The effect of Apigenin on glycometabolism and cell death in an anaplastic thyroid cancer cell line.
1/5 보강
PICO 자동 추출 (휴리스틱, conf 2/4)
유사 논문P · Population 대상 환자/모집단
추출되지 않음
I · Intervention 중재 / 시술
Apigenin relative to the control group
C · Comparison 대조 / 비교
추출되지 않음
O · Outcome 결과 / 결론
The scratch assays revealed that Apigenin treatment of cancer cell lines inhibited cell migration as compared to control. [CONCLUSION] These findings demonstrate the possibility of targeting the glucose facilitators' pathway for making thyroid cancer cells more susceptible to programmed cell death.
[AIMS AND BACKGROUND] A more pronounced characteristic of cancer cells is the energy dependence on glucose, which mitigated by glucose transporters.
APA
Heydarzadeh S, Moshtaghie AA, et al. (2023). The effect of Apigenin on glycometabolism and cell death in an anaplastic thyroid cancer cell line.. Toxicology and applied pharmacology, 475, 116626. https://doi.org/10.1016/j.taap.2023.116626
MLA
Heydarzadeh S, et al.. "The effect of Apigenin on glycometabolism and cell death in an anaplastic thyroid cancer cell line.." Toxicology and applied pharmacology, vol. 475, 2023, pp. 116626.
PMID
37437745 ↗
Abstract 한글 요약
[AIMS AND BACKGROUND] A more pronounced characteristic of cancer cells is the energy dependence on glucose, which mitigated by glucose transporters. The comprehension of the regulatory mechanisms behind the Warburg effect holds promise for developing therapeutic interventions for cancers. Studies are lacking which targeted the GLUTs for treatment of malignancy of thyroid tumors. In our current investigation, we have undertaken this study to determine the potential of Apigenin, plant derived flavonoid in modulating tumor apoptosis by targeting GLUTs expression in SW1736 cell line of anaplastic thyroid carcinoma.
[MATERIAL METHODS] Flow cytometry with propidium iodide staining was used to determine cell apoptosis. For glucose uptake detection, the "GOD-PAP" enzymatic colorimetric test was used to measure the direct glucose levels inside the cells. To determine the expression of GLUT1 and GLUT3 mRNA in the SW1736 cell line qRT-PCR was employed. Protein levels of GLUT1 and GLUT3 in the SW1736 cell line were detected with western blotting. Also, the scratch wound healing assay was conducted for cell migration.
[RESULTS] According to qRT-PCR analysis, the levels of GLUT1 and GLUT3 mRNA were lower in the group that received Apigenin relative to the control group. The Apigenin treatment of SW1736 cells decreased protein expression of the GLUT1 and GLUT3 levels in conformity to qRT-PCR. The scratch assays revealed that Apigenin treatment of cancer cell lines inhibited cell migration as compared to control.
[CONCLUSION] These findings demonstrate the possibility of targeting the glucose facilitators' pathway for making thyroid cancer cells more susceptible to programmed cell death.
[MATERIAL METHODS] Flow cytometry with propidium iodide staining was used to determine cell apoptosis. For glucose uptake detection, the "GOD-PAP" enzymatic colorimetric test was used to measure the direct glucose levels inside the cells. To determine the expression of GLUT1 and GLUT3 mRNA in the SW1736 cell line qRT-PCR was employed. Protein levels of GLUT1 and GLUT3 in the SW1736 cell line were detected with western blotting. Also, the scratch wound healing assay was conducted for cell migration.
[RESULTS] According to qRT-PCR analysis, the levels of GLUT1 and GLUT3 mRNA were lower in the group that received Apigenin relative to the control group. The Apigenin treatment of SW1736 cells decreased protein expression of the GLUT1 and GLUT3 levels in conformity to qRT-PCR. The scratch assays revealed that Apigenin treatment of cancer cell lines inhibited cell migration as compared to control.
[CONCLUSION] These findings demonstrate the possibility of targeting the glucose facilitators' pathway for making thyroid cancer cells more susceptible to programmed cell death.
🏷️ 키워드 / MeSH 📖 같은 키워드 OA만
같은 제1저자의 인용 많은 논문 (5)
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- Regulation of iodine-glucose flip-flop in SW1736 anaplastic thyroid cancer cell line.
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