Abstract
The dihydrolipoyl acetyltransferase (E2) component of the mammalian pyruvate dehydrogenase complex forms a 60-subunit core in which E2's inner domain forms a dodecahedron shaped structure surrounded by its globular outer domains that are connected to each other and the inner domain by 2-3-kDa mobile hinge regions. Two of the outer domains are approximately 10 kDa lipoyl domains, an NH2-terminal one, E2L1, and, after the first hinge region a second one, E2L2. The pyruvate dehydrogenase kinase binds tightly to the lipoyl domain region of the oligomeric E2 core and phosphorylates and inactivates the pyruvate dehydrogenase (E1) component. We wished to determine whether lipoyl domain constructs prepared by recombinant techniques from a cDNA for human E2 could bind the bovine E1 kinase and, that being the case, to pursue which lipoyl domain the kinase binds. We also wished to gain insights into how a molecule of kinase tightly bound to the E2 core can rapidly phosphorylate 20-30 molecules of the pyruvate dehydrogenase (E1) component which are also bound to an outer domain of the E2 core. We prepared recombinant constructs consisting of the entire lipoyl domain region or the individual lipoyl domains with or without the intervening hinge region. Constructs were made and used both as free lipoyl domains and fused to glutathione S-transferase (GST). Using GSH-Sepharose to selectively bind GST constructs, tightly bound kinase was shown to rapidly transfer in a highly preferential way from intact E2 core to GST constructs containing the E2L2 domain rather than to ones containing only the E2L1 domain. GST-E2L2-kinase complexes could be eluted from GSH-Sepharose with glutathione. Delipoylation of E2L2 by treatment with lipoamidase eliminated kinase binding supporting a direct role of the lipoyl prosthetic group in this association. Transfer to and selective binding of the kinase by E2L2 but not E2L1 was also demonstrated with free constructs using a sucrose gradient procedure to separate the large E2 core from the various lipoyl domain constructs. E2L2 but not E2L1 increased the activity of resolved kinase by up to 43%. We conclude that the kinase selectively binds to the inner lipoyl domain of E2 subunits and that this association involves its lipoyl prosthetic group. We further suggest that transfer of tightly bound kinase between E2L2 domains occurs by a direct interchange mechanism without formation of free kinase (model presented).(ABSTRACT TRUNCATED AT 400 WORDS)
Highlights
DK18320, by a grant from the Kansas Affiliate of the American Heart Association, and by Agriculture Experiment Station Contribution 956-J
The remaining globular domain, in the exterior region of the mammalian E2 oligomer, functions in the binding of the El component [5, 6] and is designated the E2 B domain. This small (~46 amino acid) domain is flanked on its NH2 terminal side by a relatively large, ~36 amino acid, hinge region (H2), that connects it to the E2 L 2 domain and on its COOH-terminal side by a -20 amino acid hinge region that connects it and the entire flexible, exterior structure to the oligomer-forming inner domain of E2
In early work to address this question of how an E2-bound kinase molecule rapidly phosphorylates many E2-bound El tetramers, studies were conducted with very dilute complex which led to a major portion of the El but little kinase dissociating from the E2 core
Summary
Vol 270, No., Issue of January 13, pp. 793--800, 1995 Printed in U.S.A. Binding of the Pyruvate Dehydrogenase Kinase to Recombinant Constructs Containing the Inner Lipoyl Domain of the Dihydrolipoyl Acetyltransferase Component*. We have suggested that transfer involves a direct interchange of the kinase (i.e. without any free kinase) between the exterior lipoyl domain regions of the E2 core [9] Such movement at the surface of the assembled E2 core would explain how a kinase molecule is able to both bind tightly to E2 core and still phosphorylate 20-30 El tetramers that are bound to the E2 B domain at the surface of the E2 core. We have made the individual domains E2 L1 and E2 L Z and those domains with the connecting HI hinge region attached, E2 L1 'H 1 and E2H1.LZ' and made the bilipoyl domain structure, E2L1.H1.LZ' Several E2 subunits of bacterial PDCs contain two or three lipoyl domains; no roles have been described that are performed in a specific or even highly preferential manner by one of the lipoyl domains in an E2. We have characterized the effects of the individual and bilipoyl domain constructs on kinase activity
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