Selection of Carbonic Anhydrase Variants Displayed on Phage

Hunt, Jennifer A.; Fierke, Carol A.

doi:10.1074/jbc.272.33.20364

Cited by 70 publications

(44 citation statements)

References 63 publications

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“…If these observed rates of CadC-metal encounter complex formation reflect true bimolecular rate constants, they are equal to, or orders of magnitude larger, than those reported for other metalloproteins, including Bacillus cereus b-lactamase (10 7 M À1 s À1 for Zn(II)) [45], Zn(II) E9 endonuclease (10 6 M À1 s À1 ) [28], Mn(II) FosA (3 · 10 5 M À1 s À1 ) [27], Bi(III)-transferrin (2 · 10 5 M À1 s À1 ) [46], Zn(II) carbonic anhydrase (10 5 M À1 s À1 ) [47] and Cu(II)-azurin (2.2 · 10 3 M À1 s À1 ) [37]. Although rapid, k obs1 for Pb(II)-CadC complex is slower than association rate constant for the binding of Zn(II) to reduced glutathione [48].…”

Section: The Role Of Kinetics In Metal Regulationmentioning

confidence: 99%

Kinetics of metal binding by the toxic metal-sensing transcriptional repressor Staphylococcus aureus pI258 CadC

Busenlehner

Giedroc

2006

Journal of Inorganic Biochemistry

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Section: The Role Of Kinetics In Metal Regulationmentioning

confidence: 99%

Kinetics of metal binding by the toxic metal-sensing transcriptional repressor Staphylococcus aureus pI258 CadC

Busenlehner

Giedroc

2006

Journal of Inorganic Biochemistry

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“…187 Fierke and co-workers conducted a series of studies in which they measured the affinities of different metals to HCA II and its active site mutants to determine the basis of selectivity for zinc in this protein. 251,311,321,322 The investigators looked at the influence of hydrophobic core residues Phe93, Phe95, and Trp97 on binding of metals and found that substitution of those residues with smaller side chains reduced the affinity of the protein to Zn II and Co II but increased the affinity to Cu II . 311,321 X-ray analysis of the mutants revealed new cavities formed in the core of the protein and shifts in the positions of metal-coordinating His94 and secondshell ligand Gln92.…”

Section: Metalloenzyme Variantsmentioning

confidence: 99%

“…251,311,321,322 The investigators looked at the influence of hydrophobic core residues Phe93, Phe95, and Trp97 on binding of metals and found that substitution of those residues with smaller side chains reduced the affinity of the protein to Zn II and Co II but increased the affinity to Cu II . 311,321 X-ray analysis of the mutants revealed new cavities formed in the core of the protein and shifts in the positions of metal-coordinating His94 and secondshell ligand Gln92. 251 The investigators concluded that the aromatic residues, although they do not directly coordinate the metal, preorient the metal-binding side chains in such a fashion as to favor tetrahedral zinc-binding geometry and to destabilize alternative geometries.…”

Section: Metalloenzyme Variantsmentioning

confidence: 99%

Carbonic Anhydrase as a Model for Biophysical and Physical-Organic Studies of Proteins and Protein−Ligand Binding

et al. 2008

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I. Introduction to Carbonic Anhydrase (CA) and to the Review 948 1. Introduction: Overview of CA as a Model 948 1.1. Value of Models 950 1.2. Objectives and Scope of the Review 950 2. Overview of Enzymatic Activity 950 3. Medical Relevance 951 II. Structure and Structure−Function Relationships of CA 953 4. Global and Active-Site Structure 953 4.1. Structure of Isoforms 953 4.2. Isolation and Purification 954 4.3. Crystallization 954 4.4. Structures Determined by X-ray Crystallography and NMR 955 4.4.1. Structures Determined by X-ray Crystallography 955 4.4.2. Structure Determined by NMR 955 4.5. Global Structural Features 963 4.6. Structure of the Binding Cavity 964 4.7. Zn II -Bound Water 965 5. Metalloenzyme Variants 966 6. Structure−Function Relationships in the Catalytic Active Site of CA 968 6.1. Effects of Ligands Directly Bound to Zn II 968 6.2. Effects of Indirect Ligands 969 7. Physical-Organic Models of the Active Site of CA 969 III. Using CA as a Model to Study Protein−Ligand Binding 970 8. Assays for Measuring Thermodynamic and Kinetic Parameters for Binding of Substrates and Inhibitors 970 8.1. Overview 970 8.

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“…Ϫ1 at pH 7.0, 30°C) (20). Noteworthy, incubation of 40 M wild type Hsp33 in 2 mM TPEN showed that the apparent half-time of zinc release was only 160 Ϯ 10 min at 23°C.…”

mentioning

confidence: 99%

Redox Switch of Hsp33 Has a Novel Zinc-binding Motif

Jakob¹,

Eser²,

Bardwell³

2000

Journal of Biological Chemistry

178

166

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The chaperone activity of the heat shock protein Hsp33 is regulated by reversible disulfide bond formation. Oxidized Hsp33 is active, and reduced Hsp33 is inactive. We show that zinc binding is essential for the function of this redox switch. Our results reveal that Hps33 contains a new, high affinity (K a > 10 17 M ؊1 ), zincbinding motif in the form Cys-X-Cys-X 27-32 -Cys-X-X-Cys. All four conserved cysteines within this motif act to coordinate a single zinc atom. Experiments where reduced wild type Hsp33 is reconstituted with cobalt or cadmium demonstrate that the metal-coordinating cysteines are present as highly reactive thiolate anions. This ionization may allow for the fast and successful activation of the chaperone function of Hsp33 upon incubation in oxidizing agents.

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Selection of Carbonic Anhydrase Variants Displayed on Phage

Cited by 70 publications

References 63 publications

Kinetics of metal binding by the toxic metal-sensing transcriptional repressor Staphylococcus aureus pI258 CadC

Kinetics of metal binding by the toxic metal-sensing transcriptional repressor Staphylococcus aureus pI258 CadC

Carbonic Anhydrase as a Model for Biophysical and Physical-Organic Studies of Proteins and Protein−Ligand Binding

Redox Switch of Hsp33 Has a Novel Zinc-binding Motif

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