Evaluating toxicity and level of DNA damage in human fetal lung cells upon exposure to 5-methyltetrahydrofolate (bioactive folate).

IF 1.9 Q3 NUTRITION & DIETETICS Nutrition and health Pub Date : 2024-12-18 DOI:10.1177/02601060241302895
Chetna Karkera, Alireza G Senejani
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Abstract

Background: Folic acid (FA) supplementation is widely regarded as a key nutritional intervention during pregnancy due to its protective effect against neural tube defects. Recent research has reported FA supplementation outcomes on offspring's health, with increased incidences of allergy/respiratory problems. Aim: This study evaluates if increased levels of 5-methyltetrahydrofolate (5-MTHF) are associated with DNA modification, leading to disruption of cell proliferation in fetal lung cells and increasing susceptibility to asthma. Methods: Two fetal lung cells, MRC5 and IMR90, were treated with nine concentrations of 5-MTHF for six time points. Cell viability was evaluated using Trypan Blue staining. Flow cytometry analysis to quantify DNA content in cells was done with a propidium iodide stain. Followed by 1.6 mM glutathione treatment to alleviate the oxidative stress caused by 5-MTHF. A quantitative test for DNA damage was executed using neutral and alkaline comet assay. Gene expression study for five genes namely MTR, MTHFD1, XRCC1, Pol β, and epidermal growth factor receptor (EGFR) was evaluated using a 2-step quantitative reverse transcription polymerase chain reaction. Results: Fetal lung cell survival rate remained unaffected with 5-MTHF concentration below 1.25 µM. Beyond this concentration, cell viability is reduced with an increase in concentration. Cell cycle analysis revealed cell arrest in the G1 phase. The antioxidant activity of glutathione led the cells to bypass this arrest. Precisely, 10 and 50 µM 5-MTHF concentrations led to double-strand DNA breaks and single-strand DNA breaks. Gene expression study revealed lower expression of the MTR gene and higher expression of MTHFD1, EGFR, XRCC1, and DNA Pol β gene with an increase in 5-MTHF concentration. Conclusion: 5-MTHF concentration higher than 1.25 µM led to DNA damage in MRC5 and IMR90 human fetal lung cells.

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评估人类胎儿肺细胞接触 5-甲基四氢叶酸(生物活性叶酸)后的毒性和 DNA 损伤程度。
背景:叶酸(FA)的补充由于其对神经管缺陷的保护作用而被广泛认为是孕期重要的营养干预措施。最近的研究报告了补充FA对后代健康的影响,增加了过敏/呼吸问题的发生率。目的:本研究评估5-甲基四氢叶酸(5-MTHF)水平升高是否与DNA修饰相关,从而导致胎儿肺细胞增殖中断并增加对哮喘的易感。方法:用9种浓度的5-MTHF处理6个时间点的2个胎儿肺细胞MRC5和IMR90。台盼蓝染色法检测细胞活力。用碘化丙啶染色进行流式细胞术分析以定量细胞中的DNA含量。随后给予1.6 mM谷胱甘肽处理,缓解5-MTHF引起的氧化应激。采用中性和碱性彗星法对DNA损伤进行定量检测。采用两步定量逆转录聚合酶链反应对MTR、MTHFD1、XRCC1、Pol β和表皮生长因子受体(EGFR) 5个基因的表达进行研究。结果:5-MTHF浓度低于1.25µM时,胎儿肺细胞存活率未受影响。超过这个浓度,细胞活力随着浓度的增加而降低。细胞周期分析显示细胞阻滞在G1期。谷胱甘肽的抗氧化活性使细胞绕过了这种阻滞。精确地说,10µM和50µM 5-MTHF浓度导致双链DNA断裂和单链DNA断裂。基因表达研究显示,随着5-MTHF浓度的升高,MTR基因的表达降低,MTHFD1、EGFR、XRCC1和DNA Pol β基因的表达升高。结论:5-MTHF浓度高于1.25µM可导致人胎肺细胞MRC5和IMR90 DNA损伤。
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来源期刊
Nutrition and health
Nutrition and health Medicine-Medicine (miscellaneous)
CiteScore
3.50
自引率
0.00%
发文量
160
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