The Deacylation Mechanism of AmpC [beta]-Lactamase at Ultrahigh Resolution

Chen, Yu; Minasov, George; Roth, Tomer A; Prati, Fabio; Shoichet, Brian K

doi:10.1021/ja056806m

Title: The Deacylation Mechanism of AmpC [beta]-Lactamase at Ultrahigh Resolution

Journal Article · Fri Mar 05 00:00:00 EST 2010 · J. Am. Chem. Soc.

DOI:https://doi.org/10.1021/ja056806m· OSTI ID:1007741

Chen, Yu; Minasov, George; Roth, Tomer A; Prati, Fabio; Shoichet, Brian K ^[1]

Degli

{beta}-Lactamases confer bacterial resistance to {beta}-lactam antibiotics, such as penicillins. The characteristic class C {beta}-lactamase AmpC catalyzes the reaction with several key residues including Ser64, Tyr150, and Lys67. Here, we describe a 1.07 {angstrom} X-ray crystallographic structure of AmpC {beta}-lactamase in complex with a boronic acid deacylation transition-state analogue. The high quality of the electron density map allows the determination of many proton positions. The proton on the Tyr150 hydroxyl group is clearly visible and is donated to the boronic oxygen mimicking the deacylation water. Meanwhile, Lys67 hydrogen bonds with Ser64O{gamma}, Asn152O{delta}1, and the backbone oxygen of Ala220. This suggests that this residue is positively charged and has relinquished the hydrogen bond with Tyr150 observed in acyl-enzyme complex structures. Together with previous biochemical and NMR studies, these observations indicate that Tyr150 is protonated throughout the reaction coordinate, disfavoring mechanisms that involve a stable tyrosinate as the general base for deacylation. Rather, the hydroxyl of Tyr150 appears to be well positioned to electrostatically stabilize the negative charge buildup in the tetrahedral high-energy intermediate. This structure, in itself, appears consistent with a mechanism involving either Tyr150 acting as a transient catalytic base in conjunction with a neutral Lys67 or the lactam nitrogen as the general base. Whereas mutagenesis studies suggest that Lys67 may be replaced by an arginine, disfavoring the conjugate base mechanism, distinguishing between these two hypotheses may ultimately depend on direct determination of the pKa of Lys67 along the reaction coordinate.

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

Sponsoring Organization:: USDOE

OSTI ID:: 1007741

Journal Information:: J. Am. Chem. Soc., Vol. 128, Issue (9) ; 03, 2006; ISSN 0002-7863

Country of Publication:: United States

Language:: ENGLISH

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08 HYDROGEN
ANTIBIOTICS
ARGININE
BORONIC ACIDS
BUILDUP
ELECTRON DENSITY
HYDROGEN
LACTAMS
MUTAGENESIS
NITROGEN
OXYGEN
PROTONS
RESIDUES
RESOLUTION
TRANSIENTS
WATER

Title: The Deacylation Mechanism of AmpC [beta]-Lactamase at Ultrahigh Resolution

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