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海笋发光法主要检测活化的人类中性粒细胞释放的超氧阴离子。

Pholasin chemiluminescence detects mostly superoxide anion released from activated human neutrophils.

作者信息

Müller T, Davies E V, Campbell A K

机构信息

Department of Medical Biochemistry, University of Wales College of Medicine, Heath Park, Cardiff, UK.

出版信息

J Biolumin Chemilumin. 1989 Jul-Sep;3(3):105-13. doi: 10.1002/bio.1170030304.

DOI:10.1002/bio.1170030304
PMID:2551131
Abstract

The bioluminescent oxygen metabolite indicator protein pholasin was characterized with respect to the type and location of reactive oxygen metabolites detected in suspensions of stimulated human neutrophils. Whereas pholasin detected reactive oxygen metabolites from neutrophil suspensions stimulated with soluble agents, particulate stimulants were apparently not effective triggering agents for pholasin-dependent neutrophil chemiluminescence. Neutrophils stimulated with fMet-Leu-Phe (1 to 100 nmol/l) showed maximum pholasin-dependent chemiluminescence 45 to 60 s after stimulation. The time of maximum chemiluminescence was virtually independent of fMet-Leu-Phe concentration. In contrast, the time to reach maximum light emission increased from 60 s with 100 nmol/l phorbol ester to 295 s with 1 nmol/l phorbol ester. Significant inhibition of stimulated chemiluminescence was caused by both superoxide dismutase (20 micrograms/ml, 80% inhibition) and reduction of the oxygen concentration in the incubation medium to less than 0.5 mumol/l (95% inhibition). In contrast, the myeloperoxidase inhibitor sodium azide (0.1 mmol/l) afforded only 50% inhibition of the pholasin-dependent neutrophil chemiluminescence. Our results show that pholasin detects superoxide radicals released from cells stimulated by soluble stimulants but not intracellular oxidative activity elicited by particulate stimulants.

摘要

对生物发光氧代谢物指示剂蛋白磷光蛋白进行了表征,涉及在受刺激的人中性粒细胞悬液中检测到的活性氧代谢物的类型和位置。虽然磷光蛋白能检测到由可溶性试剂刺激的中性粒细胞悬液中的活性氧代谢物,但颗粒状刺激物显然不是磷光蛋白依赖性中性粒细胞化学发光的有效触发剂。用fMet-Leu-Phe(1至100 nmol/l)刺激的中性粒细胞在刺激后45至60秒显示出最大的磷光蛋白依赖性化学发光。最大化学发光时间实际上与fMet-Leu-Phe浓度无关。相比之下,达到最大发光的时间从100 nmol/l佛波酯时的60秒增加到1 nmol/l佛波酯时的295秒。超氧化物歧化酶(20微克/毫升,80%抑制率)和将孵育培养基中的氧浓度降低到小于0.5微摩尔/升(95%抑制率)均导致刺激的化学发光受到显著抑制。相比之下,髓过氧化物酶抑制剂叠氮化钠(0.1毫摩尔/升)仅对磷光蛋白依赖性中性粒细胞化学发光产生50%的抑制作用。我们的结果表明,磷光蛋白能检测到由可溶性刺激物刺激的细胞释放的超氧自由基,但不能检测到颗粒状刺激物引发的细胞内氧化活性。

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