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次氯酸诱导的人中性粒细胞和龈沟液胶原酶的激活可被抗坏血酸盐抑制。

Hypochlorous acid induced activation of human neutrophil and gingival crevicular fluid collagenase can be inhibited by ascorbate.

作者信息

Suomalainen K, Sorsa T, Lindy O, Saari H, Konttinen Y T, Uitto V J

机构信息

Department of Periodontology, University of Helsinki, Finland.

出版信息

Scand J Dent Res. 1991 Oct;99(5):397-405. doi: 10.1111/j.1600-0722.1991.tb01047.x.

Abstract

Interstitial collagenase either obtained from human neutrophils by phorbol myristate acetate (PMA) induced degranulation or isolated from human gingival crevicular fluid was found to be activated by addition of an oxidative agent, hypochlorous acid (HOCl). Collagenase released by PMA stimulated neutrophils was completely in latent form but underwent partial autoactivation during 16 h incubation at 22 degrees C in the presence of soy bean trypsin inhibitor. The partial autoactivation was potentiated to complete activation of released collagenase after addition of exogenous HOCl. Ascorbate prevented this activation of neutrophil collagenase. Isolated human gingival crevicular fluid collagenase represented an apparent Mr of 70 kD in completely latent form, whereas 70/54 kD enzyme species were detected for partially autoactive form of the enzyme. Western blot analysis of gingival crevicular fluid using a polyclonal antibody raised against purified human neutrophil collagenase revealed the same 70/54 kD molecular forms of the enzyme. The latent gingival crevicular fluid collagenase was also activated by HOCl and this activation could be prevented by ascorbate. Activation of the 70 kD latent collagenase by HOCl as well as by other non-proteolytic activators such as an organomercurial compound (phenylmercuric chloride) and a gold(I) compound (gold thioglucose) was not associated with detectable changes in apparent Mr, whereas trypsin activation resulted in fragmentation of 70 kD enzyme to 54 kD species. Our results provide further evidence for the neutrophil origin of gingival crevicular fluid collagenase and suggest that, in addition to proteolytic activation, oxidative and antioxidative agents seem to be able to regulate neutrophil collagenase activity.

摘要

通过佛波醇肉豆蔻酸酯乙酸酯(PMA)诱导脱颗粒从人中性粒细胞中获得的间质胶原酶,或从人龈沟液中分离出的间质胶原酶,被发现可通过添加氧化试剂次氯酸(HOCl)而激活。PMA刺激的中性粒细胞释放的胶原酶完全处于潜伏形式,但在22℃、存在大豆胰蛋白酶抑制剂的情况下孵育16小时期间会发生部分自身激活。添加外源性HOCl后,部分自身激活被增强至释放的胶原酶完全激活。抗坏血酸可阻止中性粒细胞胶原酶的这种激活。分离出的人龈沟液胶原酶以完全潜伏形式呈现出约70kD的表观分子量,而对于该酶的部分自身激活形式则检测到70/54kD的酶种类。使用针对纯化的人中性粒细胞胶原酶产生的多克隆抗体对龈沟液进行蛋白质印迹分析,揭示了该酶相同的70/54kD分子形式。潜伏的龈沟液胶原酶也可被HOCl激活,且这种激活可被抗坏血酸阻止。HOCl以及其他非蛋白水解激活剂如有机汞化合物(苯基汞氯化物)和金(I)化合物(金硫葡萄糖)对70kD潜伏胶原酶的激活与表观分子量的可检测变化无关,而胰蛋白酶激活则导致70kD酶裂解为54kD种类。我们的结果为龈沟液胶原酶的中性粒细胞来源提供了进一步证据,并表明,除了蛋白水解激活外,氧化和抗氧化剂似乎也能够调节中性粒细胞胶原酶的活性。

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