髓过氧化物酶在吞噬人单核细胞鲁米诺依赖性化学发光反应中的作用。

S Seim
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摘要

在体外分化过程中,鲁米诺依赖性化学发光(CL)-吞噬反应稳步下降,到培养第4天约为初始值的10%。在同一时期,单核细胞裂解物的髓过氧化物酶(MPO)活性也出现平行下降,鲁米诺依赖性cl -反应峰值与MPO活性密切相关。平行培养中吞噬单核细胞的lucigenin依赖性cl -反应在体外培养4天后下降到初始值的85%左右。化学发光是测定在发光氨或荧光素溶液中加入一定量的H2O2或酶促生成的H2O2通量。辣根过氧化物酶(HRPO)显著提高了鲁米诺依赖性CL,而对lucigenin依赖性CL无显著影响。用粗MPO萃取物代替HRPO得到了类似的结果。尽管有证据表明,过氧化物酶可以增强鲁米诺依赖性CL,但在实验培养基中添加HRPO并没有增加4日龄吞噬单核细胞的鲁米诺依赖性CL反应。
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Role of myeloperoxidase in the luminol-dependent chemiluminescence response of phagocytosing human monocytes.

The luminol-dependent chemiluminescence (CL)-response of phagocytosing declined steadily during in vitro differentiation and was approximately 10% of the initial value by the fourth day of culture. A parallel decline in myeloperoxidase (MPO)-activity of monocyte cell lysates was observed during the same period, and a close correlation was found between peak luminol-dependent CL-response and MPO-activity. The lucigenin-dependent CL-response of phagocytosing monocytes in parallel cultures declined to about 85% of the initial value during four days of in vitro culture. Chemiluminescence was determined in solutions of luminol or lucigenin subjected to fixed amounts of H2O2 or enzymatically generated fluxes of H2O2. Horseradish peroxidase (HRPO) markedly enhanced the luminol-dependent CL but not the lucigenin-dependent CL of this cell-free system. Similar results were obtained when a crude MPO extract was substituted for the HRPO. Despite this evidence that luminol-dependent CL is enhanced by peroxidases, addition of HRPO to the assay medium did not increase the luminol-dependent CL-response of four days old, phagocytosing monocytes.

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