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用荧光ADP类似物甲酰二磷酸对线粒体的ADP/ATP载体进行的研究。

Studies of the ADP/ATP carrier of mitochondria with fluorescent ADP analogue formycin diphosphate.

作者信息

Graue C, Klingenberg M

出版信息

Biochim Biophys Acta. 1979 Jun 5;546(3):539-50. doi: 10.1016/0005-2728(79)90086-0.

Abstract

The ADP/ATP carrier was studied by a fluorescent substrate, formycin diphosphate which is the only fluorescent ADP analogue to bind. Its low quantum yield, short decay time and spectral overlap with tryptophan has as yet prevented its wider use. By incorporating fluorescent acceptors of formycin diphosphate fluorescence, anthracene-maleimide and vinylanthracene, into the membrane, these difficulties were circumvented. Only bound formycin diphosphate transfers energy to the probes so that the secondary emission of these probes is a measure for membrane-bound formycin diphosphate. The fluorescent transfer is inhibited by ADP, bongkrekate and carboxyatractylate whether added before or after incubation of formycin diphosphate showing that only binding to the adenine nucleotide carrier is measured. It also shows directly that the earlier demonstrated ADP fixation by bongkrekate is indeed a displacement into the matrix. The fluorescence decay time of the bound formycin diphosphate is measured as 1.95 ns compared to 0.95 ns of the free formycin diphosphate, indicating that formycin diphosphate is bound at the carrier in a non-polar environment. The depolarization decay time was found to be larger than 15 ns, indicating that carrier-bound formycin diphosphate is immobile within this time period.

摘要

通过荧光底物二磷酸(formycin)对ADP/ATP载体进行了研究,二磷酸(formycin)是唯一能结合的荧光ADP类似物。其低量子产率、短衰减时间以及与色氨酸的光谱重叠至今仍阻碍了它的更广泛应用。通过将二磷酸(formycin)荧光的荧光受体——蒽马来酰亚胺和乙烯基蒽掺入膜中,克服了这些困难。只有结合的二磷酸(formycin)能将能量转移到探针上,因此这些探针的二次发射是膜结合二磷酸(formycin)的一种测量方法。无论在二磷酸(formycin)孵育之前还是之后添加,ADP、邦克雷酸和羧基苍术苷都会抑制荧光转移,这表明测量的只是与腺嘌呤核苷酸载体的结合。这也直接表明,先前证明的邦克雷酸对ADP的固定实际上是向基质中的置换。结合的二磷酸(formycin)的荧光衰减时间测得为1.95纳秒,而游离二磷酸(formycin)的荧光衰减时间为0.95纳秒,这表明二磷酸(formycin)在非极性环境中结合在载体上。发现去极化衰减时间大于15纳秒,这表明在这段时间内载体结合的二磷酸(formycin)是不动的。

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