Your search keyword '"Eccleston JF"' showing total 87 results

1. Interaction of a fluorescent analogue of GDP with elongation factor Tu: steady-state and time-resolved fluorescence studies.

Author

Eccleston, JF, Gratton, E, and Jameson, DM

Subjects

Absorption, Fluorescamine, Guanine Nucleotides, Guanosine Diphosphate, Peptide Elongation Factor Tu, Protein Binding, Spectrometry, Fluorescence, Time Factors, Medicinal and Biomolecular Chemistry, Biochemistry and Cell Biology, Medical Biochemistry and Metabolomics, Biochemistry & Molecular Biology

Abstract

A fluorescent derivative of GDP was prepared by the reaction of 2'-amino-2'-deoxy-GDP with fluorescamine. This derivative binds tightly (KD approximately 4.5 X 10(-8) M) to elongation factor Tu (EF-Tu) from Escherichia coli. The emission properties, including spectra, polarizations, and lifetimes, for fluorescamine-GDP free in solution and bound to EF-Tu are presented. Emission data on the fluorescamine-ethylamine conjugate are also given. A multifrequency phase and modulation lifetime study (using nine modulation frequencies over the range of 2-80 MHz) indicated that the emissions of these three systems were well characterized by single exponential decays corresponding to 1.45 ns for the fluorescamine-ethylamine derivative in buffer and to 7.74 and 11.03 ns for the fluorescamine-GDP derivative free in buffer and bound to EF-Tu, respectively. Multifrequency differential polarized phase fluorometry results indicated a rotational relaxation time of the protein-probe complex of approximately 88 ns; these data also indicated the lack of significant local motion for the probe. Addition of excess GDP to the EF-Tu-probe complex led to displacement of the fluorescamine-GDP derivative as evidenced by the change in both the steady-state and dynamic polarization values. The observed increase in fluorescence intensity upon displacement allowed us to follow the kinetics of the dissociation reaction; a dissociation rate constant of 5.0 X 10(-3) S-1 was determined. These results demonstrate the utility of this 2'-amino-2'-deoxy-GDP analogue as a probe of guanosine nucleotide dependent systems.

Published

1987

2. Intrinsic fluorescence of elongation factor Tu in its complexes with GDP and elongation factor Ts.

Author

Jameson, DM, Gratton, E, and Eccleston, JF

Subjects

Fluorescence, Guanine Nucleotide Exchange Factors, Guanine Nucleotides, Guanosine Diphosphate, Mathematics, Peptide Elongation Factor Tu, Peptide Elongation Factors, Protein Binding, Protein Conformation, Proteins, Spectrometry, Fluorescence, Time Factors, Medicinal and Biomolecular Chemistry, Biochemistry and Cell Biology, Medical Biochemistry and Metabolomics, Biochemistry & Molecular Biology

Abstract

The intrinsic fluorescence properties of elongation factor Tu (EF-Tu) in its complexes with GDP and elongation factor Ts (EF-Ts) have been investigated. The emission spectra for both complexes are dominated by the tyrosine contribution upon excitation at 280 nm whereas excitation at 300 nm leads to exclusive emission from the single tryptophan residue (Trp-184) of EF-Tu. The fluorescence lifetime of this tryptophan residue in both complexes was investigated by using a multifrequency phase fluorometer which achieves a broad range of modulation frequencies utilizing the harmonic content of a mode-locked laser. These results indicated a heterogeneous emission with major components near 4.8 ns for both complexes. Quenching experiments on both complexes indicated limited accessibility of the tryptophan residue to acrylamide and virtually no accessibility to iodide ion. The quenching patterns exhibited by EF-Tu-GDP and EF-Tu X EF-Ts were, however, different; both quenchers were more efficient at quenching the emission from the EF-Tu x EF-Ts complex. Steady-state and dynamic polarization measurements revealed limited local mobility for the tryptophan in the EF-Tu x GDP complex whereas formation of the EF-Tu x EF-Ts complex led to a dramatic increase in this local mobility.

Published

1987

3. Sedimentation equilibrium studies.

Author

Taylor IA, Rittinger K, and Eccleston JF

Subjects

Macromolecular Substances chemistry, Molecular Weight, Solutions chemistry, Macromolecular Substances isolation & purification, Protein Interaction Mapping methods, Protein Interaction Maps

Abstract

The reversible formation of protein-protein interactions plays a crucial role in many biological processes. In order to carry out a thorough quantitative characterization of these interactions it is essential to establish the oligomerization state of the individual components first. The sedimentation equilibrium method is ideally suited to perform these studies because it allows a reliable, accurate, and absolute value of the solution molecular weight of a macromolecule to be obtained. This technique is independent of the shape of the macromolecule under investigation and allows the determination of equilibrium constants for a monomer-multimer self-associating system.

Published

2015

4. Structure of mammalian AMPK and its regulation by ADP.

Author

Xiao B, Sanders MJ, Underwood E, Heath R, Mayer FV, Carmena D, Jing C, Walker PA, Eccleston JF, Haire LF, Saiu P, Howell SA, Aasland R, Martin SR, Carling D, and Gamblin SJ

Subjects

AMP-Activated Protein Kinases genetics, Adenosine Monophosphate metabolism, Adenosine Monophosphate pharmacology, Adenosine Triphosphate metabolism, Adenosine Triphosphate pharmacology, Allosteric Regulation drug effects, Allosteric Regulation genetics, Animals, Binding Sites, Crystallography, X-Ray, Enzyme Activation drug effects, Enzyme Activation genetics, Kinetics, Magnesium metabolism, Mammals, Models, Molecular, Phosphorylation drug effects, Phosphorylation genetics, Protein Binding, Protein Structure, Tertiary drug effects, Protein Structure, Tertiary genetics, Thermodynamics, AMP-Activated Protein Kinases chemistry, AMP-Activated Protein Kinases metabolism, Adenosine Diphosphate metabolism, Adenosine Diphosphate pharmacology

Abstract

The heterotrimeric AMP-activated protein kinase (AMPK) has a key role in regulating cellular energy metabolism; in response to a fall in intracellular ATP levels it activates energy-producing pathways and inhibits energy-consuming processes. AMPK has been implicated in a number of diseases related to energy metabolism including type 2 diabetes, obesity and, most recently, cancer. AMPK is converted from an inactive form to a catalytically competent form by phosphorylation of the activation loop within the kinase domain: AMP binding to the γ-regulatory domain promotes phosphorylation by the upstream kinase, protects the enzyme against dephosphorylation, as well as causing allosteric activation. Here we show that ADP binding to just one of the two exchangeable AXP (AMP/ADP/ATP) binding sites on the regulatory domain protects the enzyme from dephosphorylation, although it does not lead to allosteric activation. Our studies show that active mammalian AMPK displays significantly tighter binding to ADP than to Mg-ATP, explaining how the enzyme is regulated under physiological conditions where the concentration of Mg-ATP is higher than that of ADP and much higher than that of AMP. We have determined the crystal structure of an active AMPK complex. The structure shows how the activation loop of the kinase domain is stabilized by the regulatory domain and how the kinase linker region interacts with the regulatory nucleotide-binding site that mediates protection against dephosphorylation. From our biochemical and structural data we develop a model for how the energy status of a cell regulates AMPK activity.

Published

2011

5. Mechanism of interaction between single-stranded DNA binding protein and DNA.

Author

Kunzelmann S, Morris C, Chavda AP, Eccleston JF, and Webb MR

Subjects

Carbocyanines metabolism, Coumarins metabolism, DNA Helicases chemistry, DNA, Bacterial chemistry, DNA, Single-Stranded chemistry, DNA-Binding Proteins chemistry, Escherichia coli Proteins chemistry, Fluorescent Dyes metabolism, Protein Binding, Spectrometry, Fluorescence, DNA Helicases metabolism, DNA, Bacterial metabolism, DNA, Single-Stranded metabolism, DNA-Binding Proteins metabolism, Escherichia coli Proteins metabolism

Abstract

A single-stranded DNA binding protein (SSB), labeled with a fluorophore, interacts with single-stranded DNA (ssDNA), giving a 6-fold increase in fluorescence. The labeled protein is the adduct of the G26C mutant of the homotetrameric SSB from Escherichia coli and a diethylaminocoumarin {N-[2-(iodoacetamido)ethyl]-7-diethylaminocoumarin-3-carboxamide}. This adduct can be used to assay production of ssDNA during separation of double-stranded DNA by helicases. To use this probe effectively, as well as to investigate the interaction between ssDNA and SSB, the fluorescent SSB has been used to develop the kinetic mechanism by which the protein and ssDNA associate and dissociate. Under conditions where approximately 70 base lengths of ssDNA wrap around the tetramer, initial association is relatively simple and rapid, possibly diffusion-controlled. The kinetics are similar for a 70-base length of ssDNA, which binds one tetramer, and poly(dT), which could bind several. Under some conditions (high SSB and/or low ionic strength), a second tetramer binds to each 70-base length, but at a rate 2 orders of magnitude slower than the rate of binding of the first tetramer. Dissociation kinetics are complex and greatly accelerated by the presence of free wild-type SSB. The main route of dissociation of the fluorescent SSB x ssDNA complex is via association first with an additional SSB and then dissociation. Comparison of binding data with different lengths of ssDNA gave no evidence of cooperativity between tetramers. Analytical ultracentrifugation was used to determine the dissociation constant for labeled SSB(2) x dT(70) to be 1.1 microM at a high ionic strength (200 mM NaCl). Shorter lengths of ssDNA were tested for binding: only when the length is reduced to 20 bases is the affinity significantly reduced.

Published

2010

6. Three-dimensional molecular mapping in a microfluidic mixing device using fluorescence lifetime imaging.

Author

Robinson T, Valluri P, Manning HB, Owen DM, Munro I, Talbot CB, Dunsby C, Eccleston JF, Baldwin GS, Neil MA, de Mello AJ, and French PM

Subjects

Calibration, Equipment Design, Fluorescence, Imaging, Three-Dimensional, Kinetics, Microfluidic Analytical Techniques instrumentation, Microscopy, Fluorescence instrumentation, Time Factors, Microfluidics, Microscopy, Fluorescence methods

Abstract

Fluorescence lifetime imaging (FLIM) is used to quantitatively map the concentration of a small molecule in three dimensions in a microfluidic mixing device. The resulting experimental data are compared with computational fluid-dynamics (CFD) simulations. A line-scanning semiconfocal FLIM microscope allows the full mixing profile to be imaged in a single scan with submicrometer resolution over an arbitrary channel length from the point of confluence. Following experimental and CFD optimization, mixing times down to 1.3+/-0.4 ms were achieved with the single-layer microfluidic device.

Published

2008

7. Structural analysis reveals an amyloid form of the human papillomavirus type 16 E1--E4 protein and provides a molecular basis for its accumulation.

