Activities and Structure-Function Analysis of Fission Yeast Inositol Pyrophosphate (IPP) Kinase-Pyrophosphatase Asp1 and Its Impact on Regulation of <i>pho1</i> Gene Expression.

Overview

abstract

Inositol pyrophosphates (IPPs) are signaling molecules that regulate cellular phosphate homeostasis in diverse eukaryal taxa. In fission yeast, mutations that increase 1,5-IP₈ derepress the PHO regulon while mutations that ablate IP₈ synthesis are PHO hyper-repressive. Fission yeast Asp1, the principal agent of 1,5-IP₈ dynamics, is a bifunctional enzyme composed of an N-terminal IPP kinase domain and a C-terminal IPP pyrophosphatase domain. Here we conducted a biochemical characterization and mutational analysis of the autonomous Asp1 kinase domain (aa 1-385). Reaction of Asp1 kinase with IP₆ and ATP resulted in both IP₆ phosphorylation to 1-IP₇ and hydrolysis of the ATP γ-phosphate, with near-equal partitioning between productive 1-IP₇ synthesis and unproductive ATP hydrolysis under optimal kinase conditions. By contrast, reaction of Asp1 kinase with 5-IP₇ is 22-fold faster than with IP₆ and is strongly biased in favor of IP₈ synthesis versus ATP hydrolysis. Alanine scanning identified essential constituents of the active site. We deployed the Ala mutants to show that derepression of pho1 expression correlated with Asp1's kinase activity. In the case of full-length Asp1, the activity of the C-terminal pyrophosphatase domain stifled net phosphorylation of the 1-position during reaction of Asp1 with ATP and either IP₆ or 5-IP₇. We report that inorganic phosphate is a concentration-dependent enabler of net IP₈ synthesis by full-length Asp1 in vitro, by virtue of its antagonism of IP₈ turnover. IMPORTANCE Expression of the fission yeast phosphate regulon is sensitive to the intracellular level of the inositol pyrophosphate (IPP) signaling molecule 1,5-IP₈. IP₈ dynamics are determined by Asp1, a bifunctional enzyme comprising N-terminal IPP 1-kinase and C-terminal IPP 1-pyrophosphatase domains that catalyze IP₈ synthesis and catabolism, respectively. Here, we interrogated the activities and specificities of the Asp1 kinase domain and full length Asp1. We find that reaction of Asp1 kinase with 5-IP₇ is 22-fold faster than with IP₆ and is strongly biased in favor of IP₈ synthesis versus the significant unproductive ATP hydrolysis seen during its reaction with IP₆. We report that full-length Asp1 catalyzes futile cycles of 1-phosphate phosphorylation by its kinase component and 1-pyrophosphate hydrolysis by its pyrophosphatase component that result in unproductive net consumption of the ATP substrate. Net synthesis of 1,5-IP₈ is enabled by physiological concentrations of inorganic phosphate that selectively antagonize IP₈ turnover.