Fluoride Inhibition of Enolase: Crystal Structure and Thermodynamics

Qin, Jie; Chai, Geqing; Brewer, John M; Lovelace, Leslie L; Lebioda, Lukasz

doi:10.1021/bi051558s

Title: Fluoride Inhibition of Enolase: Crystal Structure and Thermodynamics

Journal Article · Fri Dec 03 00:00:00 EST 2010 · Biochemistry-US

DOI:https://doi.org/10.1021/bi051558s· OSTI ID:1007700

Qin, Jie; Chai, Geqing; Brewer, John M; Lovelace, Leslie L; Lebioda, Lukasz ^[1]

Enolase is a dimeric metal-activated metalloenzyme which uses two magnesium ions per subunit: the strongly bound conformational ion and the catalytic ion that binds to the enzyme-substrate complex inducing catalysis. The crystal structure of the human neuronal enolase-Mg{sub 2}F{sub 2}P{sub i} complex (enolase fluoride/phosphate inhibitory complex, EFPIC) determined at 1.36 {angstrom} resolution shows that the combination of anions effectively mimics an intermediate state in catalysis. The phosphate ion binds in the same site as the phosphate group of the substrate/product, 2-phospho-d-glycerate/phosphoenolpyruvate, and induces binding of the catalytic Mg{sup 2+} ion. One fluoride ion bridges the structural and catalytic magnesium ions while the other interacts with the structural magnesium ion and the ammonio groups of Lys 342 and Lys 393. These fluoride ion positions correspond closely to the positions of the oxygen atoms of the substrate's carboxylate moiety. To relate structural changes resulting from fluoride, phosphate, and magnesium ions binding to those that are induced by phosphate and magnesium ions alone, we also determined the structure of the human neuronal enolase-Mg{sub 2}Pi complex (enolase phosphate inhibitory complex, EPIC) at 1.92 {angstrom} resolution. It shows the closed conformation in one subunit and a mixture of open and semiclosed conformations in the other. The EPFIC dimer is essentially symmetric while the EPIC dimer is asymmetric. Isothermal titration calorimetry data confirmed binding of four fluoride ions per dimer and yielded K{sub b} values of 7.5 x 10{sup 5} {+-} 1.3 x 10{sup 5}, 1.2 x 10{sup 5} {+-} 0.2 x 10{sup 5}, 8.6 x 10{sup 4} {+-} 1.6 x 10{sup 4}, and 1.6 x 10{sup 4} {+-} 0.7 x 10{sup 4} M{sup -1}. The different binding constants indicate negative cooperativity between the subunits; the asymmetry of EPIC supports such an interpretation.

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Research Organization:: Argonne National Lab. (ANL), Argonne, IL (United States). Advanced Photon Source (APS)

Sponsoring Organization:: USDOE

OSTI ID:: 1007700

Journal Information:: Biochemistry-US, Vol. 45, Issue (3) ; 03, 2006; ISSN 0006-2960

Country of Publication:: United States

Language:: ENGLISH

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36 MATERIALS SCIENCE
ANIONS
ASYMMETRY
ATOMS
CALORIMETRY
CATALYSIS
CRYSTAL STRUCTURE
DIMERS
FLUORIDES
MAGNESIUM IONS
MIXTURES
OXYGEN
PHOSPHATES
RESOLUTION
THERMODYNAMICS
TITRATION

Title: Fluoride Inhibition of Enolase: Crystal Structure and Thermodynamics

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