Author

McIntosh PB, Martin SR, Jackson DJ, Khan J, Isaacson ER, Calder L, Raj K, Griffin HM, Wang Q, Laskey P, Eccleston JF, and Doorbar J

Subjects

Amino Acid Sequence, Animals, Biopsy, COS Cells, Chlorocebus aethiops, Gene Deletion, Humans, Molecular Sequence Data, Protein Conformation, Protein Folding, Protein Structure, Secondary, Protein Structure, Tertiary, Sequence Homology, Amino Acid, Human papillomavirus 16 metabolism

Abstract

The abundant human papillomavirus (HPV) type 16 E4 protein exists as two distinct structural forms in differentiating epithelial cells. Monomeric full-length 16E1--E4 contains a limited tertiary fold constrained by the N and C termini. N-terminal deletions facilitate the assembly of E1--E4 into amyloid-like fibrils, which bind to thioflavin T. The C-terminal region is highly amyloidogenic, and its deletion abolishes amyloid staining and prevents E1--E4 accumulation. Amyloid-imaging probes can detect 16E1--E4 in biopsy material, as well as 18E1--E4 and 33E1--E4 in monolayer cells, indicating structural conservation. Our results suggest a role for fibril formation in facilitating the accumulation of E1--E4 during HPV infection.

Published

2008

8. Hydrodynamic characterization of the SufBC and SufCD complexes and their interaction with fluorescent adenosine nucleotides.

Author

Petrovic A, Davis CT, Rangachari K, Clough B, Wilson RJ, and Eccleston JF

Subjects

Electrophoresis, Polyacrylamide Gel, Fluorescent Dyes, Kinetics, Spectrometry, Fluorescence, Adenosine Diphosphate chemistry, Adenosine Triphosphate chemistry, Bacterial Proteins chemistry

Abstract

Bacteria, as well as the plastid organelles of algae and higher plants, utilize proteins of the suf operon. These are involved in Fe-S cluster assembly, particularly under conditions of iron limitation or oxidative stress. Genetic experiments in some organisms found that the ATPase SufC is essential, though its role in Fe-S biogenesis remains unclear. To ascertain how interactions with other individual Suf proteins affect the activity of SufC we coexpressed it with either SufB or SufD from Thermotoga maritima and purified the resulting SufBC and SufCD complexes. Analytical ultracentrifuge and multiangle light-scattering measurements showed that the SufBC complex exists in solution as the tetrameric SufB(2)C(2) species, whereas SufCD exists as an equilibrium mixture of SufCD and SufC(2)D(2). Transient kinetic studies of the complexes were made using fluorescent 2'(3')-O-(N-methylanthraniloyl-(mant) analogues of ATP and ADP. Both SufBC and SufCD bound mantATP and mantADP much more tightly than does SufC alone. Compared to the cleavage step of the mantATPase of SufC alone, that of SufBC was accelerated 180-fold and that of SufCD only fivefold. Given that SufB and SufD have 20% sequence identity and similar predicted secondary structures, the different hydrodynamic properties and kinetic mechanisms of the two complexes are discussed.

Published

2008

9. Rapid kinetic techniques.

Author

Eccleston JF, Martin SR, and Schilstra MJ

Subjects

Anisotropy, Kinetics, Molecular Probes chemistry, Chemistry Techniques, Analytical instrumentation, Chemistry Techniques, Analytical methods

Abstract

The elementary steps in complex biochemical reaction schemes (isomerization, dissociation, and association reactions) ultimately determine how fast any system can react in responding to incoming signals and in adapting to new conditions. Many of these steps have associated rate constants that result in subsecond responses to incoming signals or externally applied changes. This chapter is concerned with the techniques that have been developed to study such rapidly reacting systems in vitro and to determine the values of the rate constants for the individual steps. We focus principally on two classes of techniques: (1) flow techniques, in which two solutions are mixed within a few milliseconds and the ensuing reaction monitored over milliseconds to seconds, and (2) relaxation techniques, in which a small perturbation to an existing equilibrium is applied within a few microseconds and the response of the system is followed over microseconds to hundreds of milliseconds. These reactions are most conveniently monitored by recording the change in some optical signal, such as absorbance or fluorescence. We discuss the instrumentation that is (commercially) available to study fast reactions and describe a number of optical probes (chromophores) that can be used to monitor the changes. We discuss the experimental design appropriate for the different experimental techniques and reaction mechanisms, as well as the fundamental theoretical concepts behind the analysis of the data obtained.

Published

2008

10. Structural basis for AMP binding to mammalian AMP-activated protein kinase.

Author

Xiao B, Heath R, Saiu P, Leiper FC, Leone P, Jing C, Walker PA, Haire L, Eccleston JF, Davis CT, Martin SR, Carling D, and Gamblin SJ

Subjects

AMP-Activated Protein Kinases, Animals, Binding Sites, Crystallography, X-Ray, Humans, Models, Molecular, Protein Structure, Tertiary, Rats, Structure-Activity Relationship, Surface Properties, Adenosine Monophosphate chemistry, Adenosine Monophosphate metabolism, Multienzyme Complexes chemistry, Multienzyme Complexes metabolism, Protein Serine-Threonine Kinases chemistry, Protein Serine-Threonine Kinases metabolism

Abstract

AMP-activated protein kinase (AMPK) regulates cellular metabolism in response to the availability of energy and is therefore a target for type II diabetes treatment. It senses changes in the ratio of AMP/ATP by binding both species in a competitive manner. Thus, increases in the concentration of AMP activate AMPK resulting in the phosphorylation and differential regulation of a series of downstream targets that control anabolic and catabolic pathways. We report here the crystal structure of the regulatory fragment of mammalian AMPK in complexes with AMP and ATP. The phosphate groups of AMP/ATP lie in a groove on the surface of the gamma domain, which is lined with basic residues, many of which are associated with disease-causing mutations. Structural and solution studies reveal that two sites on the gamma domain bind either AMP or Mg.ATP, whereas a third site contains a tightly bound AMP that does not exchange. Our binding studies indicate that under physiological conditions AMPK mainly exists in its inactive form in complex with Mg.ATP, which is much more abundant than AMP. Our modelling studies suggest how changes in the concentration of AMP ([AMP]) enhance AMPK activity levels. The structure also suggests a mechanism for propagating AMP/ATP signalling whereby a phosphorylated residue from the alpha and/or beta subunits binds to the gamma subunit in the presence of AMP but not when ATP is bound.

Published

2007

11. Structural studies on Plasmodium vivax merozoite surface protein-1.

Author

Babon JJ, Morgan WD, Kelly G, Eccleston JF, Feeney J, and Holder AA

Subjects

Animals, Dimerization, Humans, Merozoite Surface Protein 1 genetics, Models, Molecular, Multiprotein Complexes, Nuclear Magnetic Resonance, Biomolecular, Plasmodium vivax genetics, Plasmodium vivax pathogenicity, Protein Structure, Tertiary, Protein Subunits, Recombinant Proteins chemistry, Recombinant Proteins genetics, Static Electricity, Merozoite Surface Protein 1 chemistry, Plasmodium vivax chemistry

Abstract

Plasmodium vivax infection is the second most common cause of malaria throughout the world. Like other Plasmodium species, P. vivax has a large protein complex, MSP-1, located on the merozoite surface. The C-terminal MSP-1 sub-unit, MSP-1(42), is cleaved during red blood cell invasion, causing the majority of the complex to be shed and leaving only a small 15kDa sub-unit, MSP-1(19), on the merozite surface. MSP-1(19) is considered a strong vaccine candidate. We have determined the solution structure of MSP-1(19) from P. vivax using nuclear magnetic resonance (NMR) and show that, like in other Plasmodium species, it consists of two EGF-like domains that are oriented head-to-tail. The protein has a flat, disk-like shape with a highly charged surface. When MSP-1(19) is part of the larger MSP-1(42) precursor it exists as an independent domain with no stable contacts to the rest of the sub-unit. Gel filtration and analytical ultracentrifugation experiments indicate that P. vivax MSP-1(42) exists as a dimer in solution. MSP-1(19) itself is a monomer, however, 35 amino-acids immediately upstream of its N-terminus are sufficient to cause dimerization. Our data suggest that if MSP-1(42) exists as a dimer in vivo, secondary processing would cause the dissociation of two tightly linked MSP-1(19) proteins on the merozoite surface just prior to invasion.

Published

2007

12. The kinetic mechanism of the SufC ATPase: the cleavage step is accelerated by SufB.

Author

Eccleston JF, Petrovic A, Davis CT, Rangachari K, and Wilson RJ

Subjects

Adenosine Diphosphate analogs & derivatives, Adenosine Diphosphate genetics, Adenosine Diphosphate metabolism, Adenosine Triphosphatases genetics, Adenosine Triphosphate analogs & derivatives, Adenosine Triphosphate genetics, Adenosine Triphosphate metabolism, Bacterial Proteins metabolism, Chromatography, High Pressure Liquid, Escherichia coli genetics, Fluorescence Polarization, Fluorescent Dyes metabolism, Iron-Sulfur Proteins genetics, Iron-Sulfur Proteins metabolism, Kinetics, Operon, Phosphorus metabolism, Protein Conformation, Thermotoga maritima chemistry, ortho-Aminobenzoates metabolism, Adenosine Triphosphatases metabolism, Bacterial Proteins genetics

Abstract

Protein products of the suf operon are involved in iron-sulfur metabolism. SufC is an ATPase that can interact with SufB in the absence of nucleotide. We have studied the transient kinetics of the SufC ATPase mechanism using the fluorescent ATP analogue, 2'(3')-O-N-methylanthraniloyl-ATP (mantATP). mantATP initially binds to SufC weakly. A conformational change of the SufC.mantATP complex then occurs followed by the very slow cleavage of mantATP to mantADP and the rapid release of Pi. In the presence of SufB, the cleavage step is accelerated and the release of mantADP is inhibited. Both of these effects promote the formation of a SufC.mantADP complex. In the absence and presence of SufB, mantADP remains more tightly bound to SufC than mantATP. These studies provide a basis for how the SufB and -C proteins interact in the processes involved in regulating iron-sulfur transfer.

Published

2006

13. Cooperative hydrogen bond interactions in the streptavidin-biotin system.

Author

Hyre DE, Le Trong I, Merritt EA, Eccleston JF, Green NM, Stenkamp RE, and Stayton PS

Subjects

Calorimetry, Crystallography, X-Ray, Hydrogen Bonding, Kinetics, Models, Molecular, Mutation, Protein Binding, Streptavidin genetics, Biotin chemistry, Streptavidin chemistry, Thermodynamics

Abstract

The thermodynamic and structural cooperativity between the Ser45- and D128-biotin hydrogen bonds was measured by calorimetric and X-ray crystallographic studies of the S45A/D128A double mutant of streptavidin. The double mutant exhibits a binding affinity approximately 2x10(7) times lower than that of wild-type streptavidin at 25 degrees C. The corresponding reduction in binding free energy (DeltaDeltaG) of 10.1 kcal/mol was nearly completely due to binding enthalpy losses at this temperature. The loss of binding affinity is 11-fold greater than that predicted by a linear combination of the single-mutant energetic perturbations (8.7 kcal/mol), indicating that these two mutations interact cooperatively. Crystallographic characterization of the double mutant and comparison with the two single mutant structures suggest that structural rearrangements at the S45 position, when the D128 carboxylate is removed, mask the true energetic contribution of the D128-biotin interaction. Taken together, the thermodynamic and structural analyses support the conclusion that the wild-type hydrogen bond between D128-OD and biotin-N2 is thermodynamically stronger than that between S45-OG and biotin-N1.

