Thermodynamic analysis of Kex2 activity: The acylation and deacylation steps are potassium- and substrate-dependent.

Biophys Chem

Centro Interdisciplinar de Investigação Bioquímica, Universidade de Mogi das Cruzes - UMC, Av. Cândido Xavier de Almeida e Souza, 200, Sala 1S-15, Vila Partênio, CEP: 08780-911 Mogi das Cruzes, SP, Brazil. Electronic address:

Published: April 2018

Kex2 is the prototype of a large family of eukaryotic subtilisin-related proprotein-processing proteases that cleave at sites containing pairs of basic residues. Here, we studied the effects of KCl on the individual rate constants of association, dissociation, acylation and deacylation and determined the thermodynamic parameters at each step of the Kex2 reaction. Potassium bound Kex2 with K=20.3mM. The order in which potassium entered the reaction system modified the effect of activation or inhibition, which depended on the size of the substrate. A possible allosteric potassium binding site at the S subsite was involved in activation, and a distant site located between the catalytic domain and the P-domain was involved in inhibition. Potassium decreased the energetic barriers of almost all steps of catalysis. The acylation of Ac-PMYKR-AMC in the absence of potassium was the rate-limiting step. Therefore, for substrates containing a P-Arg, the deacylation step is not necessarily the rate-limiting event, and other residues at the P' positions may participate in controlling the acylation and deacylation steps. Thus, it is reasonable to conclude that potassium is involved in the processing of the α-mating factor that promotes Ca mobilization by activating a high-affinity Ca-influx system to increase the cytosolic [Ca], resulting in the activation of channels that are essential for the survival of Saccharomyces cerevisiae cells.

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Source
http://dx.doi.org/10.1016/j.bpc.2017.11.007DOI Listing

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