Carlos Garcı́a scite author profile

Factors governing the folding pathways and the stability of apomyoglobin have been examined by replacing the distal histidine at position 64 with phenylalanine (H64F). Acid and urea-induced unfolding experiments using CD and fluorescence techniques reveal that the mutant H64F apoprotein is significantly more stable than wild-type apoMb. Kinetic refolding studies of this variant also show a significant difference from wild-type apoMb. The amplitude of the burst phase ellipticity in stopped-flow CD measurements is increased over that of wild-type, an indication that the secondary structure content of the earliest kinetic intermediate is greater in the mutant than in the wild-type protein. In addition, the overall rate of folding is markedly increased. Hydrogen exchange pulse labeling was used to establish the structure of the initial intermediate formed during the burst phase of the H64F mutant. NMR analysis of the samples obtained at different refolding times indicates that the burst phase intermediate contains a stabilized E helix as well as the A, G, and H helices previously found in the wild-type kinetic intermediate. Replacement of the polar distal histidine residue with a nonpolar residue of similar size and shape appears to stabilize the E helix in the early stages of folding due to improved hydrophobic packing. The presence of a hydrophilic histidine at position 64 thus exacts a price in the stability and folding efficiency of the apoprotein, but this residue is nevertheless highly conserved among myoglobins due to its importance in function.

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Ketoconazole-induced conformational changes in the active site of cytochrome P450eryF

Cupp‐Vickery

Garcı́a

Hofacre

et al. 2001

Journal of Molecular Biology

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Quench‐flow experiments combined with mass spectrometry show apomyoglobin folds through an obligatory intermediate

et al. 1999

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Folding of apomyoglobin is characterized by formation of a compact intermediate that contains substantial helicity. To determine whether this intermediate is obligatory or whether the protein can fold directly into the native state via an alternate parallel pathway, we have combined quench-flow hydrogen-exchange pulse labeling techniques with electrospray ionization mass spectrometry. The mass spectra of apomyoglobin obtained at various refolding times suggest that apomyoglobin indeed folds through a single pathway containing an obligatory intermediate with a significant hydrogenbonded secondary structure content.

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Solution Structure of the Ribosome-binding Domain ofE. coliTranslation Initiation Factor IF3. Homology with the U1A Protein of the Eukaryotic Spliceosome

Garcı́a

Fortier

Blanquet

et al. 1995

Journal of Molecular Biology

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Carlos Garcı́a

Crystal Structure of Putidaredoxin, the [2Fe–2S] Component of the P450cam Monooxygenase System from Pseudomonas putida

Changes in the Apomyoglobin Folding Pathway Caused by Mutation of the Distal Histidine Residue

Ketoconazole-induced conformational changes in the active site of cytochrome P450eryF

Quench‐flow experiments combined with mass spectrometry show apomyoglobin folds through an obligatory intermediate

Solution Structure of the Ribosome-binding Domain ofE. coliTranslation Initiation Factor IF3. Homology with the U1A Protein of the Eukaryotic Spliceosome

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