Published

2006

14. Fluorescence-based assays.

Author

Eccleston JF, Hutchinson JP, and Jameson DM

Subjects

Animals, Fluorescence, Fluorescence Resonance Energy Transfer, Fluorescent Dyes, Fluorometry instrumentation, Humans, Protein Binding, Spectrometry, Fluorescence, Fluorometry methods

Published

2005

15. Sedimentation equilibrium studies.

Author

Taylor IA, Eccleston JF, and Rittinger K

Subjects

Animals, Macromolecular Substances, Molecular Weight, Protein Binding, Protein Structure, Quaternary, Proteins metabolism, Ultracentrifugation instrumentation, Proteins chemistry, Ultracentrifugation methods

Abstract

The reversible formation of protein-protein interactions plays a crucial role in many biological processes. In order to carry out a thorough quantitative characterization of these interactions, it is essential to establish the oligomerization state of the individual components first. The sedimentation equilibrium method is ideally suited to perform these studies because it allows a reliable, accurate, and absolute value of the solution molecular weight of a macromolecule to be obtained. This technique is independent of the shape of the macromolecule under investigation and allows the determination of equilibrium constants for a monomer-multimer self-associating system.

Published

2004

16. The mechanism of Ras GTPase activation by neurofibromin.

Author

Phillips RA, Hunter JL, Eccleston JF, and Webb MR

Subjects

Binding Sites, Catalysis, Coumarins metabolism, Enzyme Activation, Guanosine Diphosphate metabolism, Humans, Hydrolysis, Neurofibromin 1 metabolism, Oxygen metabolism, Phosphates metabolism, Protein Binding, Protein Conformation, GTP Phosphohydrolases metabolism, Guanosine Triphosphate metabolism, Neurofibromin 1 pharmacology, Proto-Oncogene Proteins p21(ras) metabolism, ortho-Aminobenzoates metabolism

Abstract

Individual rate constants have been determined for each step of the Ras.GTP hydrolysis mechanism, activated by neurofibromin. Fluorescence intensity and anisotropy stopped-flow measurements used the fluorescent GTP analogue, mantGTP (2'(3')-O-(N-methylanthraniloyl)GTP), to determine rate constants for binding and release of neurofibromin. Quenched flow measurements provided the kinetics of the hydrolytic cleavage step. The fluorescent phosphate sensor, MDCC-PBP was used to measure phosphate release kinetics. Phosphate-water oxygen exchange, using (18)O-substituted GTP and inorganic phosphate (P(i)), was used to determine the extent of reversal of the hydrolysis step and of P(i) binding. The data show that neurofibromin and P(i) dissociate from the NF1.Ras.GDP.P(i) complex with identical kinetics, which are 3-fold slower than the preceding cleavage step. A model is presented in which the P(i) release is associated with the change of Ras from "GTP" to "GDP" conformation. In this model, the conformation change on P(i) release causes the large change in affinity of neurofibromin, which then dissociates rapidly.

Published

2003

17. Parasite plastids: maintenance and functions.

Author

Wilson RJ, Rangachari K, Saldanha JW, Rickman L, Buxton RS, and Eccleston JF

Subjects

Amino Acid Sequence, Animals, Bacterial Proteins chemistry, Bacterial Proteins genetics, Bacterial Proteins metabolism, Models, Molecular, Molecular Sequence Data, Oxidative Stress, Plant Proteins chemistry, Plant Proteins genetics, Plant Proteins metabolism, Protozoan Proteins chemistry, Protozoan Proteins genetics, Evolution, Molecular, Plasmodium falciparum genetics, Plasmodium falciparum physiology, Plastids genetics, Plastids physiology, Protozoan Proteins metabolism

Abstract

Malaria and related parasites retain a vestigial, but biosynthetically active, plastid organelle acquired far back in evolution from a red algal cell. The organelle appears to be essential for parasite transmission from cell to cell and carries the smallest known plastid genome. Why has this genome been retained? The genes it carries seem to be dedicated to the expression of just two "housekeeping" genes. We speculate that one of these, called ycf24 in plants and sufB in bacteria, is tied to an essential "dark" reaction of the organelle--fatty acid biosynthesis. "Ball-park" clues to the function of bacterial suf genes have emerged only recently and point to the areas of iron homeostasis, [Fe-S] cluster formation and oxidative stress. We present experimental evidence for a physical interaction between SufB and its putative partner SufC (ycf16). In both malaria and plants, SufC is encoded in the nucleus and specifies an ATPase that is imported into the plastid.

Published

2003

18. The 2'-O- and 3'-O-Cy3-EDA-ATP(ADP) complexes with myosin subfragment-1 are spectroscopically distinct.

Author

Oiwa K, Jameson DM, Croney JC, Davis CT, Eccleston JF, and Anson M

Subjects

Adenosine Diphosphate analogs & derivatives, Adenosine Triphosphate analogs & derivatives, Anisotropy, Isomerism, Macromolecular Substances, Molecular Conformation, Motion, Protein Binding, Adenosine Diphosphate chemistry, Adenosine Triphosphate chemistry, Fluorescence Polarization methods, Myosin Subfragments chemistry, Spectrometry, Fluorescence methods

Abstract

Ribose-modified highly-fluorescent sulfoindocyanine ATP and ADP analogs, 2'(3')-O-Cy3-EDA-AT(D)P, with kinetics similar to AT(D)P, enable myosin and actomyosin ATPase enzymology with single substrate molecules. Stopped-flow studies recording both fluorescence and anisotropy during binding to skeletal muscle myosin subfragment-1 (S1) and subsequent single-turnover decay of steady-state intermediates showed that on complex formation, 2'-O- isomer fluorescence quenched by 5%, anisotropy increased from 0.208 to 0.357, and then decayed with turnover rate k(cat) 0.07 s(-1); however, 3'-O- isomer fluorescence increased 77%, and anisotropy from 0.202 to 0.389, but k(cat) was 0.03 s(-1). Cy3-EDA-ADP.S1 complexes with vanadate (V(i)) were studied kinetically and by time-resolved fluorometry as stable analogs of the steady-state intermediates. Upon formation of the 3'-O-Cy3-EDA-ADP.S1.V(i) complex fluorescence doubled and anisotropy increased to 0.372; for the 2'-O- isomer, anisotropy increased to 0.343 but fluorescence only 6%. Average fluorescent lifetimes of 2'-O- and 3'-O-Cy3-EDA-ADP.S1.V(i) complexes, 0.9 and 1.85 ns, compare with approximately 0.7 ns for free analogs. Dynamic polarization shows rotational correlation times higher than 100 ns for both Cy3-EDA-ADP.S1.V(i) complexes, but the 2'-O-isomer only has also a 0.2-ns component. Thus, when bound, 3'-O-Cy3-EDA-ADP's fluorescence is twofold brighter with motion more restricted and turnover slower than the 2'-O-isomer; these data are relevant for applications of these analogs in single molecule studies.

Published

2003

19. H-NS oligomerization domain structure reveals the mechanism for high order self-association of the intact protein.

Author

Esposito D, Petrovic A, Harris R, Ono S, Eccleston JF, Mbabaali A, Haq I, Higgins CF, Hinton JC, Driscoll PC, and Ladbury JE

Subjects

Amino Acid Sequence, Amino Acid Substitution, Bacterial Proteins genetics, Bacterial Proteins metabolism, Carbon Isotopes, DNA, Bacterial chemistry, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, Dimerization, Glucose metabolism, Molecular Sequence Data, Mutagenesis, Site-Directed, Nitrogen Isotopes, Nuclear Magnetic Resonance, Biomolecular, Oligopeptides chemistry, Proline metabolism, Protein Conformation, Protein Folding, Protein Structure, Secondary, Salmonella typhimurium chemistry, Sequence Deletion, Solutions, Structure-Activity Relationship, Water chemistry, Bacterial Proteins chemistry, DNA-Binding Proteins chemistry, Models, Molecular

Abstract

H-NS plays a role in condensing DNA in the bacterial nucleoid. This 136 amino acid protein comprises two functional domains separated by a flexible linker. High order structures formed by the N-terminal oligomerization domain (residues 1-89) constitute the basis of a protein scaffold that binds DNA via the C-terminal domain. Deletion of residues 57-89 or 64-89 of the oligomerization domain precludes high order structure formation, yielding a discrete dimer. This dimerization event represents the initial event in the formation of high order structure. The dimers thus constitute the basic building block of the protein scaffold. The three-dimensional solution structure of one of these units (residues 1-57) has been determined. Activity of these structural units is demonstrated by a dominant negative effect on high order structure formation on addition to the full length protein. Truncated and site-directed mutant forms of the N-terminal domain of H-NS reveal how the dimeric unit self-associates in a head-to-tail manner and demonstrate the importance of secondary structure in this interaction to form high order structures. A model is presented for the structural basis for DNA packaging in bacterial cells.

Published

2002

20. Structural and biochemical characterization of a fluorogenic rhodamine-labeled malarial protease substrate.

Author

Blackman MJ, Corrie JE, Croney JC, Kelly G, Eccleston JF, and Jameson DM

Subjects

Animals, Kinetics, Peptides chemistry, Rhodamines metabolism, Spectrometry, Fluorescence, Spectrophotometry, Substrate Specificity, Subtilisins metabolism, Plasmodium falciparum chemistry, Protozoan Proteins, Subtilisins chemistry

Abstract

Activation of the proenzyme form of the malarial protease PfSUB-1 involves the autocatalytic cleavage of an Asp-Asn bond within the internal sequence motif (215)LVSADNIDIS(224). A synthetic decapeptide based on this sequence but with the N- and C-terminal residues replaced by cysteines (Ac-CVSADNIDIC-OH) was labeled with 5- or 6-isomers of iodoacetamidotetramethylrhodamine (IATR). The doubly labeled peptides have low fluorescence because of ground-state, noncovalent dimerization of the rhodamines. Cleavage of either peptide by recombinant PfSUB-1 results in dissociation of the rhodamine dimers, which abolishes the self-quenching and consequently leads to an approximately 30-fold increase in the fluorescence. This spectroscopic signal provides a continuous assay of proteolysis, enabling quantitative kinetic measurements to be made, and has also enabled the development of a fluorescence-based assay suitable for use in high-throughput screens for inhibitors of PfSUB-1. The structure of the rhodamine dimer in the 6-IATR-labeled peptide was shown by NMR to be a face-to-face stacking of the xanthene rings. Time-resolved fluorescence measurements suggest that the doubly labeled peptides exist in an equilibrium consisting of rhodamines involved in dimers (closed forms) and rhodamines not involved in dimers (open forms). These data also indicate that the rhodamine dimers fluoresce and that the associated lifetimes are subnanosecond.

