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67 results on '"H. Taniuchi"'

1. Formation of a biologically active, ordered complex from two overlapping fragments of cytochrome c

Author

R R Hantgan and H Taniuchi

Subjects
Cytochrome, biology, Stereochemistry, Cytochrome c, Tryptophan, Cell Biology, Biochemistry, Cytochrome b2, chemistry.chemical_compound, Protein structure, chemistry, biology.protein, Cyanogen bromide, Molecular Biology, Heme, Peptide sequence
Abstract

A noncovalent complex of the apoprotein (1-104) and cyanogen bromide heme fragment containing residues 1 to 65, (1-65) H, has been prepared from horse heart cytochrome c. Conditions under which the redundant portions of the ferrous complex can be removed by limited trypsin digestion have been devised. The complementing fragments have been isolated from the derived complexes and four apofragments and one heme fragment have been identified in the amino acid sequence of cytochrome c. They are (39-104), (40-104), (54-104), (56-104), and (1-53)H. The formation of an ordered ferric complex composed of one heme fragment and one apofragment for the cases (1-53)H (39-104), (1-53)H-(40-104), (1-53)H-(54-104), and (1-53)H-(56-104) has been demonstrated by the quenching of the tryptophan 59 fluorescence and the regain of biological activity in a cytochrome b2 assay. The apparent dissociation constant has been estimated as less than 3 X 10(-7) M in all the aforementioned cases. Thus, the region (between residues 38 and 57) of the amino acid sequence permissible for cleavage without disruption of the ordered structure indicated by the present in vitro experiments corresponds to that (between residues 38 and 57) evolutionally deleted in the three-dimensional structure of Pseudomonas aeruginosa cytochrome c551 discovered by Dickerson et al. (Dickerson, R.E., Timkovich, R., and Almassy, R.J. (1976) J. Mol. Biol. 100, 473-491).

Published
1977

2. Intramolecular flip between two alternative forms of complex formed from a heme fragment and apoprotein of horse cytochrome c

Author

M A Juillerat and H Taniuchi

Subjects
chemistry.chemical_classification, education.field_of_study, biology, Stereochemistry, Cytochrome c, Kinetics, Population, Cell Biology, Biochemistry, Dissociation (chemistry), chemistry.chemical_compound, chemistry, Intramolecular force, medicine, biology.protein, Non-covalent interactions, Ferric, education, Molecular Biology, Heme, medicine.drug
Abstract

The previous studies have shown that (a) noncovalent interactions of the ferro-heme fragment of residues 1-38 and apoprotein (1-104) of horse cytochrome c simultaneously and specifically form two isomeric complexes, types I and II resembling the native protein (the redundant residues flexibly protruding from the ordered structure); (b) the type II form but not type I appears to bind to CO; and (c) residues 39-55 are more flexible for type II form than type I (Parr, G. R., and Taniuchi, H. (1981) J. Biol. Chem. 256, 125-132). In the present study, we investigated 1) kinetics and thermodynamics of interconversion between type I and II forms of complex ferro-(1-38)-H.(1-104); 2) the properties of the CO binding population; 3) the rate of dissociation of complexes ferri- and ferro-(1-38)-H.(39-104) (mimicking type II form); and 4) thermal transition of the 695-nm absorption band and biological activity of complexes. The results indicate (a) interconversion between type I and II forms of complex ferro-(1-38)-H.(1-104) occurs without going through dissociation (t1/2 less than or equal to 12 min at 10 degrees C) and is associated with delta H (= -7.2 +/- 3.7 kcal/mol at 10 degrees C) favoring type I form and delta S (= 23 +/- 13 e.u. at 10 degrees C) favoring type II; (b) the CO-binding population correlates with type II; and (c) change from the ferrous to the ferric state of heme appears to perturb the thermodynamic relationship between type I and II forms. Interpreting the results and available evidence, we suggest that "intramolecular" flip between ferro-type I and ferro-type II forms would establish the Boltzmann distribution of these two distinctly different energy states, type I form having more strengthened interatomic interactions and type II more pronounced internal motion.

