Institute of Life Science, Faculty of Medicine, Health and Life Science, Swansea University, Singleton Park, Swansea SA2 8PP, UK.
Institute of Life Science, Faculty of Medicine, Health and Life Science, Swansea University, Singleton Park, Swansea SA2 8PP, UK.
Mutat Res Genet Toxicol Environ Mutagen. 2024 May-Jun;896:503766. doi: 10.1016/j.mrgentox.2024.503766. Epub 2024 May 18.
In this paper, we studied the potential genotoxic effects of human plasma from healthy volunteers, as well as patients with gastro-oesophageal reflux disease, Barrett's oesophagus (BO) and oesophageal adenocarcinoma (OAC) using the oesophageal adenocarcinoma cell line (OE33) and the lymphoblastoid cell line (TK6). Both TK6 and OE33 cells were treated with plasma (10 % volume, replacing foetal bovine serum (FBS) or horse serum (HS)) at different time points of 4 h (for the micronucleus (Mn) assay and the invasion assay) and 24 h (for the cell cycle studies). Plasma-induced effects on DNA damage levels, cell viability and the cell cycle were studied by the micronucleus assay, cytokinesis block proliferation index (CBPI) and flow cytometry respectively. The expression of IL-8 in supernatants of TK6 cells and IFN-β in OE33 cells was also analysed by enzyme-linked immunosorbent assay (ELISA). Finally, we carried out an assessment of cellular invasion of OE33 cells following plasma treatment. The results of the micronucleus assay confirmed the genotoxicity of direct plasma treatment from some participants through the increase in DNA damage in TK6 cells. Conversely, some individual patient plasma samples reduced background levels of TK6 cell Mn frequency, in an anti-genotoxic fashion. In TK6 cells, (on average) plasma samples from patients with Barrett's oesophagus induced higher micronucleus levels than healthy volunteers (p= 0.0019). There was little difference in Mn induction when using plasma versus serum to treat the cells in vitro. Cell cycle results showed that direct plasma treatment had a marked impact on OE33 cells at 24 h (p=0.0182 for BO and p=0.0320 for OAC) by decreasing the proportion of cells in the S phase, while plasma exposure was less impactful on the cell cycle of TK6 cells. Invasion of OE33 cells was also seen to be non-significantly affected by plasma treatment of OE33 cells. The addition of N-acetyl cysteine NAC in a dose-dependent matter did not alter the formation of Mn in TK6 cells, suggesting that reactive oxygen species (ROS) are not the root cause of plasma's genotoxicity. The concentration of IL-8 in TK6 cells and IFN-β in OE33 cells was significantly higher in cells treated with OAC-derived plasma than in the untreated negative control. Collectively, our results demonstrate that plasma-specific effects are detectable which helps us better understand some important aspects of the biology of blood-based biomarkers under development.
本文研究了来自健康志愿者、胃食管反流病(GERD)、巴雷特食管(BO)和食管腺癌(OAC)患者的人血浆的潜在遗传毒性作用,使用食管腺癌细胞系(OE33)和淋巴母细胞系(TK6)。将 TK6 和 OE33 细胞分别用 10%体积的血浆(替代胎牛血清(FBS)或马血清(HS))处理 4 小时(用于微核(Mn)测定和侵袭测定)和 24 小时(用于细胞周期研究)。通过微核测定、细胞有丝分裂阻断增殖指数(CBPI)和流式细胞术分别研究血浆对 DNA 损伤水平、细胞活力和细胞周期的影响。通过酶联免疫吸附试验(ELISA)分析 TK6 细胞上清液中白细胞介素-8(IL-8)和 OE33 细胞中干扰素-β(IFN-β)的表达。最后,我们评估了血浆处理后 OE33 细胞的细胞侵袭情况。微核测定结果证实了一些参与者的直接血浆处理具有遗传毒性,因为这会增加 TK6 细胞中的 DNA 损伤。相反,一些个体患者的血浆样本以抗遗传毒性的方式降低了 TK6 细胞 Mn 频率的背景水平。在 TK6 细胞中,(平均而言)来自 BO 患者的血浆样本比健康志愿者诱导更高的微核水平(p=0.0019)。在体外用血浆和血清处理细胞时,Mn 诱导的差异很小。细胞周期结果表明,直接血浆处理在 24 小时时对 OE33 细胞有显著影响(BO 为 p=0.0182,OAC 为 p=0.0320),降低了 S 期细胞的比例,而血浆暴露对 TK6 细胞的细胞周期影响较小。OE33 细胞的侵袭也被观察到不受 OE33 细胞血浆处理的影响。N-乙酰半胱氨酸(NAC)以剂量依赖性的方式添加并没有改变 TK6 细胞中 Mn 的形成,这表明活性氧(ROS)不是血浆遗传毒性的根本原因。与未处理的阴性对照相比,OE33 细胞中来自 OAC 衍生血浆处理的细胞中白细胞介素-8(IL-8)和 OE33 细胞中干扰素-β(IFN-β)的浓度明显更高。总的来说,我们的结果表明,可以检测到血浆特异性影响,这有助于我们更好地理解正在开发的基于血液的生物标志物的生物学的一些重要方面。
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