Published

2002

21. Oligomerization and kinetic mechanism of the dynamin GTPase.

Author

Eccleston JF, Binns DD, Davis CT, Albanesi JP, and Jameson DM

Subjects

Guanosine Triphosphate metabolism, Macromolecular Substances, Protein Binding, Protein Conformation, Dynamins chemistry, Dynamins metabolism

Abstract

Dynamin is a large molecular weight GTPase. Amongst other biological processes, it is involved in clathrin-dependent endocytosis. It can self-assemble or assemble on other macromolecular structures that result in an increase in its GTPase activity. Its role in endocytosis has been variously attributed to being a force-generating enzyme or a signalling protein. Here we review evidence for the oligomeric state of dynamin at high and low ionic strength conditions. We also review work on the elementary processes of the dynamin GTPase at high ionic strength and compare these to the ATPase of the force-generating protein myosin and the GTPase of the signalling protein Ras. New data on the interaction of dynamin with a fluorescent derivative of GTPgammaS are also presented. The possible mechanism by which assembly of dynamin leads to an increase in its GTPase activity is discussed.

Published

2002

22. SufC hydrolyzes ATP and interacts with SufB from Thermotoga maritima.

Author

Rangachari K, Davis CT, Eccleston JF, Hirst EM, Saldanha JW, Strath M, and Wilson RJ

Subjects

Adenosine Triphosphatases genetics, Amino Acid Sequence, Animals, Bacterial Proteins genetics, Escherichia coli genetics, Escherichia coli metabolism, Iron metabolism, Membrane Proteins genetics, Mice, Mice, Inbred BALB C, Molecular Sequence Data, Oxidative Stress physiology, Polymerase Chain Reaction, Protein Binding physiology, Recombinant Proteins genetics, Recombinant Proteins metabolism, Sequence Analysis, Sulfur metabolism, Adenosine Triphosphatases metabolism, Adenosine Triphosphate metabolism, Bacterial Proteins metabolism, Membrane Proteins metabolism, Thermotoga maritima metabolism

Abstract

Genetic experiments in bacteria have shown the suf operon is involved in iron homeostasis and the oxidative stress response. The sufB and sufC genes that always occur together in bacteria are also found in plants, and even the malaria parasite, associated with the plastid organelle. Although the suf operon is believed to encode an iron-dependent ABC-transporter there is no direct evidence. By immunolocalization we show here that SufB and SufC are associated with the membrane of Escherichia coli. We also present kinetic studies with a recombinant version of SufC from Thermotoga maritima that shows it is an ATPase and that it interacts with SufB in vitro.

Published

2002

23. MgF(3)(-) as a transition state analog of phosphoryl transfer.

Author

Graham DL, Lowe PN, Grime GW, Marsh M, Rittinger K, Smerdon SJ, Gamblin SJ, and Eccleston JF

Subjects

Aluminum Compounds chemistry, Guanosine Diphosphate chemistry, Models, Molecular, Spectrometry, X-Ray Emission, rho GTP-Binding Proteins metabolism, Fluorides chemistry, Magnesium Compounds chemistry, Phosphorus chemistry, rho GTP-Binding Proteins chemistry

Abstract

The formation of complexes between small G proteins and certain of their effectors can be facilitated by aluminum fluorides. Solution studies suggest that magnesium may be able to replace aluminum in such complexes. We have determined the crystal structure of RhoA.GDP bound to RhoGAP in the presence of Mg(2+) and F(-) but without Al(3+). The metallofluoride adopts a trigonal planar arrangement instead of the square planar structure of AlF(4)(-). We have confirmed that these crystals contain magnesium and not aluminum by proton-induced X-ray emission spectroscopy. The structure adopted by GDP.MgF(-) possesses the stereochemistry and approximate charge expected for the transition state. We suggest that MgF3(-) may be the reagent of choice for studying phosphoryl transfer reactions.

Published

2002

24. Interaction between Ran and Mog1 is required for efficient nuclear protein import.

Author

Baker RP, Harreman MT, Eccleston JF, Corbett AH, and Stewart M

Subjects

Crystallography, X-Ray, Fungal Proteins genetics, Guanine Nucleotide Exchange Factors, Guanosine Diphosphate metabolism, Guanosine Triphosphate metabolism, Models, Molecular, Mutagenesis, Site-Directed, Nuclear Proteins chemistry, Nuclear Proteins genetics, Protein Transport, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, ran GTP-Binding Protein chemistry, ran GTP-Binding Protein genetics, DNA-Binding Proteins, Nuclear Proteins metabolism, Saccharomyces cerevisiae Proteins, ran GTP-Binding Protein metabolism

Abstract

Mog1 is a nuclear protein that interacts with Ran, the Ras family GTPase that confers directionality to nuclear import and export pathways. Deletion of MOG1 in Saccharomyces cerevisiae (Deltamog1) causes temperature-sensitive growth and defects in nuclear protein import. Mog1 has previously been shown to stimulate GTP release from Ran and we demonstrate here that addition of Mog1 to either Ran-GTP or Ran-GDP results in nucleotide release and formation of a stable complex between Mog1 and nucleotide-free Ran. Moreover, MOG1 shows synthetic lethality with PRP20, the Ran guanine nucleotide exchange factor (RanGEF) that also binds nucleotide-free Ran. To probe the functional role of the Mog1-Ran interaction, we engineered mutants of yeast Mog1 and Ran that specifically disrupt their interaction both in vitro and in vivo. These mutants indicate that the interaction interface involves conserved Mog1p residues Asp(62) and Glu(65), and residue Lys(136) in yeast Ran. Mutations at these residues decrease the ability of Mog1 to bind and release nucleotide from Ran. Furthermore, the E65K-Mog1 and K136E-Ran mutations in yeast cause temperature sensitivity and mislocalization of a nuclear import reporter protein, similar to the phenotype observed for the Deltamog1 strain. Our results indicate that a primary function of Mog1 requires binding to Ran and that the Mog1-Ran interaction is necessary for efficient nuclear protein import in vivo.

Published

2001

25. Chemistry of sulforhodamine--amine conjugates.

Author

Corrie JE, Davis CT, and Eccleston JF

Subjects

Adenosine Diphosphate metabolism, Adenosine Triphosphate metabolism, Kinetics, Magnetic Resonance Spectroscopy, Molecular Structure, Spectrum Analysis, Fluorescent Dyes chemistry, Methylamines chemistry, Rhodamines chemistry, Xanthenes chemistry

Abstract

Commercially-available sulforhodamine sulfonyl chlorides contain two isomeric monosulfonyl chlorides. Conjugates of these isomers with amines have different properties because the sulfonamide formed from one isomer can undergo ring-closure to a colorless sultam. This chemistry has been examined for a model conjugate with methylamine and for a bioconjugate with 2'(3')-O-[N-(2-aminoethyl)carbamoyl]ATP. The interaction of each isomer of the latter conjugates with myosin subfragment 1 has been characterized. Significant differences between the two isomers are observed in these interactions.

Published

2001

26. Crystal structure and functional analysis of Ras binding to its effector phosphoinositide 3-kinase gamma.

Author

Pacold ME, Suire S, Perisic O, Lara-Gonzalez S, Davis CT, Walker EH, Hawkins PT, Stephens L, Eccleston JF, and Williams RL

Subjects

Animals, Binding Sites, COS Cells, Class Ib Phosphatidylinositol 3-Kinase, Crystallography, X-Ray, Guanosine 5'-O-(3-Thiotriphosphate) chemistry, Guanosine 5'-O-(3-Thiotriphosphate) metabolism, Humans, Kinetics, Models, Molecular, Mutagenesis, Site-Directed, Neutrophils metabolism, Phosphatidylinositol 3-Kinases genetics, Protein Binding, Protein Conformation, Protein Structure, Tertiary, ras Proteins chemistry, Isoenzymes chemistry, Isoenzymes metabolism, Phosphatidylinositol 3-Kinases chemistry, Phosphatidylinositol 3-Kinases metabolism, ras Proteins metabolism

Abstract

Ras activation of phosphoinositide 3-kinase (PI3K) is important for survival of transformed cells. We find that PI3Kgamma is strongly and directly activated by H-Ras G12V in vivo or by GTPgammaS-loaded H-Ras in vitro. We have determined a crystal structure of a PI3Kgamma/Ras.GMPPNP complex. A critical loop in the Ras binding domain positions Ras so that it uses its switch I and switch II regions to bind PI3Kgamma. Mutagenesis shows that interactions with both regions are essential for binding PI3Kgamma. Ras also forms a direct contact with the PI3Kgamma catalytic domain. These unique Ras/PI3Kgamma interactions are likely to be shared by PI3Kalpha. The complex with Ras shows a change in the PI3K conformation that may represent an allosteric component of Ras activation.

Published

2000

27. Mechanism of nucleotide release from Rho by the GDP dissociation stimulator protein.

Author

Hutchinson JP and Eccleston JF

Subjects

Guanine Nucleotide Exchange Factors chemistry, Guanosine Diphosphate chemistry, Humans, Isomerism, Kinetics, Macromolecular Substances, Protein Conformation, Spectrometry, Fluorescence, ortho-Aminobenzoates chemistry, ortho-Aminobenzoates metabolism, rho GTP-Binding Proteins chemistry, rhoA GTP-Binding Protein chemistry, rhoA GTP-Binding Protein metabolism, Guanine Nucleotide Exchange Factors physiology, Guanosine Diphosphate analogs & derivatives, Guanosine Diphosphate metabolism, rho GTP-Binding Proteins metabolism

Abstract

Guanine nucleotide dissociation stimulator (GDS) promotes the release of tightly bound GDP from various Ras superfamily proteins, including RhoA, Rac1, K-Ras, Rap1A, and Rap1B. It displays no significant sequence homology to other known exchange factors for small G-proteins. Studies are reported here of the mechanism of GDS-mediated nucleotide release from RhoA using a combination of equilibrium and stopped-flow kinetic measurements, employing fluorescent N-methylanthraniloyl (mant) derivatives of GDP and 2'-deoxyGDP. It is proposed that GDS operates by an associative displacement mechanism where stimulated nucleotide release from the Rho.mantGDP complex occurs via a transiently populated ternary complex (Rho.GDS.mantGDP). In kinetic experiments where excess GDS was mixed with the Rho.mantGDP complex, stimulated mantGDP dissociation rates of 1 s(-)(1) were measured during a single turnover, representing a 5000-fold enhancement over the intrinsic rate of mantGDP dissociation from Rho. The stable, nucleotide-free binary complex Rho.GDS was isolated. When the Rho.GDS complex was mixed with excess mantGDP, a biphasic increase in fluorescence occurred, the observed rate constants of which both reached saturating values at high mantGDP concentrations. This is compelling evidence that an isomerization of the Rho.GDS.mantGDP ternary complex is an important feature of the mechanism of nucleotide release.

