AUTHOR=Grzechowiak Marta , Sliwiak Joanna , Jaskolski Mariusz , Ruszkowski Milosz 

TITLE=Structural Studies of Glutamate Dehydrogenase (Isoform 1) From Arabidopsis thaliana, an Important Enzyme at the Branch-Point Between Carbon and Nitrogen Metabolism

JOURNAL=Frontiers in Plant Science

VOLUME=11

YEAR=2020

URL=https://www.frontiersin.org/journals/plant-science/articles/10.3389/fpls.2020.00754

DOI=10.3389/fpls.2020.00754

ISSN=1664-462X

ABSTRACT=<p>Glutamate dehydrogenase (GDH) releases ammonia in a reversible NAD(P)<sup>+</sup>-dependent oxidative deamination of glutamate that yields 2-oxoglutarate (2OG). In current perception, GDH contributes to Glu homeostasis and plays a significant role at the junction of carbon and nitrogen assimilation pathways. GDHs are members of a superfamily of ELFV (Glu/Leu/Phe/Val) amino acid dehydrogenases and are subdivided into three subclasses, based on coenzyme specificity: NAD<sup>+</sup>-specific, NAD<sup>+</sup>/NADP<sup>+</sup> dual-specific, and NADP<sup>+</sup>-specific. We determined in this work that the mitochondrial <italic>At</italic>GDH1 isozyme from <italic>A. thaliana</italic> is NAD<sup>+</sup>-specific. Altogether, <italic>A. thaliana</italic> expresses three GDH isozymes (<italic>At</italic>GDH1-3) targeted to mitochondria, of which <italic>At</italic>GDH2 has an extra EF-hand motif and is stimulated by calcium. Our enzymatic assays of <italic>At</italic>GDH1 established that its sensitivity to calcium is negligible. <italic>In vivo</italic> the <italic>At</italic>GDH1-3 enzymes form homo- and heterohexamers of varied composition. We solved the crystal structure of recombinant <italic>At</italic>GDH1 in the apo-form and in complex with NAD<sup>+</sup> at 2.59 and 2.03 Å resolution, respectively. We demonstrate also that both in the apo form and in 1:1 complex with NAD<sup>+</sup>, it forms <italic>D</italic><sub>3</sub>-symmetric homohexamers. A subunit of <italic>At</italic>GDH1 consists of domain I, which is involved in hexamer formation and substrate binding, and of domain II which binds coenzyme. Most of the subunits in our crystal structures, including those in NAD<sup>+</sup> complex, are in open conformation, with domain II forming a large (albeit variable) angle with domain I. One of the subunits of the <italic>At</italic>GDH1-NAD<sup>+</sup> hexamer contains a serendipitous 2OG molecule in the active site, causing a dramatic (∼25°) closure of the domains. We provide convincing evidence that the N-terminal peptide preceding domain I is a mitochondrial targeting signal, with a predicted cleavage site for mitochondrial processing peptidase (MPP) at Leu17-Leu18 that is followed by an unexpected potassium coordination site (Ser27, Ile30). We also identified several MPD [(+/-)-2-methyl-2,4-pentanediol] binding sites with conserved sequence. Although <italic>At</italic>GDH1 is insensitive to MPD in our assays, the observation of druggable sites opens a potential for non-competitive herbicide design.</p>