5-羟基- 2,3 -二氢酞嗪- 1,4 -二酮和鲁米诺共底物在增强化学发光反应中检测辣根过氧化物酶的比较。

L J Kricka, X Ji, G H Thorpe, B Edwards, J Voyta, I Bronstein
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引用次数: 11

摘要

评价了5-羟基- 2,3 -二氢酞嗪- 1,4 -二酮(HDP)作为共底物在化学发光检测辣根过氧化物酶中的应用。几种取代的芳基硼酸衍生物(4-苯基,4-碘)作为过氧化物酶催化反应的有效促进剂。螯合剂(EDTA)和表面活性剂(Tween-20和[聚(乙烯苄基)三烷基氯化磷-聚(乙烯苄基)三辛基氯化磷共聚物])的加入可调制HDP和鲁米诺的背景光发射以及信号的强度和持续时间。然而,在过氧化物酶实验中发现HDP不如鲁米诺。比较研究表明,在500 amol的过氧化物酶下,使用基于商业发光胺的信号试剂比hdp - edta - twein -20试剂的S/B高10倍(S/B t = 0 min 21.8 vs 1.7, S/B t = 10 min 17.8 vs 2.0)。
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Comparison of 5-hydroxy-2, 3-dihydrophthalazine-1, 4-dione and luminol as co-substrates for detection of horseradish peroxidase in enhanced chemiluminescent reactions.

The utility of 5-hydroxy-2, 3-dihydrophthalazine-1, 4-dione (HDP) as a co-substrate for the chemiluminescent detection of horseradish peroxidase was assessed. Several substituted aryl boronic acid derivatives (4-phenyl, 4-iodo) acted as potent enhancers of the peroxidase catalyzed reaction. Addition of chelating agents (EDTA) and surfactants (Tween-20 and [poly (vinylbenzyl)tributylphosphonium chloride-poly (vinylbenzyl) trioctylphosphonium chloride copolymer]) modulated background light emission and the intensity and duration of the signal from both HDP and luminol. However, HDP was found to be inferior to luminol in the peroxidase assay. Comparative studies revealed that at 500 amol of peroxidase the S/B was ten-fold higher using a commercial luminol-based signal reagent as compared with an HDP-EDTA-Tween-20 reagent (S/B t = 0 min 21.8 vs 1.7, S/B t = 10 min 17.8 vs 2.0).

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