Perlman H, Liu H, Georganas C, Koch A E, Shamiyeh E, Haines G K, Pope R M
Northwestern University Medical School and the Veterans Administration Chicago Healthcare System, Lakeside Division, IL 60611, USA.
Arthritis Rheum. 2001 Dec;44(12):2899-908. doi: 10.1002/1529-0131(200112)44:12<2899::aid-art478>3.0.co;2-x.
To examine the relationship between apoptosis and the expression of antiapoptotic proteins in the pathogenesis of experimental inflammatory arthritis.
Clinical and histologic assessment of adjuvant-induced arthritis (AIA) was performed over a 42-day period. The induction of apoptosis was measured by TUNEL analysis, and the antiapoptotic proteins, Bcl-2 and FLIP, were examined by immunohistochemistry with the use of monospecific antibodies. The percentage of Bcl-2- and FLIP-positive cells was correlated with histologic markers of AIA.
Arthritis developed by day 14 following adjuvant injection. Few TUNEL-positive cells were observed between days 0 and 21, indicating that apoptosis did not occur at these time points. An increase in the number of TUNEL-positive cells was observed at day 28, particularly outside sites of cartilage or bone erosion, which dramatically declined by day 35. Immunohistochemical analyses of Bcl-2 and FLIP revealed that the synovium was positive for Bcl-2 and FLIP on day 0. On day 14, Bcl-2 was present at the sites of early erosions and correlated with the erosion and inflammation scores. FLIP was also highly expressed at sites of erosion and was localized to the pannus starting on day 21. Although TUNEL positivity peaked at day 28, a time point in which Bcl-2 and FLIP were present, the areas that displayed intense positivity for expression of Bcl-2 and FLIP were TUNEL negative. In addition, the number of neutrophils in the synovial lining and pannus significantly decreased from day 28 to day 35, suggesting that the cells undergoing apoptosis were neutrophils. Furthermore, at day 42 when TUNEL-positive cells were absent, Bcl-2 expression was diminished, while FLIP remained highly expressed in the pannus.
The overall percentage of TUNEL-positive cells in the ankle was <1% except on days 28 and 35 post-adjuvant injection, suggesting that in AIA, similar to rheumatoid arthritis, a lack of apoptosis may contribute to disease progression. Furthermore, Bcl-2 and FLIP are temporally and differentially expressed during the pathogenesis of AIA. Inhibition of these molecules may augment synovial apoptosis and ameliorate the disease.
研究实验性炎性关节炎发病机制中细胞凋亡与抗凋亡蛋白表达之间的关系。
在42天的时间内对佐剂诱导的关节炎(AIA)进行临床和组织学评估。通过TUNEL分析检测细胞凋亡的诱导情况,使用单特异性抗体通过免疫组织化学检测抗凋亡蛋白Bcl-2和FLIP。Bcl-2和FLIP阳性细胞的百分比与AIA的组织学标志物相关。
佐剂注射后第14天出现关节炎。在第0天至第21天期间观察到很少有TUNEL阳性细胞,表明在这些时间点未发生细胞凋亡。在第28天观察到TUNEL阳性细胞数量增加,特别是在软骨或骨侵蚀部位之外,到第35天显著下降。对Bcl-2和FLIP的免疫组织化学分析显示,滑膜在第0天对Bcl-2和FLIP呈阳性。在第14天,Bcl-2存在于早期侵蚀部位,并与侵蚀和炎症评分相关。FLIP在侵蚀部位也高度表达,并从第21天开始定位于血管翳。尽管TUNEL阳性在第28天达到峰值,此时Bcl-2和FLIP均存在,但显示Bcl-2和FLIP表达强烈阳性的区域TUNEL呈阴性。此外,滑膜衬里和血管翳中的中性粒细胞数量从第28天到第35天显著减少,表明发生凋亡的细胞是中性粒细胞。此外,在第42天,当没有TUNEL阳性细胞时,Bcl-2表达减少,而FLIP在血管翳中仍高度表达。
除佐剂注射后第28天和第35天外,踝关节中TUNEL阳性细胞的总体百分比<1%,这表明在AIA中,与类风湿关节炎类似,细胞凋亡缺乏可能导致疾病进展。此外,Bcl-2和FLIP在AIA发病机制中存在时间和差异表达。抑制这些分子可能会增加滑膜细胞凋亡并改善疾病。
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