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ICAM‐1‐expressing pocket epithelium, LFA‐1‐expressing T cells in gingival tissue and gingival crevicular fluid as features characterizing inflammatory cell invasion and exudation in adult periodontitis

CD11a 白细胞介素2受体 病理 牙周炎 结缔组织 流式细胞术 外周血单个核细胞 单克隆抗体 医学 生物 化学 分子生物学 抗体 免疫学 T细胞 内科学 CD18型 体外 免疫系统 生物化学
作者
Yumi Takeuchi,Katsuya Sakurai,I. F. Ike,Hiromasa Yoshie,Keisuke Kawasaki,Kohji Hara
出处
期刊:Journal of Periodontal Research [Wiley]
卷期号:30 (6): 426-435 被引量:29
标识
DOI:10.1111/j.1600-0765.1995.tb01297.x
摘要

Activated T lymphocytes constitute a major component of inflammatory cells in the early periodontal lesion, and also appear in the gingival crevicular fluid. In an attempt to clarify the relationship between the ICAM‐1 (CD54) expression of pocket epithelium in gingiva and the infiltrating lymphocyte population, we carried out an analysis of CD11a + (LFA‐lα), CD25 + (IL‐2Rα) and CD4 + (Th) cells subjacent to ICAM‐1‐expressing pocket epithelia and CD11a + CD25 + CD4 + cells in gingival crevicular fluid (GCF). GCF was collected by crevicular washing from 16 patients with periodontitis (P group) and 3 subjects with healthy gingiva (H group). Peripheral blood (PB) was collected at the same time. Mononuclear cells were isolated by Ficoll‐paque gradient centrifugation from GCF and PB. Monoclonal antibodies (mAb) to CD11a, CD25, and CD4 were used for three‐color flow cytometry. Gingival biopsies were obtained from 7 patients in P group and 3 subjects in H group. Serial cryostat sections (6 μm in thickness) were prepared from each biopsy, on which a double staining was performed. The number of CD11a + CD25 + CD4 + cells and the fluorescence intensity of FITC conjugated anti‐CD 11a were significantly higher in GCF than in PB (p≤0.001 to p≤0.01). CD11a + CD25 + CD4 + cells were not detected in GCF in H group. The pocket epithelia expressed CD54 in P group, but not in H group. The number of CD11a + , CD25 + and CD4 + cells infiltrating the connective tissue subjacent to the upper, middle and lower parts of the CD54 positive pocket epithelium (n=16) was 141±26, 38±13, 144±29 (cells/0.04 mm 2 ), respectively, whereas in the CD54 negative pocket epithelium, it was (n=5) 9±2, 3±1, 8±3. In P group, the CD11a + CD25 + CD4 + cell number in GCF correlated with CD25 + , CD11a + cells in the connective tissue subjacent to the CD54 + pocket epithelium. These results indicate that expression of ICAM‐1 in pocket epithelium is relevant to the migration of CD11a, CD25, CD4 positive cells in connective tissue subjacent to the pocket epithelium into the periodontal pocket. Assessing the relationship of our findings and other adhesion molecules would offer important clues to the understanding of T cell migration in affected gingiva.
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