Published
1987

3. A study on the role of evolutionarily invariant leucine 32 of cytochrome c

Author

H Taniuchi and M A Juillerat

Subjects
chemistry.chemical_classification, Leucine zipper, biology, Stereochemistry, Cytochrome c, Cell Biology, Biochemistry, Amino acid, Dissociation constant, chemistry.chemical_compound, chemistry, biology.protein, Isoleucine, Norvaline, Leucine, Molecular Biology, Heme
Abstract

To investigate the role of evolutionarily invariant leucine 32 of horse cytochrome c, analogs of residues 28-38, (28-38), each containing a substituted amino acid at positions 32 or 35 were synthesized using Merrifield's method. Position 35 is leucine in horse cytochrome c but replaced by nonpolar amino acids in some species. The ability of the analogs to bind to the two-fragment complex of ferri- or ferro heme fragment (1-25)H and apofragment (39-104) was measured using gel filtration and equilibrium dialysis. Replacement of leucine 32 with isoleucine, for example, increased the dissociation constant by more than 400-fold for the ferrous complex. In contrast, replacement of leucine 35 with isoleucine seems to increase it only by a small degree. Since both leucine 32 and leucine 35 are completely buried within the structure, hydrophobic interaction would not explain this striking difference. However, thermodynamic analyses and absorption spectra of the ferric complex have indicated that replacement with norvaline of leucine 32 increases both delta H and delta S (more positive) associated with formation of an intermediate three-fragment complex and decreases both delta H and delta S (more negative) associated with transformation from the intermediate to the ground state, resulting in weakening the methionine 80--S--heme-Fe bond formed in the latter step. Taking the results together with the fragment exchange studies on the ferrous complex and available evidence, we suggest that the interaction involving leucine 32 would be coupled not only with the methionine 80--S--heme-Fe bond but also with the energy state of other distant residues such as tryptophan 59, generating extra energy for modulating the binding of the complex, i.e. the force of folding. In contrast, leucine 35 would be less important even if it were involved in such coupling.

Published
1986

4. Ordered complexes of cytochrome c fragments. Kinetics of formation of the reduced (ferrous) forms

Author

H Taniuchi and G R Parr

Subjects
Sodium ascorbate, biology, Stereochemistry, Cytochrome c, Inorganic chemistry, Cell Biology, Biochemistry, Ferrous, chemistry.chemical_compound, Reaction rate constant, chemistry, Oxidation state, medicine, biology.protein, Imidazole, Ferric, Molecular Biology, Heme, medicine.drug
Abstract

The kinetics of formation of noncovalently bound ferrous complexes derived from fragments of horse heart cytochrome c have been investigated. When the reactions are initiated by combining ferrous heme fragments with an appropriate apofragment, in the presence of 50 mM imidazole, second order rate processes are observed with rate constants essentially the same as those reported with ferric heme fragments (Parr, G. R., and Taniuchi, H. (1979) J. Biol. Chem. 254, 4836-4842). An additional, probably consecutive, kinetic process is also demonstrated. If imidazole is not present in the reaction buffer, the kinetic profiles are dramatically altered. While this is partially due to aggregation (dimerization) of the ferrous heme fragments, it can nevertheless be demonstrated that the complementation reactions with apofragments are much faster than those observed with the corresponding ferric heme fragments (in the absence of imidazole). These results reflect the effect of the oxidation state of the heme iron on the folding mechanism and, thus, the manifold nature of protein folding pathways. The rate of reduction of productive ferric complexes by sodium ascorbate was investigated and biphasic reactions were found in all cases. The data indicate an equilibrium between two forms of the ferric complexes. The results of an experiment in which the complementation of ferric (1-25)H and (23-104) was carried out in the presence of sodium ascorbate indicate that the intermediate complex (Parr, G. R., and Taniuchi, H. (1980) J. Biol. Chem. 255, 8914-8918) is not reducible by ascorbate. Thus, the increase in oxidation-reduction potential occurring on formation of the productive complex from the unbound heme fragment occurs at a late stage of the overall reaction, possibly coinciding with ligation of methionine 80 to the heme iron.

Published
1981

5. Evidence of a compact structure for kinetic intermediates in the folding of a fragment complex of tuna cytochrome c

Author

H Taniuchi and G R Parr

Subjects
Reaction mechanism, biology, Cytochrome, Stereochemistry, Cytochrome c, Tryptophan, Cell Biology, Biochemistry, Residue (chemistry), Crystallography, chemistry.chemical_compound, chemistry, biology.protein, Tuna, Molecular Biology, Peptide sequence, Heme
Abstract

