[自然杀伤细胞来源外泌体中的miR-30e-3p抑制人食管鳞癌细胞的增殖和侵袭]。

Mingyue Sun, Honglin Li, Baorong Feng
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引用次数: 0

摘要

目的探讨自然杀伤(NK)细胞来源的含mir -30e-3p的外泌体(Exo)对食管鳞癌(ESCC)细胞增殖、凋亡和侵袭的影响。方法从健康供者外周血中分离扩增NK细胞,分离鉴定NK细胞来源的Exo细胞,与NEC细胞共培养,随机分为Exo1组和Exo2组。透射电镜(TEM)观察外泌体的形态和大小。Western blot检测外泌体标志物凋亡相关基因2-相互作用蛋白X(ALIX)、肿瘤易感基因101(TSG101)、CD81、calnexin的表达水平。将NC质粒、miR030e-3p的模拟物和抑制物分别送入NK细胞,并将相应的NK细胞衍生的Exo与NEC细胞共培养,将NEC细胞分为NC、Exo、模拟物和抑制物组。CCK-8法检测细胞增殖,流式细胞术检测细胞周期,annexin V-FITC/PI双染色检测细胞凋亡,TranswellTM法检测细胞侵袭能力。采用Real-time定量PCR检测miR-23b、miR-422a、miR-133b、miR-124、miR-30e-3p和miR-99a在NCE细胞和外泌体中的表达。结果NK细胞中CD56+CD3+细胞和CD56+CD16+细胞的比例分别为(0.071±0.008)%和(90.6±10.6)%。NK细胞外泌体在30 ~ 150 nm范围内,ALIX、TSG101和CD81阳性,calnexin阴性。NK细胞源性Exos抑制增殖,降低NEC细胞s期细胞比例和侵袭细胞数量,促进G1期细胞的凋亡和比例。NK细胞源性外泌体中过表达miR-30E-3p抑制NEC细胞的增殖和侵袭,阻断细胞周期,促进细胞凋亡,而NK细胞源性外泌体中低表达miR-30E-3p则相反。结论NK细胞源性外泌体中的miR-30e-3p能够抑制ESCC细胞的增殖和侵袭,阻断其细胞周期,诱导其凋亡。
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[miR-30e-3p in natural killer cell-derived exosomes inhibits the proliferation and invasion of human esophageal squamous carcinoma cells].

Objective To investigate the effects of natural killer (NK)-cell-derived miR-30e-3p-containing exosomes (Exo) on esophageal squamous cell carcinoma (ESCC) cell proliferation, apoptosis and invasion. Methods NK cells were isolated and amplified from the peripheral blood of healthy donors, and NK cell-derived Exo was isolated and identified, which were further co-cultured with NEC cells and were randomly grouped into Exo1 and Exo2 groups. Transmission electron microscopy (TEM) was used to observe the morphology and size of exosomes. Western blot analysis was used to detect the expression levels of exosome markers apoptosis related gene 2- interacting protein X(ALIX), tumor susceptibility gene 101(TSG101), CD81 and calnexin. The NC plasmids, mimics and inhibitors of miR030e-3p were respectively delivered into the NK cells, and the corresponding NK cells-derived Exo were co-cultured with NEC cells, which were divided into NC, Exo, mimic and inhibitor groups. CCK-8 assay was used to evaluate cell proliferation, flow cytometry was conducted to determine cell cycle, annexin V-FITC/PI double staining was employed to detect cell apoptosis, and TranswellTM assay was performed to detect cell invasion abilities. Real-time quantitative PCR was used to detect the expression of miR-23b, miR-422a, miR-133b, miR-124, miR-30e-3p and miR-99a in NCE cells and exosomes. Results The percentages of CD56+CD3+ cells and CD56+CD16+ cells in NK cells were (0.071±0.008)% and (90.6±10.6)%, respectively. Exosome isolated from NK cells ranged from 30 nm to 150 nm, and was positive for ALIX, TSG101 and CD81, while negative for calnexin. NK cell-derived Exos inhibited the proliferation, reduced the proportion of S-phase cells and the number of invaded cells of NEC cells, and promoted the apoptosis and the proportion of G1 phase cells. Overexpression of miR-30E-3p in NK cell-derived exosome inhibited the proliferation and invasion of NEC cells, and blocked cell cycle and promoted apoptosis, while knockdown miR-30e-3p in NK cell-derived exosomes did the opposite. Conclusion miR-30e-3p in NK cell-derived exosomes can inhibit the proliferation and invasion of ESCC cells, block their cell cycle and induce their apoptosis.

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