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角膜感染中固有免疫的新模型。

Novel model of innate immunity in corneal infection.

作者信息

Rajaiya Jaya, Zhou Xiaohong, Barequet Irina, Gilmore Michael S, Chodosh James

机构信息

Howe Laboratory, Massachusetts Eye and Ear Infirmary, Department of Ophthalmology, Harvard Medical School, 243 Charles Street, Boston, MA, 02114, USA.

Massachusetts Eye and Ear Infirmary, Howe Laboratory, 243 Charles Street, Boston, MA, 02114, USA.

出版信息

In Vitro Cell Dev Biol Anim. 2015 Sep;51(8):827-34. doi: 10.1007/s11626-015-9910-2. Epub 2015 May 15.

Abstract

The cornea functions as the major refractive interface for vision and protects the internal eye from insult. Current understanding of innate immune responses to corneal infection derives from a synthesis of in vitro and in vivo analyses. However, monolayer cell cultures and mouse models do not accurately duplicate all aspects of innate immunity in human patients. Here, we describe a three-dimensional culture system that incorporates human cells and extracellular matrix to more completely simulate the human cornea for studies of infection. Human corneal stromal fibroblasts were mixed with type I collagen in 3-μm pore size transwell inserts, and overlayed with Matrigel to simulate a human corneal stroma and epithelial basement membrane. These were then infected with a cornea-tropic adenovirus, and exposed on their inferior side to leukocytes derived from human peripheral blood. Subsequent analyses were performed with histology, confocal microscopy, ELISA, and fluorescence-activated cell sorting (FACS). CXCL8, a neutrophil chemokine shown previously as the first cytokine induced in infection of human corneal cells, increased upon adenovirus infection of facsimiles in a dose-responsive fashion. Myeloperoxidase-positive cells infiltrated infected corneal facsimiles in a sub-Matrigel location, possibly due to CXCL8 colocalization with heparan sulfate, a Matrigel constituent. Cellular infiltration was significantly inhibited by treatment with chemical inhibitors of p38 MAPK and Src kinase, both constituents of a signaling cascade previously suggested to regulate inflammation after adenovirus infection. FACS analysis determined that both virus and corneal fibroblasts were necessary for the induction of leukocyte migration into the facsimiles. The corneal facsimile, literally a cornea in a test tube, permits mechanistic studies on human tissue in a highly tractable system.

摘要

角膜作为视觉的主要屈光界面,保护眼内组织免受损伤。目前对角膜感染先天免疫反应的理解源于体外和体内分析的综合。然而,单层细胞培养和小鼠模型并不能准确复制人类患者先天免疫的所有方面。在此,我们描述了一种三维培养系统,该系统整合了人类细胞和细胞外基质,以更全面地模拟人类角膜用于感染研究。将人角膜基质成纤维细胞与I型胶原在孔径为3μm的Transwell小室中混合,并用基质胶覆盖以模拟人角膜基质和上皮基底膜。然后用嗜角膜腺病毒感染这些结构,并在其下侧暴露于源自人外周血的白细胞。随后进行组织学、共聚焦显微镜、ELISA和荧光激活细胞分选(FACS)分析。CXCL8是一种中性粒细胞趋化因子,先前被证明是人类角膜细胞感染时诱导产生的第一种细胞因子,在腺病毒感染仿制品后以剂量反应方式增加。髓过氧化物酶阳性细胞在基质胶下的位置浸润感染的角膜仿制品,这可能是由于CXCL8与基质胶成分硫酸乙酰肝素共定位所致。用p38丝裂原活化蛋白激酶和Src激酶的化学抑制剂处理可显著抑制细胞浸润,这两种成分都是先前认为在腺病毒感染后调节炎症的信号级联反应的组成部分。FACS分析确定病毒和角膜成纤维细胞对于诱导白细胞迁移到仿制品中都是必需的。角膜仿制品,实际上就是试管中的角膜,在一个高度易处理的系统中允许对人体组织进行机制研究。

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