Published

2000

28. The mechanism of GTP hydrolysis by dynamin II: a transient kinetic study.

Author

Binns DD, Helms MK, Barylko B, Davis CT, Jameson DM, Albanesi JP, and Eccleston JF

Subjects

Animals, Binding, Competitive, Chromatography, High Pressure Liquid, Dynamins, Fluorescent Dyes, GTP Phosphohydrolases chemistry, Guanosine Diphosphate analogs & derivatives, Hydrolysis, Kinetics, Protein Binding, Protein Conformation, Rats, Ultracentrifugation, ortho-Aminobenzoates, GTP Phosphohydrolases metabolism, Guanosine Triphosphate metabolism

Abstract

Dynamin II is a 98 kDa protein (870 amino acids) required for the late stages of clathrin-mediated endocytosis. The GTPase activity of dynamin is required for its function in the budding stages of receptor-mediated endocytosis and synaptic vesicle recycling. This activity is stimulated when dynamin self-associates on multivalent binding surfaces, such as microtubules and anionic liposomes. We first investigated the oligomeric state of dynamin II by analytical ultracentrifuge sedimentation equilibrium measurements at high ionic strength and found that it was best described by a monomer-tetramer equilibrium. We then studied the intrinsic dynamin GTPase mechanism by using a combination of fluorescence stopped-flow and HPLC methods using the fluorescent analogue of GTP, mantdGTP (2'-deoxy-3'-O-(N-methylanthraniloyl) guanosine-5'-triphosphate), under the same ionic strength conditions. The results are interpreted as showing that mantdGTP binds to dynamin in a two-step mechanism. The dissociation constant of mantdGTP binding to dynamin, calculated from the ratio of the off-rate to the on-rate (k(off)/k(on)), was 0.5 microM. Cleavage of mantdGTP then occurs to mantdGDP and P(i) followed by the rapid release of mantdGDP and P(i). No evidence of reversibility of hydrolysis was observed. The cleavage step itself is the rate-limiting step in the mechanism. This mechanism more closely resembles that of the Ras family of proteins involved in cell signaling than the myosin ATPase involved in cellular motility.

Published

2000

29. Comparative single-molecule and ensemble myosin enzymology: sulfoindocyanine ATP and ADP derivatives.

Author

Oiwa K, Eccleston JF, Anson M, Kikumoto M, Davis CT, Reid GP, Ferenczi MA, Corrie JE, Yamada A, Nakayama H, and Trentham DR

Subjects

Actins metabolism, Actomyosin metabolism, Animals, Fluorescent Dyes, Kinetics, Muscle Contraction, Muscle Fibers, Skeletal physiology, Myosin Subfragments metabolism, Rabbits, Stochastic Processes, Substrate Specificity, Adenosine Diphosphate analogs & derivatives, Adenosine Diphosphate metabolism, Adenosine Triphosphate analogs & derivatives, Adenosine Triphosphate metabolism, Muscle, Skeletal physiology, Myosins metabolism

Abstract

Single-molecule and macroscopic reactions of fluorescent nucleotides with myosin have been compared. The single-molecule studies serve as paradigms for enzyme-catalyzed reactions and ligand-receptor interactions analyzed as individual stochastic processes. Fluorescent nucleotides, called Cy3-EDA-ATP and Cy5-EDA-ATP, were derived by coupling the dyes Cy3.29.OH and Cy5.29.OH (compounds XI and XIV, respectively, in, Bioconjug. Chem. 4:105-111)) with 2'(3')-O-[N-(2-aminoethyl)carbamoyl]ATP (EDA-ATP). The ATP(ADP) analogs were separated into their respective 2'- and 3'-O-isomers, the interconversion rate of which was 30[OH(-)] s(-1) (0.016 h(-1) at pH 7.1) at 22 degrees C. Macroscopic studies showed that 2'(3')-O-substituted nucleotides had properties similar to those of ATP and ADP in their interactions with myosin, actomyosin, and muscle fibers, although the ATP analogs did not relax muscle as well as ATP did. Significant differences in the fluorescence intensity of Cy3-nucleotide 2'- and 3'-O-isomers in free solution and when they interacted with myosin were evident. Single-molecule studies using total internal reflection fluorescence microscopy showed that reciprocal mean lifetimes of the nucleotide analogs interacting with myosin filaments were one- to severalfold greater than predicted from macroscopic data. Kinetic and equilibrium data of nucleotide-(acto)myosin interactions derived from single-molecule microscopy now have a biochemical and physiological framework. This is important for single-molecule mechanical studies of motor proteins.

Published

2000

30. Distances between DNA and ATP binding sites in the TyrR-DNA complex.

Author

Sawyer WH, Chan RY, Eccleston JF, Davidson BE, Samat SA, and Yan Y

Subjects

Adenosine Triphosphate metabolism, Binding Sites, DNA, Bacterial metabolism, Energy Transfer, Escherichia coli chemistry, Fluorescence Polarization, Macromolecular Substances, Models, Molecular, Oligonucleotides chemistry, Oligonucleotides metabolism, Repressor Proteins metabolism, Rhodamines chemistry, Rhodamines metabolism, Spectrometry, Fluorescence, Adenosine Triphosphate chemistry, DNA, Bacterial chemistry, Escherichia coli Proteins, Repressor Proteins chemistry

Abstract

The Escherichia coli regulatory protein TyrR controls the expression of eight transcription units that encode proteins involved in the biosynthesis and transport of aromatic amino acids. It binds to DNA as a homodimer with a subunit molecular mass of 57 640 Da, each of which has a single site for the binding of ATP within a central structural domain. This paper reports distances between four sites on the DNA and the ATP binding site as determined by fluorescence resonance energy transfer. The DNA was a 30mer containing a centrally located binding site for TyrR. Replacement of a thymidine residue with an aminouridine residue at positions -9, -7, -3, and 2 of the palindromic oligonucleotide sequence enabled the placement of a single fluorescein group along the major groove of the DNA. The energy transfer acceptor was ATP labeled with a rhodamine group through positions 2' and 3' of the ribose, positions that are known to cause minimal interference with the binding of ATP to protein. The dissociation constant for the binding of rhodamine-ATP to TyrR was 300 nM as determined by steady-state fluorescence anisotropy titrations. The energy transfer efficiencies were determined by measuring the level of quenching of donor fluorescence on binding rhodamine-ATP to the TyrR-DNA complex. The experimental transfer efficiencies were compared to theoretical values calculated for a model of the DNA-TyrR complex in which the position of the ATP binding site was allowed to vary over the surface of the monomer unit. Theory was written to account for the transfer from one donor to two acceptors, one on each monomer unit of the TyrR dimer. The results indicate that the ATP binding site is about 40-45 A from the nearest point on the DNA and distant from the DNA helix-turn-helix binding domain. The effects of ATP binding of (i) increasing the TyrR binding affinity by a factor of 4-5 and (ii) permitting the binding of the tyrosine corepressor must therefore occur because of a significant allosteric change in the conformation of the protein.

Published

2000

31. Purification and characterization of guanine nucleotide dissociation stimulator protein.

Author

Hutchinson JP, Rittinger K, and Eccleston JF

Subjects

Flow Injection Analysis, Guanine Nucleotide Exchange Factors genetics, Guanosine Diphosphate analogs & derivatives, Guanosine Diphosphate metabolism, Protein Binding, Recombinant Fusion Proteins metabolism, Sequence Analysis, Protein, rho GTP-Binding Proteins metabolism, Guanine Nucleotide Exchange Factors metabolism

Published

2000

32. Magnesium fluoride-dependent binding of small G proteins to their GTPase-activating proteins.

Author

Graham DL, Eccleston JF, Chung CW, and Lowe PN

Subjects

Aluminum metabolism, Guanosine Diphosphate metabolism, Kinetics, Magnesium Chloride pharmacology, Magnetic Resonance Spectroscopy, Neurofibromin 1, Protein Binding, Protein Conformation, Proteins metabolism, Sodium Fluoride pharmacology, X-Ray Diffraction, ras Proteins metabolism, rhoB GTP-Binding Protein metabolism, Fluorides metabolism, GTPase-Activating Proteins metabolism, Magnesium Compounds metabolism, Monomeric GTP-Binding Proteins metabolism

Abstract

GTPase-activating proteins (GAPs) enhance the intrinsic GTPase activity of small G proteins, such as Ras and Rho, by contributing a catalytic arginine to the active site. An intramolecular arginine plays a similar role in heterotrimeric G proteins. Aluminum fluoride activates the GDP form of heterotrimeric G proteins, and enhances binding of the GDP form of small G proteins to their GAPs. The resultant complexes have been interpreted as analogues of the transition state of the hydrolytic reaction. Here, equilibrium binding has been measured using scintillation proximity assays to provide quantitative information on the fluoride-mediated interaction of Ras and Rho proteins with their respective GAPs, neurofibromin (NF1) and RhoGAP. High-affinity fluoride-mediated complex formation between Rho.GDP and RhoGAP occurred in the absence of aluminum; however, under these conditions, magnesium was required. Additionally, the novel observation was made of magnesium-dependent, fluoride-mediated binding of Ras.GDP to NF1 in the absence of aluminum. Aluminum was required for complex formation when the concentration of magnesium was low. Thus, either aluminum fluoride or magnesium fluoride can mediate the high-affinity binding of Rho. GDP or Ras.GDP to GAPs. It has been reported that magnesium fluoride can activate heterotrimeric G proteins. Thus, magnesium-dependent fluoride effects might be a general phenomenon with G proteins. Moreover, these data suggest that some protein.nucleotide complexes previously reported to contain aluminum fluoride may in fact contain magnesium fluoride.

Published

1999

33. Correlation between self-association modes and GTPase activation of dynamin.

Author

Binns DD, Barylko B, Grichine N, Atkinson MA, Helms MK, Jameson DM, Eccleston JF, and Albanesi JP

Subjects

Animals, Brain enzymology, Cattle, Dose-Response Relationship, Drug, Dynamins, Kinetics, Microtubules metabolism, Models, Biological, Sodium Chloride pharmacology, Time Factors, Tubulin metabolism, Ultracentrifugation, GTP Phosphohydrolases metabolism

Abstract

The GTPase activity of dynamin is obligatorily coupled, by a mechanism yet unknown, to the internalization of clathrin-coated endocytic vesicles. Dynamin oligomerizes in vitro and in vivo and both its mechanical and enzymatic activities appear to be mediated by this self-assembly. In this study we demonstrate that dynamin is characterized by a tetramer/monomer equilibrium with an equilibrium constant of 1.67 x 10(17) M(-3). Stopped-flow fluorescence experiments show that the association rate constant for 2'(3')-O-N-methylanthraniloyl (mant)GTP is 7.0 x 10(-5) M(-1) s(-1) and the dissociation rate constant is 2.1 s(-1), whereas the dissociation rate constant for mantdeoxyGDP is 93 s(-1). We also demonstrate the cooperativity of dynamin binding and GTPase activation on a microtubule lattice. Our results indicate that dynamin self-association is not a sufficient condition for the expression of maximal GTPase activity, which suggests that dynamin molecules must be in the proper conformation or orientation if they are to form an active oligomer.

