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正常人类肾脏中表达HLA - DR的肾微血管内皮细胞:MHC II类分子表达的特征、分离及调控

Normal human kidney HLA-DR-expressing renal microvascular endothelial cells: characterization, isolation, and regulation of MHC class II expression.

作者信息

Muczynski Kimberly A, Ekle David M, Coder David M, Anderson Susan K

机构信息

Department of Medicine, University of Washington, Seattle, WA 98195, USA.

出版信息

J Am Soc Nephrol. 2003 May;14(5):1336-48. doi: 10.1097/01.asn.0000061778.08085.9f.

Abstract

Human, but not murine, renal peritubular and glomerular capillaries constitutively express class II major histocompatibility (MHC) proteins at high levels in normal human kidney. Expression of class II proteins on renal microvascular endothelial cells (RMEC) makes it available to circulating lymphocytes and imparts a surveillance capacity to RMEC for controlling inflammatory responses. In this report, the co-expression of HLA-DR and the endothelial marker CD31 are used to identify RMEC as a distinct population of cells within a standard renal biopsy using flow cytometry. A three-laser, multicolor flow cytometry analysis using Alexa dyes, developed for characterizing the expression of cell surface antigens, identifies RMEC as a population separate from HLA-DR-expressing leukocytes. HLA-DR RMEC co-express HLA-DP and HLA-DQ. RMEC also express the T cell costimulatory factor CD58 but not CD80, CD86, or CD40. On the basis of high HLA-DR expression, RMEC are isolated for culture using fluorescence-activated cell sorting and magnetic beads. Cultured RMEC require normal basal physiologic concentrations of gamma interferon (gammaIFN) to maintain HLA protein expression. This expression is regulated by CIITA, the MHC class II-specific transcription factor. Four tissue-specific promoters have been described for CIITA. In freshly isolated RMEC, RT-PCR and hybridization using specific oligonucleotide probes to CIITA promoter sequences identify only the statin-sensitive gammaIFN-induced promoter IV of CIITA. Therefore, the constitutive expression of HLA-DR on RMEC in normal human kidney is located in a position for immune surveillance, depends on basal physiologic concentrations of gammaIFN, and may be amenable to regulation with statins.

摘要

在正常人类肾脏中,人而非小鼠的肾周小管和肾小球毛细血管组成性地高水平表达II类主要组织相容性(MHC)蛋白。肾微血管内皮细胞(RMEC)上II类蛋白的表达使其能够与循环淋巴细胞相互作用,并赋予RMEC控制炎症反应的监测能力。在本报告中,使用流式细胞术,通过HLA-DR与内皮标志物CD31的共表达,将RMEC鉴定为标准肾活检中一个独特的细胞群体。一种使用Alexa染料开发的三激光多色流式细胞术分析方法,用于表征细胞表面抗原的表达,可将RMEC鉴定为一个与表达HLA-DR的白细胞不同的群体。表达HLA-DR的RMEC共表达HLA-DP和HLA-DQ。RMEC还表达T细胞共刺激因子CD58,但不表达CD80、CD86或CD40。基于高HLA-DR表达,使用荧光激活细胞分选和磁珠分离RMEC用于培养。培养的RMEC需要正常基础生理浓度的γ干扰素(γIFN)来维持HLA蛋白表达。这种表达受MHC II类特异性转录因子CIITA调控。已描述了CIITA的四个组织特异性启动子。在新鲜分离的RMEC中,使用针对CIITA启动子序列的特异性寡核苷酸探针进行RT-PCR和杂交,仅鉴定出CIITA的他汀类药物敏感的γIFN诱导启动子IV。因此,正常人类肾脏中RMEC上HLA-DR的组成性表达处于免疫监测位置,依赖于γIFN的基础生理浓度,并且可能适合用他汀类药物进行调控。

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