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蛋白质结合的二硝基苯基基团对抗二硝基苯基抗体单价片段的可及性。

The accessibility of protein-bound dinitrophenyl groups to univalent fragments of anti-dinitrophenyl antibody.

作者信息

Knight C G, Green N M

出版信息

Biochem J. 1976 Nov;159(2):323-33. doi: 10.1042/bj1590323.

Abstract

A series of N-(N-dinitrophenylaminoalkyl)maleimides were sythesized with alkyl-chain lengths of two, four and six carbon atoms. When these compounds reacted with the thiol group of mercaptalbumin, the tryptophan fluorescence of the protein was quenched. This change in fluorescence was used to determine the rate of reaction of the Dnp (dinitrophenyl)-maleimides with mercaptalbumin. The second-order rate constants were similar to those observed in reactions between low-molecular-weight thiol compounds and maleimides. When N-(N-Dnp-aminoalkyl)succinimidomercaptalbumins were added to univalent fragments of anti-Dnp antibody the antibody fluorescence was quenched. Florescence-quenching titrations showed that the protein-bound Dnp groups were fully available to the antibody even when the alkyl chain was short. The apparent dissociation constants were significantly greater than that of the interaction between anti-Dnp antibody and the free hapten, 6-(N-Dnp)-aminohexanoate. The antibody fluorescence was quenched efficienty by [dnp-Lys41]ribonuclease A, also with an increased dissociation constant. It could be concluded from the increase in dissociation constant that the Dnp group spent no more than 0.1% of its time in the dissociated state, available to antibody. The second-order rate constants for the association between the Dnp-mercaptablumins and the antibody were determined and were similar in magnitude to those observed in other interactions between protein and anti-protein antibody.

摘要

合成了一系列具有两个、四个和六个碳原子烷基链长度的N-(N-二硝基苯基氨基烷基)马来酰亚胺。当这些化合物与巯基白蛋白的巯基反应时,蛋白质的色氨酸荧光被猝灭。利用这种荧光变化来测定Dnp(二硝基苯基)-马来酰亚胺与巯基白蛋白的反应速率。二级反应速率常数与在低分子量硫醇化合物和马来酰亚胺之间反应中观察到的相似。当将N-(N-Dnp-氨基烷基)琥珀酰亚胺基巯基白蛋白添加到抗Dnp抗体的单价片段中时,抗体荧光被猝灭。荧光猝灭滴定表明,即使烷基链很短,与蛋白质结合的Dnp基团也能完全与抗体结合。表观解离常数明显大于抗Dnp抗体与游离半抗原6-(N-Dnp)-氨基己酸之间相互作用的解离常数。[dnp-Lys41]核糖核酸酶A也能有效地猝灭抗体荧光,其解离常数也增加。从解离常数的增加可以得出结论,Dnp基团处于可与抗体结合的解离状态的时间不超过0.1%。测定了Dnp-巯基白蛋白与抗体之间结合的二级反应速率常数,其大小与在蛋白质与抗蛋白质抗体之间的其他相互作用中观察到的相似。

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