Flow cytometric analysis of intestinal intraepithelial lymphocytes in a model of immunodeficiency in Wistar rats.

Cytometry Pub Date : 2000-10-01
M G Márquez, A Galeano, S Olmos, M E Roux
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Abstract

Background: We have shown, in a rat model of immunodeficiency, permanent alterations in the thymus and in the gut-associated lymphoid tissues. We observed by immunohistochemistry an increase in the number of gamma/delta+ T cells in the gut lamina propria and in the number of CD8alpha/alpha+, CD25+, gamma/delta+ subpopulations of intestinal intraepithelial lymphocytes (iIEL). The aim of the present study was to analyze the isolated rat iIEL by flow cytometry. Materials and Methods Cells from mesenteric lymph nodes were examined in parallel with isolated iIEL. After staining with different antibodies, samples were run on a FACScan flow cytometer. Background staining was evaluated using isotype controls. Data analysis was performed using Lysys II software (Becton Dickinson) and WinMDI 2.3 software.

Results: 1) CD8alpha/beta populations do not express TCRgamma/delta, 2) CD8alpha/alpha+ populations express TCRgamma/delta, and its percentage is significantly increased in R21, 3) CD8alpha/beta and CD8alpha/alpha iIEL express TCRalpha/beta, being the percentage of CD8alpha/alpha+ TCRalpha/beta+ iIEL increased and the percentage of CD8alpha/beta+ TCRalpha/beta+ iIEL decreased in R21, and 4) CD8alpha/alpha as well as CD8alpha/beta iIEL do express CD25 only in R21.

Conclusions: Considering the above results, we conclude that there exists an "in situ" origin and extrathymic maturation of the CD8alpha/alpha+ iIEL in the intestinal epithelium. The increase of TCRgamma/delta+ T cells may be triggered by the carbohydrate dextrin, to provide immune protection and control of inflammation at the intestinal level.

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Wistar大鼠免疫缺陷模型肠上皮内淋巴细胞的流式细胞术分析。
背景:我们在大鼠免疫缺陷模型中显示,胸腺和肠道相关淋巴组织发生永久性改变。我们通过免疫组织化学观察到肠固有层中γ / δ + T细胞数量增加,肠上皮内淋巴细胞(iIEL)中cd8 α / α +、CD25+、γ / δ +亚群数量增加。本研究的目的是用流式细胞术对分离的大鼠iIEL进行分析。材料与方法肠系膜淋巴结细胞与离体iIEL平行检测。用不同抗体染色后,样品在FACScan流式细胞仪上运行。采用同型对照评价背景染色。采用Lysys II软件(Becton Dickinson)和WinMDI 2.3软件进行数据分析。结果:1)CD8alpha/beta群体不表达TCRgamma/delta, 2) CD8alpha/alpha+群体表达TCRgamma/delta,其百分比在R21中显著升高,3)CD8alpha/beta和CD8alpha/alpha iIEL表达TCRalpha/beta /beta+ iIEL百分比在R21中升高,CD8alpha/beta+ TCRalpha/beta /beta+ iIEL百分比降低,4)CD8alpha/alpha和CD8alpha/alpha /beta iIEL仅在R21中表达CD25。结论:综合以上结果,我们认为CD8alpha/alpha+ iIEL在肠上皮中存在“原位”起源和胸腺外成熟。TCRgamma/ δ + T细胞的增加可能是由碳水化合物糊精引起的,在肠道水平上提供免疫保护和控制炎症。
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