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DNA适配体-血红素复合物的DNA增强过氧化物酶活性。

DNA-enhanced peroxidase activity of a DNA-aptamer-hemin complex.

作者信息

Travascio P, Li Y, Sen D

机构信息

Institute of Molecular Biology & Biochemistry, Simon Fraser University, Burnaby, British Columbia, Canada.

出版信息

Chem Biol. 1998 Sep;5(9):505-17. doi: 10.1016/s1074-5521(98)90006-0.

DOI:10.1016/s1074-5521(98)90006-0
PMID:9751647
Abstract

BACKGROUND

In vitro selection (SELEX) previously identified short single-stranded DNAs that specifically bound N-methylmesoporphyrin IX (NMM), a stable transition-state analogue for porphyrin-metallation reactions. Interestingly, iron(III)-protoporphyrin (hemin) was a good competitive inhibitor for the DNA-catalyzed metallation reaction, and appeared to bind strongly to the NMM-binding DNA aptamers. We investigated the peroxidase activity of the aptamer-hemin complexes to see if the DNA component of the complex, like the apoenzymes in protein peroxidases, could enhance the low intrinsic peroxidatic activity of hemin.

RESULTS

Two porphyrin-binding DNA aptamers bound hemin with submicromolar affinity. The aptamer-hemin complexes had significantly higher peroxidase activity than hemin alone, under physiological conditions. The Vobs of the PS2.M-hemin complex was 250 times greater than that of hemin alone, and significantly superior to a previously reported hemin-catalytic-antibody complex. Preliminary spectroscopic evidence suggests the coordination of the hemin iron in the complex changes, such that the complex more closely resembles horseradish peroxidase and other heme proteins rather than hemin.

CONCLUSIONS

A new class of catalytic activity for nucleic acids is reported. The aptamer-hemin complexes described are novel DNA enzymes and their study will help elucidate the structural and functional requirements of peroxidase enzymes in general and the ways that a nucleic acid 'apoenzyme' might work to enhance the intrinsic peroxidatic ability of hemin. These aptamer-hemin complexes could be regarded as prototypes for redox-catalyzing ribozymes in a primordial 'RNA world'.

摘要

背景

体外筛选(SELEX)先前鉴定出了能特异性结合N-甲基中卟啉IX(NMM)的短单链DNA,NMM是卟啉金属化反应的一种稳定过渡态类似物。有趣的是,铁(III)-原卟啉(血红素)是DNA催化金属化反应的良好竞争性抑制剂,并且似乎能与NMM结合DNA适配体强烈结合。我们研究了适配体-血红素复合物的过氧化物酶活性,以确定复合物中的DNA成分是否能像蛋白质过氧化物酶中的脱辅基酶一样,增强血红素较低的固有过氧化物活性。

结果

两种卟啉结合DNA适配体以亚微摩尔亲和力结合血红素。在生理条件下,适配体-血红素复合物的过氧化物酶活性明显高于单独的血红素。PS2.M-血红素复合物的表观反应速率(Vobs)比单独的血红素高250倍,且明显优于先前报道的血红素-催化抗体复合物。初步光谱证据表明复合物中血红素铁的配位发生了变化,使得该复合物更类似于辣根过氧化物酶和其他血红素蛋白,而不是血红素。

结论

报道了一类新的核酸催化活性。所描述的适配体-血红素复合物是新型DNA酶,对它们的研究将有助于阐明一般过氧化物酶的结构和功能要求,以及核酸“脱辅基酶”增强血红素固有过氧化物能力的作用方式。这些适配体-血红素复合物可被视为原始“RNA世界”中氧化还原催化核酶的原型。

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