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单核细胞尿激酶表达:白细胞介素的调节作用

Monocyte urokinase expression: modulation by interleukins.

作者信息

Gyetko M R, Wilkinson C C, Sitrin R G

机构信息

Pulmonary Section, Department of Veterans Affairs Medical Center, Ann Arbor, MI.

出版信息

J Leukoc Biol. 1993 May;53(5):598-601. doi: 10.1002/jlb.53.5.598.

DOI:10.1002/jlb.53.5.598
PMID:8501398
Abstract

This study delineates the regulatory effect of interleukin-1 (IL-1) and interleukin-2 (IL-2) on monocyte plasminogen activator (PA) activity. Mononuclear phagocytes regulate net PA activity by modulating the expression of urokinase-type PA (uPA) and a specific plasminogen activator inhibitor, PAI-2. To understand the regulation of mononuclear phagocyte PA activity, it is important to compare the expression of uPA and PAI-2. In this study, we determined the relative abundance of secreted PA and PA inhibitor activity in human monocyte-conditioned medium after stimulation with human recombinant IL-1 or IL-2. In agreement with our previous description of tumor necrosis factor-alpha and interferon-gamma stimulation of mononuclear phagocytes, we found no detectable PA activity in conditioned medium. Both IL-1 and IL-2 had dose-dependent effects, significantly up-regulating PA inhibitor activity in monocyte-conditioned medium (up to 11-fold). To further investigate the mechanism underlying this effect, Northern blot analysis was done to measure steady-state mRNA for uPA and PAI-2. Consistent with the increase in secreted PA inhibitor activity, we found that both IL-1 and IL-2 significantly increased steady-state mRNA for PAI-2. In addition, however, both IL-1 and IL-2 increased steady-state mRNA for uPA. IL-1 appears to increase mRNA for uPA to a greater extent than does IL-2. We conclude that IL-1 and IL-2 modulate monocyte proteolytic activity by increasing expression of uPA and PAI-2 with a resultant predominance of PAI-2. We further conclude that cytokine-specific regulation of plasminogen activity is achieved partly by varying the proportionate expression of uPA and PAI-2.

摘要

本研究阐述了白细胞介素 -1(IL -1)和白细胞介素 -2(IL -2)对单核细胞纤溶酶原激活物(PA)活性的调节作用。单核吞噬细胞通过调节尿激酶型 PA(uPA)和一种特异性纤溶酶原激活物抑制剂PAI -2的表达来调节净PA活性。为了解单核吞噬细胞PA活性的调节机制,比较uPA和PAI -2的表达情况很重要。在本研究中,我们测定了用人重组IL -1或IL -2刺激后人单核细胞条件培养基中分泌的PA和PA抑制剂活性的相对丰度。与我们之前对肿瘤坏死因子 -α和干扰素 -γ刺激单核吞噬细胞的描述一致,我们在条件培养基中未检测到可检测的PA活性。IL -1和IL -2均有剂量依赖性作用,显著上调单核细胞条件培养基中的PA抑制剂活性(高达11倍)。为进一步研究这种作用的潜在机制,进行了Northern印迹分析以测量uPA和PAI -2的稳态mRNA。与分泌的PA抑制剂活性增加一致,我们发现IL -1和IL -2均显著增加了PAI -2的稳态mRNA。然而,此外,IL -1和IL -2均增加了uPA的稳态mRNA。IL -1似乎比IL -2在更大程度上增加uPA的mRNA。我们得出结论,IL -1和IL -2通过增加uPA和PAI -2的表达来调节单核细胞的蛋白水解活性,结果PAI -2占优势。我们进一步得出结论,纤溶酶原活性细胞因子特异性调节部分是通过改变uPA和PAI -2的相对表达比例来实现的。

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