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BB大鼠糖尿病发病前后胰岛免疫细胞的定量表型和功能分析。

Quantitative phenotypic and functional analyses of islet immune cells before and after diabetes onset in the BB rat.

作者信息

Hosszufalusi N, Chan E, Teruya M, Takei S, Granger G, Charles M A

机构信息

Diabetes Research Program, University of California, Irvine.

出版信息

Diabetologia. 1993 Nov;36(11):1146-54. doi: 10.1007/BF00401059.

DOI:10.1007/BF00401059
PMID:8270129
Abstract

Inflammatory cells invading islets are thought to be mediators of islet destruction in spontaneous autoimmune diabetes mellitus. Thus methods were developed to isolate and characterize in situ islet inflammatory cells from 75-95-day-old prediabetic and diabetic BB rats. Islet inflammatory cells were structurally examined using single- and double-colour flow cytometry. Functional studies consisted of cytolytic assays using normal rat islet target cells and in situ islet or spleen effector cells. Structural data reveal natural killer cells to be the major cell population (70%) of total immune cells present in inflamed islets during prediabetes. At diabetes onset, the natural killer cell population remained at a high level (47%), but an increasing population of T cells (40%) was noted also. Analyses of T-cell subsets before and after diabetes onset revealed CD4+ T cells as predominant (50-55% of total T cells) with double-negative (CD4-CD8-) T cells (25-30%) and CD8+ T cells (15-20%) also present in significant quantities. Activated T cells accounted only for a minority of T cells (< 3%). Functional studies indicate that in situ islet-derived cytolytic effector cells are more potent killers (ten-fold) of normal islet target cells than are splenic effector cells. These data suggest that in situ islet inflammatory cells (a) can be quantitatively studied both structurally and functionally; (b) express structural phenotypes differing substantially from splenic mononuclear cell populations; (c) are considerably more cytolytic than splenic effectors; and (d) should prove informative in determining the most significant autoimmune functional events prior to and during islet beta-cell destruction.

摘要

浸润胰岛的炎症细胞被认为是自发性自身免疫性糖尿病中胰岛破坏的介质。因此,人们开发了一些方法来从75至95日龄的糖尿病前期和糖尿病BB大鼠中分离并鉴定原位胰岛炎症细胞。使用单双色流式细胞术对胰岛炎症细胞进行结构检查。功能研究包括使用正常大鼠胰岛靶细胞以及原位胰岛或脾脏效应细胞进行的细胞溶解试验。结构数据显示,自然杀伤细胞是糖尿病前期炎症胰岛中存在的总免疫细胞的主要细胞群体(70%)。在糖尿病发病时,自然杀伤细胞群体仍处于较高水平(47%),但也注意到T细胞群体在增加(40%)。对糖尿病发病前后T细胞亚群的分析显示,CD4+T细胞占主导地位(占总T细胞的50 - 55%),双阴性(CD4-CD8-)T细胞(25 - 30%)和CD8+T细胞(15 - 20%)也大量存在。活化的T细胞仅占T细胞的少数(<3%)。功能研究表明,原位胰岛来源的细胞溶解效应细胞对正常胰岛靶细胞的杀伤能力(强十倍)比脾脏效应细胞更强。这些数据表明,原位胰岛炎症细胞(a)可以在结构和功能上进行定量研究;(b)表达的结构表型与脾脏单核细胞群体有很大不同;(c)比脾脏效应细胞的细胞溶解能力强得多;(d)在确定胰岛β细胞破坏之前和期间最重要的自身免疫功能事件方面应该会提供有价值的信息。

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本文引用的文献

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Pancreatic islet function in nondiabetic and diabetic BB rats.非糖尿病和糖尿病BB大鼠的胰岛功能
Diabetes. 1993 Sep;42(9):1310-7. doi: 10.2337/diab.42.9.1310.
2
Immune islet killing mechanisms associated with insulin-dependent diabetes: three rabbit antibody-mediated islet cell cytotoxicity models.与胰岛素依赖型糖尿病相关的免疫胰岛杀伤机制:三种兔抗体介导的胰岛细胞细胞毒性模型。
Diabetologia. 1983 Oct;25(4):348-54. doi: 10.1007/BF00253200.
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Mechanisms of rat pancreatic islet allograft rejection.大鼠胰岛同种异体移植排斥反应的机制。
Diabetes Res. 1984 Jul;1(2):95-103.
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Pre-diabetes in the spontaneously diabetic BB/E rat: lymphocyte subpopulations in the pancreatic infiltrate and expression of rat MHC class II molecules in endocrine cells.
Diabetologia. 1985 Jul;28(7):464-6. doi: 10.1007/BF00280892.
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Spontaneous diabetes mellitus in the Bio-Breeding/Worcester rat. Evidence in vitro for natural killer cell lysis of islet cells.Bio-Breeding/Worcester大鼠的自发性糖尿病。胰岛细胞自然杀伤细胞裂解的体外证据。
J Clin Invest. 1986 Mar;77(3):916-24. doi: 10.1172/JCI112390.
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Preferential infiltration of macrophages during early stages of insulitis in diabetes-prone BB rats.在易患糖尿病的BB大鼠胰岛炎早期巨噬细胞的优先浸润。
Diabetes. 1988 Aug;37(8):1053-8. doi: 10.2337/diab.37.8.1053.
7
Identification of T cell subsets and class I and class II antigen expression in islet grafts and pancreatic islets of diabetic BioBreeding/Worcester rats.糖尿病BioBreeding/Worcester大鼠胰岛移植和胰岛中T细胞亚群及I类和II类抗原表达的鉴定
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8
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Diabetes. 1988 Sep;37(9):1301-4. doi: 10.2337/diab.37.9.1301.
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