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荧光法证明配体诱导的构象变化可控制F1-三磷酸腺苷酶的活性。

Fluorometric evidence for control of the activity of F1-adenosinetriphosphatase by ligand-induced conformation change.

作者信息

Wang J H

出版信息

J Bioenerg Biomembr. 1986 Apr;18(2):101-11. doi: 10.1007/BF00743479.

Abstract

The effect of ATP on the fluorescence intensity of bovine heart F1-adenosinetriphosphatase labeled at its essential Lys with 7-chloro-4-nitro-2,1,3-benzoxadiazole (N-NBD-F1) has been examined in solutions containing different concentrations of ADP. The fluorescence of N-NBD-F1 is unaffected by ATP in the absence of ADP. But when increasing amounts of ATP are added to a solution of N-NBD-F1 containing 0.37 or 1.0mM ADP, the fluorescence of N-NBD-F1 first decreases and then increases continually as the concentration of ATP is further raised. Parallel measurements of the suppression of the fluorescence of N-NBD-F1 and the inhibition of the ATPase activity of the unlabeled enzyme by ADP in the presence of ATP show a quantitative correlation between the changes in fluorescence and in ATPase activity. The data are consistent with the model for F1-ATPase with one principal catalytic beta' subunit for ATP hydrolysis and synthesis, and two auxiliary beta" subunits which control the conformation and hence the catalytic activity of beta' through interaction between all the subunits.

摘要

在含有不同浓度ADP的溶液中,研究了ATP对用7-氯-4-硝基-2,1,3-苯并恶二唑(N-NBD-F1)标记其必需赖氨酸的牛心F1-腺苷三磷酸酶荧光强度的影响。在没有ADP的情况下,N-NBD-F1的荧光不受ATP影响。但是,当向含有0.37或1.0mM ADP的N-NBD-F1溶液中加入越来越多的ATP时,随着ATP浓度进一步升高,N-NBD-F1的荧光先降低,然后持续增加。在ATP存在下,对N-NBD-F1荧光的抑制和ADP对未标记酶的ATPase活性的抑制进行平行测量,结果表明荧光变化与ATPase活性变化之间存在定量相关性。这些数据与F1-ATPase的模型一致,该模型具有一个用于ATP水解和合成的主要催化β'亚基,以及两个辅助β"亚基,它们通过所有亚基之间的相互作用控制β'的构象,从而控制其催化活性。

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