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角膜上皮细胞和基质细胞上HLA抗原表达的调节。

Modulation of HLA antigen expression on corneal epithelial and stromal cells.

作者信息

Dreizen N G, Whitsett C F, Stulting R D

机构信息

Department of Ophthalmology, Georgetown University Medical Center, Washington, DC 20007.

出版信息

Invest Ophthalmol Vis Sci. 1988 Jun;29(6):933-9.

PMID:3131265
Abstract

Human corneal epithelial cells and stromal fibroblasts in culture were incubated with gamma interferon or with medium conditioned by phytohemagglutinin (PHA)-stimulated mononuclear cells. The corneal cells were placed into suspension, assayed for class I (HLA-A,B,C) and class II (HLA-DR) antigens by indirect immunofluorescence, and analyzed with flow cytometry. Epithelial cells treated for 5 days with conditioned medium (CND-M) did not exhibit an increase in class I or an induction of class II antigen expression, although a trend toward increased class I antigen expression was present. Epithelial cells treated for 5 days with 250-500 U/ml of gamma interferon did not demonstrate an increase in class I but did show an induction of class II antigen expression; again, however, a trend toward increased class I antigen expression was present. Stromal fibroblasts treated for 3-5 days with CND-M exhibited an increase in class I antigen expression, but stromal fibroblasts treated for 1-5 days with CND-M did not show an induction of class II antigen expression. Stromal fibroblasts incubated for 1-5 days with 250-750 U/ml of gamma interferon demonstrated both an increase in class I and an induction of class II antigen expression. These data suggest that host lymphokines may intensify the process of corneal graft rejection by augmenting class I antigen expression on allogeneic cells. Moreover, the induction of class II antigen expression by host lymphokines on cells in transplanted corneal tissue may lead to host sensitization and subsequent allograft rejection.

摘要

将培养的人角膜上皮细胞和基质成纤维细胞与γ干扰素或经植物血凝素(PHA)刺激的单核细胞条件培养基一起孵育。将角膜细胞制成悬液,通过间接免疫荧光法检测I类(HLA - A、B、C)和II类(HLA - DR)抗原,并进行流式细胞术分析。用条件培养基(CND - M)处理5天的上皮细胞,I类抗原未增加,II类抗原也未诱导表达,尽管存在I类抗原表达增加的趋势。用250 - 500 U/ml的γ干扰素处理5天的上皮细胞,I类抗原未增加,但II类抗原表达有诱导;然而,同样存在I类抗原表达增加的趋势。用CND - M处理3 - 5天的基质成纤维细胞I类抗原表达增加,但用CND - M处理1 - 5天的基质成纤维细胞未显示II类抗原表达的诱导。用250 - 750 U/ml的γ干扰素孵育1 - 5天的基质成纤维细胞,I类抗原增加且II类抗原表达有诱导。这些数据表明,宿主淋巴因子可能通过增强同种异体细胞上的I类抗原表达来强化角膜移植排斥过程。此外,宿主淋巴因子在移植角膜组织细胞上诱导II类抗原表达可能导致宿主致敏及随后的同种异体移植排斥。

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