循环基质金属蛋白酶9的浓度与双链DNA自身免疫抗体成反比:对监测系统性红斑狼疮疾病活动的意义。

G S Makowski, M L Ramsby
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引用次数: 0

摘要

目的:比较循环基质金属蛋白酶(MMP)浓度与单链和双链DNA(ssDNA和dsDNA)抗体,以确定它们在系统性红斑狼疮(SLE)等炎症性关节炎疾病中的关系:成纤维细胞 MMP-2 和中性粒细胞 MMP-9 通过明胶酶谱分析,并用密度计测量。用酶联免疫法测定抗ssDNA和抗dsDNA,并根据抗体含量将样本分组如下:低抗ssDNA/低抗dsDNA抗体(第1组);高抗ssDNA/低抗dsDNA抗体(第2组);高抗ssDNA/高抗dsDNA抗体(第3组):结果:第3组样本中的MMP-9含量明显低于第1组样本。高分子量的 MMP-9 形态(130 和 225 kDa)几乎不存在。第 2 组样本含有中等浓度的 MMP-9。成纤维细胞 MMP-2 在所有组别中均无变化。补体C3和C4的平均浓度随着抗ssDNA和抗dsDNA抗体的增加而持续下降,但下降幅度不一。所有患者组的平均红细胞沉降率均升高:中性粒细胞MMP-9是一种炎症标志物,与抗dsDNA抗体成反比,而抗dsDNA抗体是系统性红斑狼疮的特异性标志物。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Concentrations of circulating matrix metalloproteinase 9 inversely correlate with autoimmune antibodies to double stranded DNA: implications for monitoring disease activity in systemic lupus erythematosus.

Aims: To compare circulating matrix metalloproteinase (MMP) concentrations with antibodies to single and double stranded DNA (ssDNA and dsDNA) to determine their relation in inflammatory arthritic diseases, such as systemic lupus erythematosus (SLE).

Methods: Fibroblast MMP-2 and neutrophil MMP-9 were resolved by gelatin zymography and measured by densitometry. Anti-ssDNA and anti-dsDNA were determined by enzyme immunoassay and samples grouped on antibody content as follows: low anti-ssDNA/low anti-dsDNA antibodies (group 1); high anti-ssDNA/low anti-dsDNA antibodies (group 2); and high anti-ssDNA/high anti-dsDNA antibodies (group 3).

Results: Group 3 samples contained significantly lower amounts of MMP-9 when compared with group 1 samples. Higher molecular weight MMP-9 forms (130 and 225 kDa) were virtually absent. Group 2 samples contained intermediate MMP-9 concentrations. Fibroblast MMP-2 was unchanged in all groups. Mean complement C3 and C4 concentrations showed a consistent, but variably significant, decrease with increasing anti-ssDNA and anti-dsDNA antibodies. The mean erythrocyte sedimentation rate was raised in all patient groups.

Conclusions: Neutrophil MMP-9, an inflammatory marker, inversely correlates with anti-dsDNA antibodies, which are a specific marker for SLE, and may be important in monitoring disease activity during antibody deposition in tissues.

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