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Tollip基因单核苷酸多态性rs5743899调节人呼吸道上皮细胞对鼻病毒感染的反应。

Tollip SNP rs5743899 modulates human airway epithelial responses to rhinovirus infection.

作者信息

Huang C, Jiang D, Francisco D, Berman R, Wu Q, Ledford J G, Moore C M, Ito Y, Stevenson C, Munson D, Li L, Kraft M, Chu H W

机构信息

Department of Medicine, National Jewish Health, Denver, CO, USA.

Department of Medicine, University of Arizona College of Medicine, Tucson, AZ, USA.

出版信息

Clin Exp Allergy. 2016 Dec;46(12):1549-1563. doi: 10.1111/cea.12793. Epub 2016 Sep 21.

Abstract

BACKGROUND

Rhinovirus (RV) infection in asthma induces varying degrees of airway inflammation (e.g. neutrophils), but the underlying mechanisms remain unclear.

OBJECTIVE

The major goal was to determine the role of genetic variation [e.g. single nucleotide polymorphisms (SNPs)] of Toll-interacting protein (Tollip) in airway epithelial responses to RV in a type 2 cytokine milieu.

METHODS

DNA from blood of asthmatic and normal subjects was genotyped for Tollip SNP rs5743899 AA, AG and GG genotypes. Human tracheobronchial epithelial (HTBE) cells from donors without lung disease were cultured to determine pro-inflammatory and antiviral responses to IL-13 and RV16. Tollip knockout and wild-type mice were challenged with house dust mite (HDM) and infected with RV1B to determine lung inflammation and antiviral response.

RESULTS

Asthmatic subjects carrying the AG or GG genotype (AG/GG) compared with the AA genotype demonstrated greater airflow limitation. HTBE cells with AG/GG expressed less Tollip. Upon IL-13 and RV16 treatment, cells with AG/GG (vs. AA) produced more IL-8 and expressed less antiviral genes, which was coupled with increased NF-κB activity and decreased expression of LC3, a hallmark of the autophagic pathway. Tollip co-localized and interacted with LC3. Inhibition of autophagy decreased antiviral genes in IL-13- and RV16-treated cells. Upon HDM and RV1B, Tollip knockout (vs. wild-type) mice demonstrated higher levels of lung neutrophilic inflammation and viral load, but lower levels of antiviral gene expression.

CONCLUSIONS AND CLINICAL RELEVANCE

Our data suggest that Tollip SNP rs5743899 may predict varying airway response to RV infection in asthma.

摘要

背景

哮喘患者感染鼻病毒(RV)会引发不同程度的气道炎症(如中性粒细胞炎症),但其潜在机制尚不清楚。

目的

主要目的是确定Toll相互作用蛋白(Tollip)的基因变异[如单核苷酸多态性(SNP)]在2型细胞因子环境中气道上皮对RV反应中的作用。

方法

对哮喘患者和正常受试者血液中的DNA进行基因分型,确定Tollip SNP rs5743899的AA、AG和GG基因型。培养无肺部疾病供体的人气管支气管上皮(HTBE)细胞,以确定其对IL-13和RV16的促炎和抗病毒反应。用屋尘螨(HDM)攻击Tollip基因敲除小鼠和野生型小鼠,并感染RV1B,以确定肺部炎症和抗病毒反应。

结果

与AA基因型相比,携带AG或GG基因型(AG/GG)的哮喘患者气流受限更明显。AG/GG基因型的HTBE细胞表达的Tollip较少。在IL-13和RV16处理后,AG/GG基因型细胞(与AA基因型相比)产生更多的IL-8,抗病毒基因表达减少,同时NF-κB活性增加,自噬途径标志蛋白LC3的表达降低。Tollip与LC3共定位并相互作用。抑制自噬会降低IL-13和RV16处理细胞中的抗病毒基因表达。在用HDM和RV1B攻击后,Tollip基因敲除小鼠(与野生型相比)肺部中性粒细胞炎症水平和病毒载量更高,但抗病毒基因表达水平更低。

结论及临床意义

我们的数据表明,Tollip SNP rs5743899可能预测哮喘患者对RV感染的不同气道反应。

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