Publications

Displaying 26 - 50 of 53

Photochemistry and Photobiology

May 1, 2006

Author(s)

Adolfas K. Gaigalas, David T. Gallagher, Kenneth D. Cole, Lili Wang, T. Singh, V Reipa

Crystal Structure of the Class IV Adenylyl Cyclase From Yersinia Pestis

March 1, 2006

Author(s)

N Smith, Sung Kim, Prasad T. Reddy, David T. Gallagher

ABSTRACT: The crystal structure of the class IV adenylyl cyclase from Yersinia pestis is reported at 1.9 resolution. The class IV fold is distinct from the previously described folds for class II and class III ACs. The dimeric Yp AC-IV folds into an

Structural analysis of ligand binding and catalysis in chorismate lyase

January 1, 2006

Author(s)

N. Smith, A. Roitberg, E. Rivera, A. Howard, Marcia J. Holden, M. Mayhew, S. Kaistha, David T. Gallagher

Structure of Alanine Dehydrogenase from Archaeoglobus: Active Site Analysis and Relation to Bacterial Cyclodeaminases and Mammalian mu Crystallin

September 3, 2004

Author(s)

David T. Gallagher, H G. Monbouquette, I Schroder, Hugh Robinson, Marcia J. Holden, N Smith

The hyperthermophilic archaeon Archaeoglobus fulgidus contains an L-Ala dehydrogenase (AlaDH, EC 1.4.1.1) that is not homologous to known bacterial dehydrogenases and appears to represent a previously unrecognized archaeal group of NAD-dependent

Local and Global Control Mechanisms in Allosteric Threonine Deaminase

June 1, 2004

Author(s)

David T. Gallagher, D Chinchilla, Herbert Lau, Edward Eisenstein

Allosteric and cooperative control signals were investigated in the tetrameric enzyme threonine deaminase. The tetramer consists of two dimers that associate at the x dyad. The structure pointed the way to use the Q175E mutation to create hybrid tetramers

Structure of C73G putidaredoxin from Pseudomonas putida

May 1, 2004

Author(s)

N Smith, M P. Mayhew, Marcia J. Holden, H Kelly, H Robinson, A Heroux, V L. Vilker, David T. Gallagher

Crystallization and Phasing of Alanine Dehydrogenase From Archaeoglobus Fulgidus

December 1, 2003

Author(s)

N Smith, M P. Mayhew, Hugh Robinson, A Heroux, D Charlton, Marcia J. Holden, David T. Gallagher

Alanine dehydrogenase (AlaDH) from the hyperthermophilic archaeon A. fudgidus is a dimer of 35 kdal chains. The gene (AF1665) is annotated as an ornithine cyclodeaminase based on homology with the ornithine deaminase/ mu crystallin enzyme family. It

X-Ray Topography of Microgravity-Grown Ribonuclease S Crystals

August 1, 2003

Author(s)

David T. Gallagher, C Stover, D Charlton, L Arnowitz, David R. Black

Crystals of the enzyme RNase S were grown at micro and unit gravity using a dialysis-based dynamically controlled device. Crystals were grown at 24 C on space shuttle flights STS 93 and STS 95. Control crystals were grown simultaneously in ground

Fluorescence Resonance Energy Transfer Between Donor-Acceptor Pair on Two Oligonucleotides Hybridized Adjacently to a DNA Template

January 1, 2003

Author(s)

Lili Wang, Adolfas K. Gaigalas, J L. Blasic, Marcia J. Holden, David T. Gallagher, R Pires

We have used fluorescein as the energy donor and rhodamine as the acceptor to measure the efficiency of fluorescence resonance energy transfer (FRET) in a set of hybridized DNA constructs. The two fluorophores are covalently attached via linkers to two

Structural Basis of Thermostability: Analysis of Stabilizing Mutations in Subtilisin BPN

July 26, 2002

Author(s)

O Almog, David Travis Gallagher, Jane E. Ladner, S Strausberg, Patrick Alexander, Phillip Bryan, G L. Gilliland

The crystal structures of two thermally stabilized subtilisin BPN' variants, S63 and S88, are reported here at 1.8 and 1.9 resolution, respectively. The micromolar affinity calcium-binding site (site A) has been deleted (δ 75-83) in these variants

