

Rangel-López, E, Robles-Bañuelos, B, Guadiana-Ramírez, N, Alvarez-Garduño, V, Galván-Arzate, S, Zazueta, C, Karasu, C, Túnez, I, Tinkov, A, Aschner, M & Santamaría, A 2022, 'Thallium Induces Antiproliferative and Cytotoxic Activity in Glioblastoma C6 and U373 Cell Cultures via Apoptosis and Changes in Cell Cycle', Neurotoxicity Research, vol. 40, no. 3, pp. 814-824. https://doi.org/10.1007/s12640-022-00514-6

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abstract = "Thallium (Tl+) is a heavy metal that causes toxicity in several organs, including the brain. Its cytotoxic profile, combined with its affinity for tumor cells when used as a radioligand for labeling these cells, suggests its potential use as antitumor therapy. In this study, glioblastoma cell lines C6 (from rat) and U373 (from human) were exposed to increased concentrations of thallium(I) acetate (5, 10, 50, 100, or 200 µM) and several toxic endpoints were evaluated, including loss of confluence and morphological changes, loss of cell viability, changes in cell cycle, and apoptosis. Tl+ was detected in cells exposed to thallium(I) acetate, demonstrating efficient uptake mechanism. Confluence in both cell lines decreased in a concentration-dependent manner (50–200 µM), while morphological changes (cell shrinkage and decreased cell volume) were more evident at exposures to higher Tl+ concentrations. For both parameters, the effects of Tl+ were more prominent in C6 cells compared to U373 cells. The same trend was observed for cell viability, with Tl+ affecting this parameter in C6 cells at low concentrations, whereas U373 cells showed greater resistance, with significant changes observed only at the higher concentrations. C6 and U373 cells treated with Tl+ also showed morphological characteristics corresponding to apoptosis. The cytotoxic effects of Tl+ were also assessed in neural and astrocytic primary cultures from the whole rat brain. Primary neural and astrocytic cultures were less sensitive than C6 and U373 cells, showing changes in cell viability at 50 and 100 µM concentrations, respectively. Cell cycle in both brain tumor cell lines was altered by Tl+ in G1/G2 and S phases. In addition, when combined with temozolamide (500 µM), Tl+ elicited cell cycle alterations, increasing SubG1 population. Combined, our novel results characterize and validate the cytotoxic and antiproliferative effects of Tl+ in glioblastoma cells.",

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author = "Edgar Rangel-L{\'o}pez and Benjam{\'i}n Robles-Ba{\~n}uelos and Natalia Guadiana-Ram{\'i}rez and Valeria Alvarez-Gardu{\~n}o and Sonia Galv{\'a}n-Arzate and Cecilia Zazueta and Cimen Karasu and Isaac T{\'u}nez and Alexey Tinkov and Michael Aschner and Abel Santamar{\'i}a",

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AU - Rangel-López, Edgar

AU - Robles-Bañuelos, Benjamín

AU - Guadiana-Ramírez, Natalia

AU - Alvarez-Garduño, Valeria

AU - Galván-Arzate, Sonia

AU - Zazueta, Cecilia

AU - Karasu, Cimen

AU - Túnez, Isaac

AU - Tinkov, Alexey

AU - Aschner, Michael

AU - Santamaría, Abel

PY - 2022/6

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N2 - Thallium (Tl+) is a heavy metal that causes toxicity in several organs, including the brain. Its cytotoxic profile, combined with its affinity for tumor cells when used as a radioligand for labeling these cells, suggests its potential use as antitumor therapy. In this study, glioblastoma cell lines C6 (from rat) and U373 (from human) were exposed to increased concentrations of thallium(I) acetate (5, 10, 50, 100, or 200 µM) and several toxic endpoints were evaluated, including loss of confluence and morphological changes, loss of cell viability, changes in cell cycle, and apoptosis. Tl+ was detected in cells exposed to thallium(I) acetate, demonstrating efficient uptake mechanism. Confluence in both cell lines decreased in a concentration-dependent manner (50–200 µM), while morphological changes (cell shrinkage and decreased cell volume) were more evident at exposures to higher Tl+ concentrations. For both parameters, the effects of Tl+ were more prominent in C6 cells compared to U373 cells. The same trend was observed for cell viability, with Tl+ affecting this parameter in C6 cells at low concentrations, whereas U373 cells showed greater resistance, with significant changes observed only at the higher concentrations. C6 and U373 cells treated with Tl+ also showed morphological characteristics corresponding to apoptosis. The cytotoxic effects of Tl+ were also assessed in neural and astrocytic primary cultures from the whole rat brain. Primary neural and astrocytic cultures were less sensitive than C6 and U373 cells, showing changes in cell viability at 50 and 100 µM concentrations, respectively. Cell cycle in both brain tumor cell lines was altered by Tl+ in G1/G2 and S phases. In addition, when combined with temozolamide (500 µM), Tl+ elicited cell cycle alterations, increasing SubG1 population. Combined, our novel results characterize and validate the cytotoxic and antiproliferative effects of Tl+ in glioblastoma cells.

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Thallium Induces Antiproliferative and Cytotoxic Activity in Glioblastoma C6 and U373 Cell Cultures via Apoptosis and Changes in Cell Cycle

Abstract

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