circBIRC6通过miR-944/CD44轴促进PD-L1介导的非小细胞肺癌免疫逃逸

doi:10.3969/j.issn.1006-6233.2022.12.006

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摘要 目的: 通过观察环状RNA(circRNA)BIRC6(circBIRC6)在非小细胞肺癌(NSCLC)中的表达探讨其在肿瘤细胞免疫逃逸中的作用及分子机制。方法: 体外培养人NSCLC细胞系(H1975、HCC827、H1650、H1299和A549)和人正常肺上皮细胞系(BEAS-2B),qRT-PCR检测检测circBIRC6、miR-944和分化簇44(CD44)、程序性细胞死亡配体1(PD-L1)的表达。取A549细胞,分为正常对照(NC)组、si-NC组、si-circBIRC6组、si-circBIRC6+anti-NC组、si-circBIRC6+anti-miR-944组。转染48h后,采用qRT-PCR和Western blot检测细胞中circBIRC6、miR-944和CD44、PD-L1的mRNA和蛋白表达水平;MTT法检测细胞增殖活性,Transwell小室检测细胞迁移、侵袭能力;将A549细胞与CD8⁺T细胞共培养,台盼蓝染色测定共培养系统中CD8⁺T细胞活力,流式细胞术检测共培养系统中CD8⁺T细胞凋亡,ELISA法检测共培养细胞培养上清液中可溶性PD-L1(sPD-L1)、干扰素-γ(INF-γ)、肿瘤坏死因子α(TNF-α)、颗粒酶B和穿孔素水平,验证敲低circBIRC6在NSCLC免疫逃逸中的作用。通过双荧光素酶报告(DLRA)、RNA免疫沉淀(RIP)和RNA pull-down实验验证A549细胞中circBIRC6、miR-944和CD44的调控机制。结果: circBIRC6和CD44、PD-L1在NSCLC中呈高表达,miR-944呈低表达。敲低circBIRC6(0.36±0.05比1.01±0.12)可上调miR-944(3.45±0.38比0.99±0.10),抑制CD44 mRNA(0.39±0.05比1.00±0.10)、CD44蛋白(0.25±0.05比0.64±0.07)和PD-L1 mRNA(0.31±0.04比1.00±0.13)、PD-L1蛋白(0.17±0.03比0.52±0.06)表达,降低A549细胞增殖活力和迁移、侵袭能力(均P<0.05)。在共培养系统中,敲低circBIRC6的A549细胞可激活CD8⁺T细胞[(68.35±7.20)%比(35.82±4.14)%],抑制CD8⁺T细胞凋亡[(23.85±3.76)%比(56.01±6.22)%],降低sPD-L1水平,增加IFN-γ、TNF-α、颗粒酶B和穿孔素水平(均P<0.05)。下调miR-944可减弱circBIRC6敲低对A549细胞增殖、迁移和侵袭及CD8⁺T细胞活化的影响。DLRA、RIP和RNA pull-down实验证实circBIRC6可以靶向并结合A549细胞中的miR-944,且CD44是miR-944的靶标。结论: 敲低A549细胞中的circBIRC6可通过下调PD-L1的表达和分泌,激活肿瘤微环境中的CD8⁺T细胞,进而抑制NSCLC的免疫逃逸;其分子机制可能与miR-944/CD44轴对PD-L1的调控作用有关。

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关键词 ：非小细胞肺癌, 环状RNA, circBIRC6, miR-944, 分化簇44, 程序性细胞死亡配体1, 免疫逃逸