Published

1999

34. The conserved arginine in rho-GTPase-activating protein is essential for efficient catalysis but not for complex formation with Rho.GDP and aluminum fluoride.

Author

Graham DL, Eccleston JF, and Lowe PN

Subjects

Alanine genetics, Arginine genetics, Catalysis, GTP Phosphohydrolases genetics, GTP Phosphohydrolases metabolism, GTP-Binding Proteins genetics, Guanosine Diphosphate analogs & derivatives, Guanylyl Imidodiphosphate metabolism, Humans, Lysine genetics, Macromolecular Substances, Protein Binding genetics, Rho Factor genetics, ortho-Aminobenzoates metabolism, Aluminum Compounds metabolism, Arginine metabolism, Conserved Sequence, Fluorides metabolism, GTP-Binding Proteins metabolism, GTPase-Activating Proteins, Guanosine Diphosphate metabolism, Rho Factor metabolism

Abstract

The Rho family of small GTP-binding proteins are downregulated by an intrinsic GTPase, which is enhanced by GTPase-activating proteins (GAPs). RhoGAPs contain a single conserved arginine residue that has been proposed to be involved in catalysis. Here, the role of this arginine has been elucidated by mutagenesis followed by determination of catalytic and equilibrium binding constants using single-turnover kinetics, isothermal titration calorimetry, and scintillation proximity assays. The turnover numbers for wild-type, R282A, and R282K RhoGAPs were 5.4, 0.023, and 0.010 s-1, respectively. Thus, the function of this arginine could not be replaced by lysine or alanine. Nevertheless, the R282A mutation had a minimal effect on the binding affinity of RhoGAP for either Rho. GTP or Rho.GMPPNP, which confirms the importance of the arginine residue for catalysis as opposed to formation of the protein-protein complex. The R282A mutant RhoGAP still increased the hydrolysis rate of Rho.GTP by 160-fold, whereas the wild-type enzyme increased it by 38000-fold. We conclude that this arginine contributes half of the total reduction of activation energy of catalysis. In the presence of aluminum fluoride, the R282A mutant RhoGAP binds almost as well as the wild type to Rho.GDP, demonstrating that the conserved arginine is not required for this interaction. The affinity of wild-type RhoGAP for the triphosphate form of Rho is similar to that for Rho.GDP with aluminum fluoride. These last two observations show that this complex is not associated with the free energy changes expected for the transition state, although the Rho.GDP.AlF4-.RhoGAP complex might well be a close structural approximation.

Published

1999

35. Purine nucleoside phosphorylase: its use in a spectroscopic assay for inorganic phosphate and for removing inorganic phosphate with the aid of phosphodeoxyribomutase.

Author

Nixon AE, Hunter JL, Bonifacio G, Eccleston JF, and Webb MR

Subjects

Acyclovir pharmacology, Catalysis, Enzyme Inhibitors pharmacology, Kinetics, Phosphotransferases antagonists & inhibitors, Phosphates analysis, Phosphotransferases chemistry, Purine-Nucleoside Phosphorylase chemistry, Spectrometry, Fluorescence methods

Abstract

The kinetics of the phosphorolysis of 7-methylated guanosine analogues catalyzed by purine nucleoside phosphorylase has been analyzed to understand the use of this system as a "Pi mop" to remove Pi from solutions and as a spectroscopic assay for Pi at micromolar concentrations. An expression system was developed for the phosphorylase from Escherichia coli: this protein (subunit molecular mass 26 kDa) and one from a commercial source (29 kDa) were used in this study. Rates of >50 s-1 were obtained for the phosphorolysis at 30 degrees C, so that when the phosphorylase is coupled to the phosphatase being studied, rates of Pi release from the phosphatase can be measured close to this rate. The kinetic mechanism appears to obey the Michaelis-Menten model in the steady state with the bond cleavage rate limiting. Slow hydrolysis of ribose-1-phosphate to Pi catalyzed by the phosphorylase limits the efficiency of the Pi mop. To overcome this, phosphodeoxyribomutase was used to catalyze the conversion of ribose-1-phosphate to ribose-5-phosphate, enabling the Pi mop to remove large amounts of Pi quantitatively. Acyclovir diphosphate provides a simple method to switch off the Pi mop as it is a tight inhibitor (Kd 12 nM) of purine nucleoside phosphorylase., (Copyright 1998 Academic Press.)

Published

1998

36. The importance of two conserved arginine residues for catalysis by the ras GTPase-activating protein, neurofibromin.

Author

Sermon BA, Lowe PN, Strom M, and Eccleston JF

Subjects

Amino Acid Sequence, Base Sequence, Binding Sites, Catalysis, Conserved Sequence, DNA Primers, GTPase-Activating Proteins, Humans, Kinetics, Mutagenesis, Site-Directed, Neurofibromin 1, Point Mutation, Polymerase Chain Reaction, Recombinant Proteins chemistry, Recombinant Proteins metabolism, ras GTPase-Activating Proteins, Arginine, Proteins chemistry, Proteins metabolism

Abstract

Ras proteins are guanine-nucleotide binding proteins that have a low intrinsic GTPase activity that is enhanced 10(5)-fold by the GTPase-activating proteins (GAPs) p120-GAP and neurofibromin. Comparison of the primary sequences of RasGAPs shows two invariant arginine residues (Arg1276 and Arg1391 of neurofibromin). In this study, site-directed mutagenesis was used to change each of these residues in the catalytic domain of neurofibromin (NF1-334) to alanine. The ability of the mutant proteins to bind to Ras.GTP and to stimulate their intrinsic GTPase rate was then determined by kinetic methods under single turnover conditions using a fluorescent analogue of GTP. The separate contributions of each of these residues to catalysis and binding affinity to Ras were measured. Both the R1276A and the R1391A mutant NF1-334 proteins were 1000-fold less active than wild-type NF1-334 in activating the GTPase when measured at saturating concentrations. In contrast, there was only a minor effect of either mutation on NF1-334 affinity for wild-type Ha-Ras. These data are consistent with both arginines being required for efficient catalysis. Neither arginine is absolutely essential, because the mutant NF1-334 proteins increase the intrinsic Ras.GTPase by at least 100-fold. The roles of Arg1276 and Arg1391 in neurofibromin are consistent with proposals based on the recently published x-ray structure of p120-GAP complexed with Ras.

Published

1998

37. Structure at 1.65 A of RhoA and its GTPase-activating protein in complex with a transition-state analogue.

Author

Rittinger K, Walker PA, Eccleston JF, Smerdon SJ, and Gamblin SJ

Subjects

Arginine chemistry, Cell Cycle Proteins chemistry, Crystallography, X-Ray, Enzyme Activation, GTP Phosphohydrolases chemistry, GTP-Binding Proteins genetics, Hydrogen Bonding, Hydrolysis, Models, Molecular, Mutation, Protein Conformation, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, cdc42 GTP-Binding Protein, rhoA GTP-Binding Protein, GTP-Binding Proteins chemistry, GTPase-Activating Proteins

Abstract

Small G proteins of the Rho family, which includes Rho, Rac and Cdc42Hs, regulate phosphorylation pathways that control a range of biological functions including cytoskeleton formation and cell proliferation. They operate as molecular switches, cycling between the biologically active GTP-bound form and the inactive GDP-bound state. Their rate of hydrolysis of GTP to GDP by virtue of their intrinsic GTPase activity is slow, but can be accelerated by up to 10(5)-fold through interaction with rhoGAP, a GTPase-activating protein that stimulates Rho-family proteins. As such, rhoGAP plays a crucial role in regulating Rho-mediated signalling pathways. Here we report the crystal structure of RhoA and rhoGAP complexed with the transition-state analogue GDP.AlF4- at 1.65 A resolution. There is a rotation of 20 degrees between the Rho and rhoGAP proteins in this complex when compared with the ground-state complex Cdc42Hs.GMPPNP/rhoGAP, in which Cdc42Hs is bound to the non-hydrolysable GTP analogue GMPPNP. Consequently, in the transition state complex but not in the ground state, the rhoGAP domain contributes a residue, Arg85(GAP) directly into the active site of the G protein. We propose that this residue acts to stabilize the transition state of the GTPase reaction. RhoGAP also appears to function by stabilizing several regions of RhoA that are important in signalling the hydrolysis of GTP.

Published

1997

38. Crystal structure of a small G protein in complex with the GTPase-activating protein rhoGAP.

Author

Rittinger K, Walker PA, Eccleston JF, Nurmahomed K, Owen D, Laue E, Gamblin SJ, and Smerdon SJ

Subjects

Arginine chemistry, Crystallography, X-Ray, Enzyme Activation, GTP Phosphohydrolases metabolism, Guanosine Triphosphate analogs & derivatives, Guanosine Triphosphate chemistry, Models, Molecular, Protein Conformation, cdc42 GTP-Binding Protein, Cell Cycle Proteins chemistry, GTP-Binding Proteins chemistry, GTPase-Activating Proteins

Abstract

Small G proteins transduce signals from plasma-membrane receptors to control a wide range of cellular functions. These proteins are clustered into distinct families but all act as molecular switches, active in their GTP-bound form but inactive when GDP-bound. The Rho family of G proteins, which includes Cdc42Hs, activate effectors involved in the regulation of cytoskeleton formation, cell proliferation and the JNK signalling pathway. G proteins generally have a low intrinsic GTPase hydrolytic activity but there are family-specific groups of GTPase-activating proteins (GAPs) that enhance the rate of GTP hydrolysis by up to 10(5) times. We report here the crystal structure of Cdc42Hs, with the non-hydrolysable GTP analogue GMPPNP, in complex with the GAP domain of p50rhoGAP at 2.7A resolution. In the complex Cdc42Hs interacts, mainly through its switch I and II regions, with a shallow pocket on rhoGAP which is lined with conserved residues. Arg 85 of rhoGAP interacts with the P-loop of Cdc42Hs, but from biochemical data and by analogy with the G-protein subunit G(i alpha1), we propose that it adopts a different conformation during the catalytic cycle which enables it to stabilize the transition state of the GTP-hydrolysis reaction.

