[Circ_0000263 improves radiosensitivity of Hela cells by inhibiting the activity of telomerase protein through miR-338-3p/TERT].

C Wang, Y K Huo, M Y Li, C Li, X H Shen, S J Wang, Y F Liu, Z X Jiang
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引用次数: 0

Abstract

Objective: To explore the effect and molecular mechanism of circ_0000263 on HeLa cell activity, apoptosis, telomerase activity, and radiosensitivity. Methods: The Hela cells were divided into si-NC, si-circ, vector, circ_0000263, anti-NC, anti-miR-338-3p, miR-NC, miR-338-3p, si-circ+anti-NC, si-circ+ anti-miR-338-3p, si-circ+vector, si-circ+TERT, sh-NC, sh-circ groups. Reverse transcription-quantitative real-time polymerase chain reaction (RT-qPCR) was used to detect the expressions of circ_0000263 and miR-338-3p. Cell clone formation array was used to detect cell survival; cell counting kit-8 (CCK-8) to detect cell proliferation; flow cytometry to detect apoptosis; western blot method to detect the expressions of proliferating cell nuclear antigen (PCNA), Cleaved-casp3, telomerase reverse transcriptase (TERT) proteins; double luciferase assay to detect the targeting relationships of circ_0000263 and miR-338-3p, miR-338-3p and TERT; telomere repeat amplification enzyme linked immunosorbent assay (TRAR-ELISA) to detect telomerase activity. Results: Circ_0000263 was highly expressed in Hela cells, miR-338-3p was low expressed, and TERT was highly expressed; circ_0000263 was also highly expressed in Hela cells treated with radiation (P<0.05). Knockdown of circ_0000263 inhibited the clone formation and cell proliferation ability of HeLa cells, and enhanced the radiosensitivity and apoptosis of HeLa cells. In contrast, knockdown of circ_0000263 decreased PCNA protein expression level and enhanced Cleaved-casp3 protein expression level in HeLa cells (P<0.05). The apoptosis rate in the si-circ group was (13.19±1.12)%, which was higher than (6.80±0.62)% of si-NC group (P<0.05). The apoptosis rate in the si-circ+4 Gy group was (24.82±1.57)%, which was higher than (17.00±0.96)% of si-NC+4 Gy group (P<0.05). Circ_0000263 targeted regulated miR-338-3p, and miR-338-3p targeted regulated TERT. MiR-338-3p was lowly expressed in HeLa cells, and knockdown of circ_0000263 elevated miR-338-3p expression level in HeLa cells. Circ_0000263 regulated TERT expression and inhibited telomerase activity through miR-338-3p. MiR-338-3p/TERT can restore the effect of circ_0000263 on the radiosensitivity of Hela cells. The apoptosis rate in the si-circ+anti-NC group was (27.37±0.89)%, which was higher than (18.22±1.18)% of the si-circ+anti-miR-338-3p group (P<0.05). The apoptosis rate in the si-circ+vector group was (27.55±0.48)%, which was higher than (20.10±0.68)% of si-circ+TERT group (P<0.05). After 72 hours of radiation by 4 Gy, the cell survival fraction of si-circ+anti-NC group was 0.41±0.02, which was lower than 0.66±0.03 of the si-circ+anti-miR-338-3p group (P<0.05); the cell survival fraction of si-circ+vector group was 0.42±0.05, which was lower than 0.70±0.03 of si-circ+TERT group (P<0.05). Conclusion: Inhibiting the expression of circ_0000263 supresses the proliferation of Hela cells by regulating miR-338-3p/TERT, promotes apoptosis, inhibits telomerase activity, increases the radiosensitivity of cancer cells, and provides a theoretical basis for improving the radiosensitivity of Hela cells.

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[Circ_0000263通过miR-338-3p/TERT抑制端粒酶蛋白的活性,从而提高Hela细胞的放射敏感性】。]
研究目的探讨circ_0000263对HeLa细胞活性、凋亡、端粒酶活性和放射敏感性的影响及分子机制。方法将 Hela 细胞分为 si-NC 组、si-circ 组、载体组、circ_0000263 组、anti-NC 组、anti-miR-338-3p 组、miR-NC 组、miR-338-3p 组、si-circ+anti-NC 组、si-circ+anti-miR-338-3p 组、si-circ+载体组、si-circ+TRT 组、sh-NC 组、sh-circ 组。采用逆转录-实时定量聚合酶链反应(RT-qPCR)检测 circ_0000263 和 miR-338-3p 的表达。细胞克隆形成阵列检测细胞存活;细胞计数试剂盒-8(CCK-8)检测细胞增殖;流式细胞仪检测细胞凋亡;Western印迹法检测增殖细胞核抗原(PCNA)、裂解-casp3、端粒酶逆转录酶(TERT)蛋白的表达;双荧光素酶试验检测circ_0000263与miR-338-3p、miR-338-3p与TERT的靶向关系;端粒重复扩增酶联免疫吸附试验(TRAR-ELISA)检测端粒酶活性。结果Circ_0000263在Hela细胞中高表达,miR-338-3p低表达,TERT高表达;Circ_0000263在经辐射处理的Hela细胞中也高表达(P<0.05)。敲除 circ_0000263 可抑制 HeLa 细胞的克隆形成和细胞增殖能力,增强 HeLa 细胞的辐射敏感性和凋亡能力。相反,敲除 circ_0000263 会降低 HeLa 细胞 PCNA 蛋白表达水平,提高 Cleaved-casp3 蛋白表达水平(P<0.05)。si-circ 组的细胞凋亡率为(13.19±1.12)%,高于 si-NC 组的(6.80±0.62)%(P<0.05)。si-circ+4 Gy组的细胞凋亡率为(24.82±1.57)%,高于si-NC+4 Gy组的(17.00±0.96)%(P<0.05)。Circ_0000263靶向调控miR-338-3p,miR-338-3p靶向调控TERT。MiR-338-3p在HeLa细胞中低表达,而敲除circ_0000263可提高HeLa细胞中miR-338-3p的表达水平。Circ_0000263 通过 miR-338-3p 调节 TERT 的表达并抑制端粒酶的活性。MiR-338-3p/TERT 可以恢复 circ_0000263 对 Hela 细胞辐射敏感性的影响。si-circ+anti-NC 组的细胞凋亡率为(27.37±0.89)%,高于 si-circ+anti-miR-338-3p 组的(18.22±1.18)%(P<0.05)。si-circ+vector 组的细胞凋亡率为(27.55±0.48)%,高于 si-circ+TERT 组的(20.10±0.68)%(P<0.05)。4Gy照射72小时后,si-circ+抗NC组细胞存活率为(0.41±0.02)%,低于si-circ+抗miR-338-3p组的(0.66±0.03)%(P<0.05);si-circ+载体组细胞存活率为(0.42±0.05)%,低于si-circ+TERT组的(0.70±0.03)%(P<0.05)。结论抑制circ_0000263的表达可通过调控miR-338-3p/TERT抑制Hela细胞的增殖,促进细胞凋亡,抑制端粒酶活性,提高癌细胞的放射敏感性,为提高Hela细胞的放射敏感性提供理论依据。
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中华肿瘤杂志
中华肿瘤杂志 Medicine-Medicine (all)
CiteScore
1.40
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10433
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