Abstract：Objective: To observe the expression of circular RNA (circRNA) BIRC6 (circBIRC6) in non-small cell lung cancer (NSCLC) and to explore its role and molecular mechanism in tumor cell immune escape. Methods: Human NSCLC cell lines (H1975, HCC827, H1650, H1299, and A549) and human normal lung epithelial cell lines (BEAS-2B) were cultured in vitro. The expressions of circBIRC6, miR-944, cluster of differentiation 44 (CD44) and programmed cell death ligand 1 (PD-L1) were detected by qRT-PCR. A549 cells were collected and separated into normal control (NC) group, si-NC group, si-circBIRC6 group, si-circBIRC6+anti-NC group, and si-circBIRC6+anti-miR-944 group. 48h after transfection, qRT-PCR and Western blot were applied to detect the mRNA and protein expression levels of circBIRC6, miR-944, CD44 and PD-L1 in cells; MTT assay was applied to detect cell proliferation activity; Transwell chambers were used to detect cell migration and invasion ability; A549 cells were co-cultured with CD8⁺ T cells; Trypan blue staining was applied to determine CD8⁺T cell viability in co-culture systems; flow cytometry was applied to detect CD8⁺T cell apoptosis in co-culture systems; ELISA was applied to detect the levels of soluble PD-L1 (sPD-L1), interferon-γ (INF-γ), tumor necrosis factor alpha (TNF-α), granzyme B, and perforin in culture supernatants of co-cultured cells; the role of knockdown of circBIRC6 in NSCLC immune escape was validated. Dual-luciferase reporter (DLRA), RNA immunoprecipitation (RIP) and RNA pull-down experiments were applied to validate the regulatory mechanisms of circBIRC6, miR-944 and CD44 in A549 cells. Results: CircBIRC6, CD44 and PD-L1 were highly expressed in NSCLC, while miR-944 was lowly expressed in NSCLC. Knockdown of circBIRC6 (0. 36±0. 05 vs 1. 01±0. 12) could up-regulate miR-944 (3. 45±0. 38 vs 0. 99±0. 10), inhibit the expression of CD44 mRNA (0. 39±0. 05 vs 1. 00±0. 10), CD44 protein (0. 25±0. 05 vs 0. 64±0. 07)and PD-L1 mRNA (0. 31±0. 04 vs 1. 00±0. 13), PD-L1 protein (0. 17±0. 03 vs 0. 52±0. 06), and greatly reduce the proliferation, migration and invasion abilities of A549 cells (all P<0. 05). In the co-culture system, knockdown of circBIRC6 in A549 cells could activate CD8⁺T cells [(68. 35±7. 20) % vs (35. 82±4. 14) %], inhibit the apoptosis of CD8⁺T cells [(23. 85±3. 76) % vs (56. 01±6. 22) %], reduce the level of sPD-L1 in the supernatant, increase the levels of IFN-γ, TNF-α, granzyme B and perforin (all P<0. 05). Down-regulation of miR-944 increased the expressions of CD44 and PD-L1, and attenuated the effects of circBIRC6 knockdown on the proliferation, migration and invasion of A549 cells and activation of CD8⁺ T cells (all P<0. 05). DLRA, RIP and RNA pull-down experiments confirmed that circBIRC6 could target and bind to miR-944 in A549 cells, and CD44 was the target of miR-944. Conclusion: Knockdown of circBIRC6 in A549 cells can activate CD8⁺ T cells in the tumor microenvironment by down-regulating the expression and secretion of PD-L1, thereby inhibiting the immune escape of NSCLC. The molecular mechanism may be related to the regulatory effect of miR-944/CD44 axis on PD-L1.

Key words： Non-small cell lung cancer Circular RNA CircBIRC6 miR-944 Cluster of differentiation 44 Programmed death receptor ligand 1 Immune escape

基金资助:湖北省卫生健康委科研项目,(编号:WJ2019M238)

通讯作者: 任丹

引用本文:

张田, 任丹, 李杰. circBIRC6通过miR-944/CD44轴促进PD-L1介导的非小细胞肺癌免疫逃逸[J]. 河北医学, 2022, 28(12): 1969-1977.
ZHANG Tian, REN Dan, et al. CircBIRC6 Promotes PD-L1-Mediated Immune Escape in Non-Small Cell Lung Cancer through miR-944/CD44 Axis. HeBei Med, 2022, 28(12): 1969-1977.

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http://www.hbyxzzs.cn/CN/10.3969/j.issn.1006-6233.2022.12.006 或 http://www.hbyxzzs.cn/CN/Y2022/V28/I12/1969

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