检验医学 ›› 2022, Vol. 37 ›› Issue (2): 177-182.DOI: 10.3969/j.issn.1673-8640.2022.02.017

• 基础研究·论著 • 上一篇    下一篇

RSV感染气液相界面培养人支气管上皮细胞模型的建立及其对HMGB1和pMLKL表达的影响

王娟, 廖焕金, 李延宁, 戈伊芹, 李佳()   

  1. 上海交通大学附属第一人民医院检验医学中心,上海 200080
  • 收稿日期:2020-12-30 修回日期:2021-05-22 出版日期:2022-02-28 发布日期:2022-03-15
  • 通讯作者: 李佳
  • 作者简介:李 佳,E-mail: 1124lijia@163.com
    王 娟,女,1985年生,硕士,主管技师,主要从事哮喘和呼吸道免疫相关研究。
  • 基金资助:
    国家自然科学基金项目(81971509);国家自然科学基金项目(81871267);上海市“医苑新星”青年医学人才培养资助计划-临床检验项目(HWJRS201972)

RSV infection of air-liquid interface cultured human bronchial epithelial cell and its effect on HMGB1 and pMLKL expressions

WANG Juan, LIAO Huanjin, LI Yanning, GE Yiqin, LI Jia()   

  1. Department of Clinical Laboratory,Shanghai General Hospital,Shanghai Jiao Tong University School of Medicine,Shanghai 200080,China
  • Received:2020-12-30 Revised:2021-05-22 Online:2022-02-28 Published:2022-03-15
  • Contact: LI Jia

摘要:

目的 构建呼吸道合胞病毒(RSV)感染气液相界面(ALI)培养的人支气管上皮细胞(hBEC)模型,为深入研究呼吸道病毒致病机制提供更接近体内环境的细胞模型;通过分析RSV感染对高迁移率族蛋白1(HMGB1)和磷酸化混合系列蛋白激酶样结构域(pMLKL)表达的影响,探讨RSV感染损伤支气管上皮的致病机制。方法 将hBEC接种到Transwell膜上,进行液体浸没式培养,细胞汇合度达100%后转ALI培养,倒置显微镜观察细胞生长状态。细胞分化成熟后按照以下分组分别感染RSV病毒:6 h对照组,6 h感染复数(MOI)1.0组,6 h MOI 3.0组,24 h对照组,24 h MOI 1.0组,24 h MOI 3.0组。每组3个复孔。通过免疫荧光染色确认RSV感染效果和RSV感染对细胞核蛋白HMGB1和pMLKL表达的影响。结果 经细胞扩展期液体浸没式培养4~10 d后,细胞汇合度达100%。转ALI培养约4周后,细胞条索状分布越来越清晰,且分泌肉眼可见的黏液,形成黏液层,将Transwell膜石蜡包埋切片,得到典型的假复层上皮HE染色结果。经抗RSV抗体免疫荧光染色确认,MOI为3.0感染24 h RSV病毒成功感染细胞;抗HMGB1和抗pMLKL免疫荧光双染色结果显示,该感染条件下,细胞核内出现粉色荧光[为蓝色4',6-二脒基-2-苯基吲哚(DAPI)和红色HMGB1荧光Merge结果],证实RSV感染后出现HMGB1核表达;而RSV感染前后均未见pMLKL表达。结论 通过在Transwell膜上液体浸没式扩展培养和ALI分化培养,可获得分化良好的hBEC,且能较长时间维持其形态及功能,可为呼吸道病毒感染及其他常见呼吸道疾病研究提供更接近体内环境的细胞模型。在MOI 3.0 24 h条件下,RSV成功感染该细胞模型,并引起损伤相关分子蛋白HMGB1核表达。

关键词: 人支气管上皮细胞, 气液相界面培养, 呼吸道合胞病毒, 高迁移率族蛋白1, 磷酸化混合系列蛋白激酶样结构域

Abstract:

Objective To construct a respiratory syncytial virus(RSV) infected the model of air-liquid interface(ALI)cultured human bronchial epithelial cells(hBEC),and to provide a cell model closer to the in vivo environment for further study of respiratory virus pathogenesis. By analyzing the effect of RSV infection on the expressions of high mobility group box protein 1(HMGB1) and phosphorylated mixed-lineage kinase domain-like protein(pMLKL),to investigate the injury pathogenesis caused by RSV. Methods The hBEC was inoculated on Transwell membrane and cultured unsubmerged mode. After the confluence of 100%,cells were transferred to ALI culture. After the cells were differentiated and matured,they were infected respectively with RSV according to the following groups:6 h control group,6 h MOI 1.0 group,6 h MOI 3.0 group,24 h control group,24 h MOI 1.0 group,24 h MOI 3.0 group,each group with 3 repeated holes. The effect of RSV infection on the expressions of HMGB1 and pMLKL was confirmed by immunofluorescence staining. Results After 4-10 d of submerged culture,the cell confluence reached 100%. Then,cells were transferred to ALI interface culture. After about 4 weeks,the distribution of cell bands became clearer,and visible mucus was secreted to form a mucus layer. HE staining showed typical pseudostratified epithelium,and immunofluorescence staining showed that RSV successfully infected cells at MOI 3.0 24 h. Anti-HMGB1 and anti-pMLKL immunofluorescence staining showed that under the condition of infection,there was pink fluorescence in the nucleus [blue 4',6-diamidino-2-phenylindole(DAPI)and red HMGB1 fluorescence merged results],which confirmed the expression of HMGB1 after RSV infection. However,there was no pMLKL expression neither before nor after RSV infection. Conclusions The well-differentiated hBEC can be obtained by submerged and ALI culture,which maintain cell morphology and function for a long time,and provide a cell model for respiratory virus infection and other common respiratory disease studies. At MOI 3.0 24 h,RSV successfully infects the cell model and causes the expression of HMGB1.

Key words: Human bronchial epithelial cell, Air-liquid interface culture, Respiratory syncytial virus, High mobility group box protein 1, Phosphorylated mixed-lineage kinase domain-like protein

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