Synchrotron White-Beam X-Ray Topography of Ribonuclease S Crystals

April 1, 2002

Author(s)

W M. Vetter, David Travis Gallagher, M Dudley

With careful experimental design indexed synchrotron white-beam X-ray topographs of ribonuclease S crystals at ambient temperature could be recorded with a definition and contrast comparable to that of monochromatic beam topographs of other proteins

Chorismate Lyase: Kinetics and Engineering for Stability

January 31, 2002

Author(s)

Marcia J. Holden, M P. Mayhew, David T. Gallagher, V L. Vilker

By removing the enolpyruvyl group from chorismate, chorismate lyase (CL) produces p-hydroxybenzoate (p-HB) for the ubiquinone biosynthetic pathway. We have analyzed CL by several spectroscopic and chemical techniques and measured its kinetic (k cat = 1.7x

Protein Packing Interactions and Polymorphy of Chorismate Lyase From E. Coli

November 1, 2001

Author(s)

David T. Gallagher

The enzyme chorismate lyase from E. coli crystallizes in three well characterized polymorphs in identical conditions. Wild-type enzyme tends to aggregate, even in the presence of reducing agent, and yields monoclinic crystals that grow in intricate

The Crystal Structure of Chorismate Lyase Shows a New Fold and a Tightly Retained Product

August 15, 2001

Author(s)

David T. Gallagher, M P. Mayhew, Marcia J. Holden, A J. Howard, K J. Kim, V L. Vilker

The enzyme chorismate lyase (CL) catalyzes the removal of pyruvate from chorismate to produce 4-hydroxy benzoate (4HB) for the ubiquinone pathway. In Escherichia coli, CL is monomeric with 164 residues; we have determined the structure of the CL product

Applying X-Ray Topography and Diffractometry to Improve Protein Crystal Growth

February 21, 2001

Author(s)

David R. Black, L Arnowitz, David T. Gallagher

In order to obtain adequate diffraction data to determine the structure of the protein of interest, crystal quality is important. Although in this context there may be no single concise definition of quality, it must involve adequate size, singleness

Probing Protein Interaction Through Crystal Growth Structure, Mutation, and Mechanism in Subtilisin s88

May 1, 2000

Author(s)

Q Pan, David Travis Gallagher

Observations of systematic variation in the shapes of protein crystals have unique potential to report chemical effects on protein-protein interactions, because diffraction can be used to image the detailed structure that links an easily controlled cause

Role of Competitive Interactions in Growth Rate Trends of Subtilsin s88 Crystals

May 1, 2000

Author(s)

D Asthagirl, A Lenhoff, David Travis Gallagher

An orthorhombic crystal form of subtilisin BPN' variant s88 exhibits a systematic variation in growth rates of its three unique faces, resulting in pronounced variations in crystal morphology as a function of the ionic strength. We have sought to explain

Crystallization and 1.1 Angstrom Diffraction of Chorismate Lyase From Escherichia Coli

February 1, 2000

Author(s)

C Stover, M P. Mayhew, Marcia J. Holden, A Howard, David Travis Gallagher

Clorismate pathway enzymes are important as producers of nonnucleotide aromatic compounds. The enzyme chorismate layase from Escherichia coli has been crystallized in four distinct forms, three of which have been characterized by x-ray diffraction. Despite

Ultrasonic Measurement of Stress in Pin and Hanger Connections

January 1, 1999

Author(s)

A V. Clark, David T. Gallagher, C S. Hehman, P A. Fuchs, M G. Lozev

Pin and hanger connections are used in bridges to suspend an interior span from the outer spans. The connections can sometimes lock up due to corrosion. If lockup ocurs the stresses in the connection are cycled due to thermal expanison and contraction of

Mechanism of Ionic Strength Dependence of Crystal Growth Rates in a Subtilsin Variant

October 1, 1998

Author(s)

David T. Gallagher, Q Pan, G L. Gilliland

An orthorhombic crystal form of subtilisin exhibits a systematic variation in growth rates of its three unique faces, resulting in pronounced morphology variations, depending on ionic strength. Several common salts cause a concentration-dependent change in