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用视紫红质合成肽诱导Lewis大鼠实验性自身免疫性葡萄膜炎

Induction of experimental autoimmune uveitis with rhodopsin synthetic peptides in Lewis rats.

作者信息

Adamus G, Schmied J L, Hargrave P A, Arendt A, Moticka E J

机构信息

Department of Ophthalmology, University of Florida, Gainesville.

出版信息

Curr Eye Res. 1992 Jul;11(7):657-67. doi: 10.3109/02713689209000739.

DOI:10.3109/02713689209000739
PMID:1521467
Abstract

Rhodopsin, a membrane protein of rod photoreceptor cells, induces an experimental autoimmune uveitis (EAU) in Lewis rats. Synthetic peptides derived from rhodopsin sequences that cover hydrophilic, exposed regions of the protein were tested for their capacity of eliciting in vitro T cell proliferation and their ability for inducing EAU in Lewis rats. Rats were injected with rhodopsin's peptides mixed in complete Freund's adjuvant containing M. tuberculosis H37Ra (5 mg/ml) three days after pretreatment with cyclophosphamide (20 mg/kg). ELISA results indicate that all peptides induce antibody responses; however antibody titers differ among sera tested. Immunization with four peptides--the amino-terminus (2-32), loop I-II (61-75), loop V-VI (230-251), and the carboxyl-terminus (324-348 and 331-342) induced both antibody and T cell responses. In all cases, the proliferative responses of cells derived from peptide-injected rats were stronger against the immunizing peptide than against native protein. Three distinct uveitogenic epitopes were identified on rhodopsin's cytoplasmic surface--within the rhodopsin carboxyl-terminus (324-348), loop I-II (61-75), and loop V-VI (230-250). Histopathologically, at the immunized doses, total destruction of the photoreceptor cell layer was observed as compared to the control group. Loop V-VI caused severe inflammation of the retina while the other pathogenic peptides produced less severe destruction with few inflammatory cells present. Our study indicates that the major immunodominant T cell epitope (331-342) is also involved in EAU induction but is not the primary uveitogenic site.

摘要

视紫红质是视杆光感受器细胞的一种膜蛋白,可在Lewis大鼠中诱发实验性自身免疫性葡萄膜炎(EAU)。对源自视紫红质序列、覆盖该蛋白亲水性暴露区域的合成肽进行了测试,以检测其体外诱导T细胞增殖的能力以及在Lewis大鼠中诱导EAU的能力。在用环磷酰胺(20mg/kg)预处理三天后,给大鼠注射与含有结核分枝杆菌H37Ra(5mg/ml)的完全弗氏佐剂混合的视紫红质肽。ELISA结果表明,所有肽均能诱导抗体反应;然而,所检测血清中的抗体滴度有所不同。用四种肽进行免疫——氨基末端(2-32)、环I-II(61-75)、环V-VI(230-251)以及羧基末端(324-348和331-342),可诱导抗体和T细胞反应。在所有情况下,源自注射肽的大鼠的细胞对免疫肽的增殖反应比对天然蛋白的反应更强。在视紫红质的细胞质表面鉴定出三个不同的葡萄膜炎原性表位——在视紫红质羧基末端(324-348)、环I-II(61-75)和环V-VI(230-250)内。组织病理学检查显示,与对照组相比,在免疫剂量下观察到光感受器细胞层完全破坏。环V-VI导致视网膜严重炎症,而其他致病肽造成的破坏较轻,炎症细胞较少。我们的研究表明,主要的免疫显性T细胞表位(331-342)也参与EAU的诱导,但不是主要的葡萄膜炎原性位点。

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