A noncovalently bound, ordered complex consisting of fragments (1-25)H and (14-103) derived from tuna cytochrome c has been prepared and characterized. The equilibrium properties of this complex are indistinguishable from those of the corresponding complex, (1-25)H X (23-104), of horse cytochrome c. The tuna species possesses a second tryptophan residue (at position 33 of the amino acid sequence and replacing the histidine residue of the horse protein) whose fluorescence is also essentially fully quenched in the native form and in the complex. It is found that for the tuna complex, the fluorescence of both tryptophans is fully quenched during the second order phase of the reaction mechanism. This provides evidence for the compact nature of the intermediate complexes formed at this stage of the complementation process (Parr, G. R., and Taniuchi, H. (1982) J. Biol. Chem. 257, 10103-10111). The observed second order rate constant for the tuna fragments is reduced by a factor of two from that for the horse fragments. During the first order kinetic phase corresponding to the transition from the intermediate complexes to the native complex, qualitative as well as quantitative differences are also observed between the tuna and the horse species. The kinetics of complementation of the "hybrid" complexes is also reported. This exchangeability of both the heme fragment and the apofragment of the complex between these two species indicates close similarity of the folding mechanism. Nonetheless, the results also serve to highlight the subtle effects exerted on the folding process by a relatively small number of changes (17%) in the amino acid sequence.

Published
1983

6. Kinetic intermediates in the formation of ordered complexes from cytochrome c fragments. Evidence that methionine ligation is a late event in the folding process

Author

G R Parr and H Taniuchi

Subjects
Methionine, biology, Stereochemistry, Cytochrome c, Kinetics, Tryptophan, Cell Biology, Biochemistry, Folding (chemistry), chemistry.chemical_compound, Protein structure, chemistry, medicine, biology.protein, Ferric, Molecular Biology, Heme, medicine.drug
Abstract

The reactions of ferric heme-containing fragments with apofragments to form ordered complexes resembling native horse heart cytochrome c have been studied under conditions which resolve the overall process into consecutive second order and first order kinetic steps. In the initial, second order step the two fragments combine to form an intermediate complex which exhibits tryptophan 59 fluorescence quenching similar to native cytochrome c, but which has not yet achieved the native ligation state of the heme iron. The existence of first order processes following the second order step is demonstrated by absorbance changes in the Soret region. the entire absorbance change at 695 nm, relating to ligation of the sulfur atom of methionine 80 to the heme iron, is also associated with these first order processes. Thus, ligation of methionine is a late event in this self ordering of the polypeptide chains. Since the conformational energy is assumed to distinctly decrease in this late process of folding (Parr, G.R., and Taniuchi, H. (1980) J. Biol. Chem. 255, 2616-2623), it would follow that small spatial rearrangements of the polypeptide chains in the late stage of folding (as manifested by the ligation of methionine) are associated with a specific decrease in energy.

Published
1980

10. Formation of an iso-1-cytochrome c-like species containing a covalently bonded heme group from the apoprotein by a yeast cell-free system in the presence of hemin

Author

C Di Bello, H Taniuchi, and G Basile

Subjects
biology, Autoxidation, Cytochrome, Chemistry, Stereochemistry, Cytochrome c, Cell Biology, Biochemistry, Dithiothreitol, chemistry.chemical_compound, Cytochrome b2, biology.protein, NAD+ kinase, Molecular Biology, Heme, Hemin
Abstract

Incubation of the 125I-labeled apoprotein, prepared from 125I-labeled iso-1-cytochrome c, with a yeast mitochondrial fraction in the presence of hemin, NADPH, and an extract of the postmitochondrial fraction at 32 +/- 1 degree C for 30 min has resulted in formation of cytochrome c-like species in yields of up to 35%. This radioactive synthesized species contains a functional group which responds to reduction with ascorbate and oxidation with K3Fe(CN)6 in that it is resistant in the reduced form and susceptible in the oxidized form to trypsin action in a manner characteristic of native cytochrome c. The functional group cannot be removed from the protein by cold HCl-acetone or 8 M urea treatment. The reduced form of the synthesized species exhibits resistance against autoxidation and the oxidized form can be reduced also by cytochrome b2. The synthesized species exhibits the same compact hydrodynamic volume of native cytochrome c. Treatment with silver sulfate followed by incubation with dithiothreitol converts the synthesized species to the original apoprotein as judged by an increase in the hydrodynamic volume. Thus, the synthesized species is indistinguishable from the original labeled iso-1-cytochrome c by these measurements; i.e. the synthesized species consists of the apoprotein to which heme is covalently attached through the thioether bond(s). The active factor of the mitochondrial fraction is heat-labile. The synthetic activity is strongly dependent on pH with a maximum approximately at pH 7.0. Hemin (or heme) appears to be required for this synthesis. The postmitochondrial fraction is inactive by itself. However, its addition markedly increases the synthetic activity. This factor is heat-stable, soluble in 80% methanol (or 75% ethanol), and insoluble in ethyl ether or ethyl acetate. Addition of NADP(H) (or NAD(H)) also increases the synthetic activity, the reduced form being more effective than the oxidized form. The postmitochondrial factor and the pyridine nucleotides appear to enhance the effect of each other. Thus, it seems that cytochrome c or a cytochrome c-like species is formed from the apoprotein and heme (or hemin) by an enzyme, cytochrome c synthetase, present in mitochondria.