Published

1997

39. Characterisation of the interaction of normal and mutant Rho-GAP with Rho family proteins.

Author

Graham DL, Eccleston JF, and Lowe PN

Subjects

Amino Acid Sequence, Arginine, Conserved Sequence, GTP Phosphohydrolases chemistry, GTPase-Activating Proteins, Guanosine Triphosphate metabolism, Kinetics, Mutagenesis, Site-Directed, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Sequence Alignment, Sequence Homology, Amino Acid, rac GTP-Binding Proteins, GTP Phosphohydrolases metabolism, GTP-Binding Proteins metabolism, Proteins chemistry, Proteins metabolism

Published

1997

40. Cloning and characterization of a rhoGAP homolog from Dictyostelium discoideum.

Author

Ludbrook SB, Eccleston JF, and Strom M

Subjects

Amino Acid Sequence, Animals, Cloning, Molecular, Dictyostelium, GTP-Binding Proteins chemistry, Humans, Molecular Sequence Data, Molecular Weight, Sequence Alignment, Substrate Specificity, src Homology Domains, GTP-Binding Proteins genetics, GTPase-Activating Proteins

Abstract

Small GTPases interact with a variety of proteins that affect nucleotide binding and cleavage. GTPase activating proteins (GAPs) are one class of these proteins that act by accelerating the intrinsic GTPase rate resulting in the formation of the biologically inactive GDP-bound form of the GTPase. For the Rho subfamily of GTPases, there is a growing number of proteins with rhoGAP activity that are identifiable by a homologous region of about 150 amino acids. We have exploited this homology using the polymerase chain reaction to clone the first rhoGAP homolog, called DdRacGAP, from the slime mold Dictyostelium discoideum. The GAP domain of DdRacGAP (amino acids 1-212), when expressed and purified from Escherichia coli, is active on both Dictyostelium and human Rho family GTPases but not human Ras. The full-length protein is 1356 amino acids in length and has several interesting homologies in addition to the GAP domain, including an SH3 domain, a dbl homology domain, and a pleckstrin homology domain.

Published

1997

41. The structure of the GTPase-activating domain from p50rhoGAP.

Author

Barrett T, Xiao B, Dodson EJ, Dodson G, Ludbrook SB, Nurmahomed K, Gamblin SJ, Musacchio A, Smerdon SJ, and Eccleston JF

Subjects

Amino Acid Sequence, Binding Sites, Crystallography, X-Ray, Enzyme Activation, Humans, Models, Molecular, Molecular Sequence Data, Sequence Homology, Amino Acid, GTP Phosphohydrolases metabolism, GTP-Binding Proteins chemistry, GTPase-Activating Proteins, Protein Conformation

Abstract

Members of the Rho family of small G proteins transduce signals from plasma-membrane receptors and control cell adhesion, motility and shape by actin cytoskeleton formation. They also activate other kinase cascades. Like all other GTPases, Rho proteins act as molecular switches, with an active GTP-bound form and an inactive GDP-bound form. The active conformation is promoted by guanine-nucleotide exchange factors, and the inactive state by GTPase-activating proteins (GAPs) which stimulate the intrinsic GTPase activity of small G proteins. Rho-specific GAP domains are found in a wide variety of large, multi-functional proteins. Here we report the crystal structure of an active 242-residue C-terminal fragment of human p50rhoGAP. The structure is an unusual arrangement of nine alpha-helices, the core of which includes a four-helix bundle. Residues conserved across the rhoGAP family are largely confined to one face of this bundle, which may be an interaction site for target G proteins. In particular, we propose that Arg 85 and Asn 194 are involved in binding G proteins and enhancing GTPase activity.

Published

1997

42. Fluorescent nucleotide analogs: synthesis and applications.

Author

Jameson DM and Eccleston JF

Subjects

Animals, Fluorescence, Fluorescent Dyes chemical synthesis, Humans, Nucleotides chemical synthesis, Fluorescent Dyes chemistry, Nucleotides chemistry

Published

1997

43. Role of guanine nucleotide-binding proteins--ras-family or trimeric proteins or both--in Ca2+ sensitization of smooth muscle.

Author

Gong MC, Iizuka K, Nixon G, Browne JP, Hall A, Eccleston JF, Sugai M, Kobayashi S, Somlyo AV, and Somlyo AP

Subjects

Animals, Carbachol pharmacology, Cell Line, Cell Membrane Permeability, Cloning, Molecular, Endothelins pharmacology, Enterotoxins pharmacology, GTP-Binding Proteins biosynthesis, GTP-Binding Proteins isolation & purification, Guanosine 5'-O-(3-Thiotriphosphate) pharmacology, Guanosine Triphosphate pharmacology, Ileum, In Vitro Techniques, Mesenteric Arteries drug effects, Mesenteric Arteries physiology, Muscle, Smooth drug effects, Muscle, Smooth, Vascular drug effects, Pertussis Toxin, Phenylephrine pharmacology, Rabbits, Recombinant Proteins biosynthesis, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Spodoptera, Staphylococcus aureus, Virulence Factors, Bordetella pharmacology, rhoA GTP-Binding Protein, Calcium pharmacology, GTP-Binding Proteins metabolism, Muscle, Smooth physiology, Muscle, Smooth, Vascular physiology

Abstract

The purpose of this study was to identify guanine nucleotide-binding proteins (G proteins) involved in the agonist- and guanosine 5'-[gamma-thio]triphosphate (GTP[gamma-S])-induced increase in the Ca2+ sensitivity of 20-kDa myosin light chain (MLC20) phosphorylation and contraction in smooth muscle. A constitutively active, recombinant val14p21rhoA.GTP expressed in the baculovirus/Sf9 system, but not the protein expressed without posttranslational modification in Escherichia coli, induced at constant Ca2+ (pCa 6.4) a slow contraction associated with increased MLC20 phosphorylation from 19.8% to 29.5% (P < 0.05) in smooth muscle permeabilized with beta-esein. The effect of val14p21rhoA.GTP was inhibited by ADP-ribosylation of the protein and was absent in smooth muscle extensively permeabilized with Triton X-100. ADP-ribosylation of endogenous p21rho with epidermal cell differentiation inhibitor (EDIN) inhibited Ca2+ sensitization induced by GTP [in rabbit mesenteric artery (RMA) and rabbit ileum smooth muscles], by carbachol (in rabbit ileum), and by endothelin (in RMA), but not by phenylephrine (in RMA), and only slowed the rate without reducing the amplitude of contractions induced in RMA by 1 microM GTP[gamma-S] at constant Ca2+ concentrations. AlF(4-)-induced Ca2+ sensitization was inhibited by both guanosine 5'-[beta-thio]diphosphate (GDP[beta-S]) and by EDIN. EDIN also inhibited, to a lesser extent, contractions induced by Ca2+ alone (pCa 6.4) in both RMA and rabbit ileum. ADP-ribosylation of trimeric G proteins with pertussis toxin did not inhibit Ca2+ sensitization. We conclude that p21rho may play a role in physiological Ca2+ sensitization as a cofactor with other messengers, rather than as a sole direct inhibitor of smooth muscle MLC20 phosphatase.

Published

1996

44. Mechanism of inhibition by arachidonic acid of the catalytic activity of Ras GTPase-activating proteins.

Author

Sermon BA, Eccleston JF, Skinner RH, and Lowe PN

Subjects

Binding, Competitive, Catalysis, Chromatography, High Pressure Liquid, GTPase-Activating Proteins, Guanosine Diphosphate metabolism, Guanosine Triphosphate metabolism, Kinetics, Neurofibromin 1, Recombinant Fusion Proteins antagonists & inhibitors, Scintillation Counting, Signal Transduction, Spectrometry, Fluorescence, Tritium, ras GTPase-Activating Proteins, ras Proteins metabolism, Arachidonic Acid pharmacology, Proteins antagonists & inhibitors

Abstract

Ras is a guanine nucleotide-binding protein that acts as a molecular switch controlling cell growth. The Ras GTPase-activating proteins (GAPs) p120-GAP and neurofibromin are candidates as Ras effectors. The GTPase-activating activity of both proteins is inhibited by mitogenic lipids, such as arachidonic acid and phosphatidic acid, and differential inhibition of the two GAPs led to the hypothesis that both were effectors in a Ras-controlled mitogenic pathway (Bollag, G., and McCormick, F. (1991) Nature 351, 576-579). We have studied the mechanism of inhibition by arachidonic acid in three ways: first, by measurements of catalytic activity under multiple turnover conditions; second, using p-((6-phenyl)-1,3,5-hexatrienyl)benzoic acid as a fluorescent probe for ligands binding to GAPs; and third, by using a scintillation proximity assay to measure direct binding of Ras to neurofibromin. We found no significant differential inhibition between p120-GAP and neurofibromin by arachidonic acid. The inhibition by arachidonic acid included a major component that is competitive with Ras GTP. These data suggest that insomuch as the mitogenic effects of lipids are mediated via inhibition of GAPs, GAPs are not Ras effector proteins. Additionally, lipids can exert a non-competitive type effect, consistent with a protein denaturing activity, making difficult extrapolations from in vitro data to the situation within cells, and possibly explaining the variability of literature data on inhibition by lipids.

Published

1996

45. Macromolecular arrangement in the aminoacyl-tRNA.elongation factor Tu.GTP ternary complex. A fluorescence energy transfer study.

Author

Watson BS, Hazlett TL, Eccleston JF, Davis C, Jameson DM, and Johnson AE

Subjects

Fluorescence Polarization, Guanosine Triphosphate analogs & derivatives, Macromolecular Substances, Models, Chemical, Molecular Conformation, Rhodamines, Spectrometry, Fluorescence, Energy Transfer, Guanosine Triphosphate chemistry, Peptide Elongation Factor Tu chemistry, RNA, Transfer, Amino Acyl chemistry

Abstract

The distance between the corner of the L-shaped transfer RNA and the GTP bound to elongation factor Tu (EF-Tu) in the aminoacyl-tRNA.EF-Tu.GTP ternary complex was measured using fluorescence energy transfer. The donor dye, fluorescein (Fl), was attached covalently to the 4-thiouridine base at position 8 of tRNAPhe, and aminoacylation yielded Phe-tRNAPhe-Fl8. The ribose of GTP was covalently modified at the 2'(3') position with the acceptor dye rhodamine (Rh) to form GTP-Rh. Formation of the Phe-tRNAPhe-Fl8.EF-Tu.GTP-Rh ternary complex was verified both by EF-Tu protection of the aminoacyl bond from chemical hydrolysis and by an EF-Tu.GTP-dependent increase in fluorescein intensity. Spectral analyses revealed that both the emission intensity and lifetime of fluorescein were greater in the Phe-tRNAPhe-Fl8.EF-Tu.GTP ternary complex than in the Phe-tRNAPhe-Fl8.EF-Tu.GTP-Rh ternary complex. These spectral differences disappeared when excess GTP was added to replace GTP-Rh in the latter ternary complex, thereby showing that excited-state energy was transferred from fluorescein to rhodamine in the ternary complex. The efficiency of singlet-singlet energy transfer was low (10-12%), corresponding to a distance between the donor and acceptor dyes in the ternary complex of 70 +/- 7 A, where the indicated uncertainty reflects the uncertainty in dye orientation. After correction for the lengths of the probe attachment tethers, the 2'(3')-oxygen of the GTP ribose and the sulfur in the s4U are separated by a minimum of 49 A. This large distance limits the possible arrangements of the EF-Tu and the tRNA in the ternary complex.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1995

46. Kinetics of interaction between normal and proline 12 Ras and the GTPase-activating proteins, p120-GAP and neurofibromin. The significance of the intrinsic GTPase rate in determining the transforming ability of ras.

