对晶状体中转基因表达的外来抗原的免疫耐受。

Immunotolerance against a foreign antigen transgenically expressed in the lens.

作者信息

Lai J C, Fukushima A, Wawrousek E F, Lobanoff M C, Charukamnoetkanok P, Smith-Gill S J, Vistica B P, Lee R S, Egwuagu C E, Whitcup S M, Gery I

机构信息

National Eye Institute, National Institutes of Health, and the Howard Hughes Medical Institute-NIH Research Scholars Program, Bethesda, Maryland 20892-1857, USA.

出版信息

Invest Ophthalmol Vis Sci. 1998 Oct;39(11):2049-57.

PMID:9761283

Abstract

PURPOSE

To extend our knowledge concerning immunotolerance against autologous lens crystallins, transgenic (Tg) mice that express a foreign antigen in their lens were generated, and the immune response against the antigen in these mice was analyzed.

METHODS

Conventional techniques were used to generate lines of Tg mice that express soluble (S-) or membrane-bound (M-) hen egg lysozyme (HEL) under the control of the alphaA-crystallin promoter. The presence of HEL in various organs was determined by the particle concentration fluorescence immunoassay (PCFIA), and reverse transcription-polymerase chain reaction technique was used to detect mRNA transcripts of the molecule. To examine the development of immunity (or tolerance), Tg mice and their wild-type controls were immunized with HEL (25 microg) in Freund's complete adjuvant and 14 days later were tested for immune response against the antigen. Cellular immunity was measured by the lymphocyte proliferation assay and cytokine production, and humoral immunity was determined by enzyme-linked immunosorbent assay.

RESULTS

Eyes of the high copy number M-HEL Tg mice were dystrophic, with disrupted lens, whereas no morphologic changes were detected in the eyes of the other Tg mouse lines. All Tg mice exhibited tolerance to HEL by their cellular and humoral immune compartments. The state of immunotolerance to HEL was retained in the Tg mice for as long as 10 months after removal of the main depot of this protein, by enucleation. Measurable amounts of HEL were found in the eyes of all Tg mice, but the protein could not be detected in the serum or in other organs by the sensitive PCFIA (with a threshold of 1 ng/ml). Yet, HEL mRNA was found in the thymus of the Tg mice, suggesting that minute amounts of the protein are expressed in this organ.

CONCLUSIONS

The unresponsiveness to HEL in the Tg mice seems to be due to a "central" mechanism of tolerance, mediated by a minuscule amount of HEL in the thymus. Conversely, the much larger amounts of HEL in the peripheral depot, the eyes, play a minor role if any in the tolerogenic process. It is further proposed that a similar mechanism of central tolerance is responsible for the immunotolerance against autologous lens crystallins.

摘要

目的

为了拓展我们关于针对自体晶状体蛋白的免疫耐受的知识，构建了在晶状体中表达外源抗原的转基因（Tg）小鼠，并分析了这些小鼠针对该抗原的免疫反应。

方法

采用常规技术构建在αA - 晶状体蛋白启动子控制下表达可溶性（S - ）或膜结合（M - ）鸡卵溶菌酶（HEL）的Tg小鼠品系。通过颗粒浓度荧光免疫测定法（PCFIA）测定各器官中HEL的存在情况，并使用逆转录 - 聚合酶链反应技术检测该分子的mRNA转录本。为了检测免疫（或耐受）的发展情况，用弗氏完全佐剂中的HEL（25微克）免疫Tg小鼠及其野生型对照，14天后检测它们针对该抗原的免疫反应。通过淋巴细胞增殖试验和细胞因子产生来测量细胞免疫，通过酶联免疫吸附测定来测定体液免疫。

结果

高拷贝数M - HEL Tg小鼠的眼睛营养不良，晶状体受损，而其他Tg小鼠品系的眼睛未检测到形态学变化。所有Tg小鼠在细胞和体液免疫方面均表现出对HEL的耐受。在摘除该蛋白的主要储存部位（眼球摘除）后，Tg小鼠对HEL的免疫耐受状态持续长达10个月。在所有Tg小鼠的眼睛中都发现了可测量的HEL量，但通过敏感的PCFIA（检测阈值为1纳克/毫升）在血清或其他器官中未检测到该蛋白。然而，在Tg小鼠的胸腺中发现了HEL mRNA，表明该器官中表达了微量的该蛋白。