Author

Eccleston JF, Moore KJ, Morgan L, Skinner RH, and Lowe PN

Subjects

GTPase-Activating Proteins, Glycine genetics, Glycine metabolism, Guanosine Triphosphate metabolism, Humans, Hydrolysis, Kinetics, Mutation, Neurofibromin 1, Osmolar Concentration, Proline genetics, Proline metabolism, ras GTPase-Activating Proteins, Cell Transformation, Neoplastic genetics, GTP Phosphohydrolases metabolism, Genes, ras, Proteins metabolism

Abstract

Single turnover and equilibrium binding measurements on the interaction of Gly-12 and Pro-12 Ras.GTP with the catalytic domains of the GTPase-activating proteins, p120-GAP and neurofibromin, have been made utilizing fluorescent 2'(3')O-(N-methylanthraniloyl)-nucleotides. These have enabled the equilibrium dissociation constants (Kd) for their initial binding and the rate constants of the hydrolysis step to be measured. p120-GAP binds to both Ras proteins with a Kd of 17 microM, whereas neurofibromin binds to both Ras proteins with a Kd of 1 microM. Both p120-GAP and neurofibromin increased the rate constant of the GTP hydrolysis step of Pro-12 Ras, but the maximal activation at 30 degrees C was 120-fold and 560-fold, as compared with 70,000- and 52,000-fold, with Gly-12 Ras. The affinity with which p120-GAP and neurofibromin binds to either Gly-12 or Pro-12 Ras protein was decreased dramatically by increasing ionic strength caused by addition of NaCl. The rate constant of the cleavage step of hydrolysis catalyzed by neurofibromin increases with increasing ionic strength, whereas that catalyzed by p120-GAP appears to be unaffected. The high ionic strength within the cell might result in a much lower overall GTPase-activating protein activity than is measured under conditions of low ionic strength in vitro, with p120-GAP being more severely inhibited. The GTP hydrolysis rate of Pro-12 Ras is 2-fold faster than that of normal Ras. The low oncogenicity of Pro-12 ras is explained by a model in which the intrinsic rates of hydrolysis and exchange, as well as GTPase-activating protein- and exchange factor-stimulated rates, are determinants of the biological activity of Ras proteins in fibroblasts.

Published

1993

47. Conformational differences between complexes of elongation factor Tu studied 19F-NMR spectroscopy.

Author

Eccleston JF, Molloy DP, Hinds MG, King RW, and Feeney J

Subjects

Aurodox chemistry, Aurodox metabolism, Guanosine Diphosphate chemistry, Guanosine Diphosphate metabolism, Guanosine Triphosphate chemistry, Guanosine Triphosphate metabolism, Magnetic Resonance Spectroscopy, Peptide Elongation Factor Tu isolation & purification, Peptide Elongation Factor Tu metabolism, Peptide Elongation Factors chemistry, Peptide Elongation Factors metabolism, Protein Conformation, Tyrosine metabolism, X-Ray Diffraction, Escherichia coli metabolism, Peptide Elongation Factor Tu chemistry

Abstract

An analogue of elongation factor Tu (EF-Tu) from Escherichia coli was prepared by biosynthetic incorporation of 3-fluorotyrosine. The 19F-NMR spectra of the binary complexes of this protein with GDP, GTP and elongation factor Ts (EF-Ts) and the ternary complexes EF-Tu.GDP.aurodox and EF-Tu.GDP.EF-Ts were measured. EF-Tu contains ten tyrosine residues and all of the complexes studied gave complex 19F spectra with overlapping resonances. EF-Tu.GDP gave a spectrum in which two signals were markedly different from those shown by the other complexes, the two resonances being shifted downfield by at least 3.4 ppm and 0.9 ppm relative to their shifts in the other complexes. Such large downfield shifts can be explained by second-order electric field shielding effects resulting from these two tyrosine residues being in a sterically constrained environment in EF-Tu.GDP and with the steric restraints being released in all of the other complexes. The X-ray diffraction structure of EF-Tu.GDP shows that Tyr87 in the N-terminal domain (domain I) and Tyr309 in the C-terminal domain (domain III) are both buried within the protein and are close to each other: these residues are in regions of EF-Tu previously implicated in the structural changes between EF-Tu.GDP and EF-Tu.GTP by other workers. If these tyrosine residues correspond to the two downfield resonances of the spectra of EF-Tu.GDP, the results from the 19F-NMR would be consistent with these earlier indications that domain I interacts closely with domain III in EF-Tu.GDP and that the amino acids between Gly83 and Gly100 are an important part of this interaction. For all the other complexes studied, these tyrosines are in a less sterically crowded environment consistent with a weaker interaction between the two domains. The 19F-NMR spectrum of the trypsin-cleaved product of EF-Tu.GDP, from which the X-ray diffraction structural data have been obtained, shows no significant differences from the native protein so that trypsin cleavage causes no large changes in the protein's structure.

Published

1993

48. Solution dynamics of p21ras proteins bound with fluorescent nucleotides: a time-resolved fluorescence study.

Author

Hazlett TL, Moore KJ, Lowe PN, Jameson DM, and Eccleston JF

Subjects

Chemical Phenomena, Chemistry, Physical, Chromatography, Gel, Coumarins, Deoxyguanine Nucleotides, Fluorescein-5-isothiocyanate, Fluorescence, Fluorescence Polarization, Guanosine Diphosphate analogs & derivatives, Guanosine Triphosphate analogs & derivatives, Macromolecular Substances, Proto-Oncogene Proteins p21(ras) metabolism, Rotation, Solutions, Spectrometry, Fluorescence, Time Factors, Fluorescent Dyes, Guanosine Diphosphate metabolism, Guanosine Triphosphate metabolism, Proto-Oncogene Proteins p21(ras) chemistry

Abstract

The solution dynamics of normal and transforming p21ras proteins in both the GTP- and GDP-bound forms were examined with time-resolved fluorescence spectroscopy. The fluorescent 2'(3')-O-(N-methylanthraniloyl) derivatives (mant derivatives) of GTP, dGTP, and GDP and the aminocoumarin and fluorescein derivatives of GTP and GDP were synthesized and used as reporter groups. The fluorescence lifetimes at 5 degrees C of the mant nucleotide derivatives increased from approximately 4 ns in solution to approximately 9 ns when bound to p21ras. At 30 degrees C, there was a 7.8% difference in lifetime between normal p21ras.mantGTP and p21ras.mantGDP, but no difference between similar complexes of the [Asp-12]p21ras protein. These data are consistent with steady-state fluorescence intensity differences among p21ras.mantGTP, p21ras.mantGDP, and the free nucleotides. Rotational correlation times for the mantGTP- and mantGDP-bound p21 proteins, N-ras, K-ras, and H-ras, were similar at 26 ns (5 degrees C), which is significantly longer than the 15-ns rotational correlation time predicted for a globular 21,000-Da protein. The p21-bound fluorescein and aminocoumarin nucleotide derivatives reported correlation times of 19 and 29 ns, respectively. Global analysis of the three fluorophore.p21 complexes with linked protein rotational correlation functions were best fit with a common rotational correlation time of 28 ns. Gel permeation chromatography of the GDP and mantGDP complexes of normal p21N-ras also showed greater apparent molecular weights than were expected in both cases, demonstrating that the high rotational correlation times obtained from time-resolved fluorescence measurements were not a result of the introduction of the fluorophore.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1993

49. Mechanism of GTP hydrolysis by p21N-ras catalyzed by GAP: studies with a fluorescent GTP analogue.

Author

Moore KJ, Webb MR, and Eccleston JF

Subjects

Chromatography, Gel, Escherichia coli, Fluorescent Dyes, GTP Phosphohydrolases metabolism, GTPase-Activating Proteins, Guanosine Diphosphate metabolism, Guanylyl Imidodiphosphate metabolism, Hydrolysis, Kinetics, Osmolar Concentration, Spectrometry, Fluorescence, ortho-Aminobenzoates metabolism, ras GTPase-Activating Proteins, Guanosine Triphosphate metabolism, Proteins metabolism, Proto-Oncogene Proteins p21(ras) metabolism

Abstract

The mechanism of the hydrolysis of GTP by p21N-ras and its activation by the catalytic domain of p120 GTPase activating protein (GAP) have been studied using a combination of chemical and fluorescence measurements with the fluorescent GTP analogue, 2'(3')-O-(N-methylanthraniloyl)GTP (mantGTP). Since the concentration of active p21 is important in these measurements, various assays for both total protein and active p21 were investigated. All assays gave good agreement except the filter binding assay of [3H]-GDP bound to p21, which gave values of 35-40% compared to the other methods. Concentrations of p21 were thus based on the absorbance of the mant-chromophore of the p21-mant-nucleotide complexes. The rate constants of the elementary steps of the p21 intrinsic GTPase activity and the GAP activated activity were similar between GTP and mantGTP. Incubation of a stoichiometric complex of p21.mantGTP results in a biphasic decrease in fluorescence. The second phase occurs with the same rate constant as the cleavage step and is accelerated by GAP. No other steps of the mechanism are affected by GAP. Incubation of a stoichiometric complex of p21.mantGpp[NH]p also results in a biphasic decrease in fluorescence even though cleavage does not occur. This is interpreted that the cleavage step of p21.GTP is preceded by and controlled by an isomerization of the p21.GTP complex. GAP accelerates the rate constant of the second fluorescence phase occurring with p21.mantGpp[NH]p. This result shows that GAP accelerates the proposed isomerization which limits GTP cleavage rather than the cleavage step itself.

Published

1993

50. The kinetic mechanism of the GAP-activated GTPase of p21 ras.

Author

Moore KJ, Lowe PN, and Eccleston JF

Subjects

GTP Phosphohydrolases chemistry, GTPase-Activating Proteins, Guanine Nucleotides metabolism, Kinetics, Oncogene Protein p21(ras) chemistry, Protein Conformation, Proteins metabolism, ras GTPase-Activating Proteins, GTP Phosphohydrolases metabolism, Oncogene Protein p21(ras) metabolism

Abstract

Guanine nucleotides modified by acetylation of the ribose moiety with the small fluorophore N-methylanthranilic acid(mant) have been shown to bind to p21 ras with similar equilibrium and kinetic rate constants as the parent nucleotides. Hydrolysis of p21.mantGTP to p21.mantGDP results in a 10% decrease in fluorescence intensity occurring at the same rate as the cleavage step. A similar process occurs with the non-hydrolysable analogue mantGMP.PNP, and this has led to the proposal that a conformational change of p21.mantGTP precedes and controls the rate of the cleavage step. The fluorescence change with p21.mantGMP.PNP is accelerated in the presence of the C-terminal catalytic domain of GAP, which is consistent with this mechanism. The same conformational change does not occur with oncogenic mutants of p21 ras, Asp-12 and Val-12, but does occur with the weakly oncogenic Pro-12 mutant. Stopped flow measurements of the interaction of GAP with p21.mantGTP show an exponential decrease in fluorescence, the rate of which does not vary linearly with GAP concentration. These data imply a rapidly reversible formation of the p21.mantGTP complex with GAP followed by the isomerization of this complex. This is at least 10(5)-fold faster than the same process in the absence of GAP.

Published

1992