Published
1980

12. The mechanism of stabilization of the structure of nuclease-T by binding of ligands

Author

H Taniuchi and J L Bohnert

Subjects
Nuclease T', symbols.namesake, Crystallography, Reaction rate constant, Ligand, Chemistry, Stereochemistry, symbols, Cell Biology, Molecular Biology, Biochemistry, Gibbs free energy
Abstract

The rate of unfolding of Nuclease-T at pH 8,20 degrees was determined as a function of concentration of the ligands deoxythymidine 3',5'-diphosphate (pdTp) and Ca2+ on the basis of the rate of exchange between free fragment, Nuclease-T(50-149) and labeled fragment, Nuclease-T-(50-149) incorporated in the structure of nuclease-T (Taniuchi, H. (1973) J. Biol. Chem. 248, 5164-5174). The rate constant of unfolding of unliganded Nuclease-T' was 4.6 times 10-4s-1. Those of Nuclease-T' bound with pdTp, with Ca2+, and with both pdtp and Ca2+ were 9.0 times 10-5, 1.6 times 10-4, and 2.2 times 10-5s-1, respectively. The association constants of pdTp and Ca2+ with Nuclease-T' were found to be 1.0 times 10-4 and 2.0 times 10-2 m-1, respectively. Those of pdTp with Nuclease-T' plus Ca2+ and of Ca2+ with Nuclease-T' plus pdTp were 4 times 10-5 and 1.4 times 10-4M-1, respectively. The calculation of free energy change on the basis of the association constants shows that the magnitude of negative free energy change involved in the binding of either of the two ligands increases by approximately 2 kcal when the other ligand is already bound. There is a correlation between the free energy change and the specifically coupled with the cooperative interacions operating throught the three-dimensional structure resulting in strengthening of the interactions throughtout the structure, including those with the ligands, without a large change in conformation.

Published
1975

13. A kinetic study of the formation of ordered complexes of ferric cytochrome c fragments

Author

G R Parr and H Taniuchi

Subjects
biology, Cytochrome c peroxidase, Cytochrome c, Inorganic chemistry, Cell Biology, Biochemistry, Dissociation (chemistry), Absorbance, Crystallography, chemistry.chemical_compound, Reaction rate constant, chemistry, biology.protein, Imidazole, Molecular Biology, Heme, Histidine
Abstract

The kinetics of complementation of ferric heme fragments and apofragments of horse heart cytochrome c have been investigated using stopped flow techniques. When changes in fluorescence are monitored, a single phase exhibiting second order kinetics is observed for all cases of productive complexes. The rate constants are independent of the presence of overlapping amino acid sequences in the apofragments but are strongly dependent on the amino acid sequences of the heme fragments. Thus for heme fragment (l-38)H, a rate constant of 2.1 X 10’ M-' s-l is obtained with apofragments (l-104), (23-104), and (56-104). For (l-53)H with (l-104) or (54-104), it is 1.5 X 10’ M-’ s-l. The complementation of (l-25)H with (l-104) or (23-104) results in a rate constant of 3.2 x 10’ M-’ s-l, which is greater by an order of magnitude than those for the other heme fragments. In the presence of 10 mM imidazole, the rate constants dramatically increase to 3.1 x 106, and 2.4 x lo6 M-’ s-l for heme fragments (l-38)H and (l-53)H, respectively, but only by approximately 2-fold for (l25)H. This result is attributed to a change in the axial coordination group of the heme iron atom in fragments (l-38)H and (l-53)H from histidine 33 (or 26) to an imidazole molecule, which in turn results in a major perturbation of the interactions between the heme moiety and its host peptide. When the complementation of the productive complexes is monitored by changes in the Soret absorbance, the data cannot be fit to either first order or second order kinetic equations. However, the results for a nonproductive complex ((l-25)H plus apofragment (39-104)) are identical in both absorbance and fluorescence modes. The data can be fit to an equilibrium process with a rate constant of formation of 1.3 x lo6 M-’ s-l and that of dissociation of 0.95 s-l. Thus, the formation of productive complexes appears to involve a second phase of the reaction which does not occur in the case of the nonproductive complex and which causes no additional fluorescence change but does result in further absorbance changes.

Published
1979

14. On the specificity of cytochrome c synthetase in recognition of the amino acid sequence of apocytochrome c

Author

H Taniuchi, B S Berlett, and C Visco

Subjects
chemistry.chemical_classification, Cytochrome c, Cell Biology, Biology, biology.organism_classification, Biochemistry, Molecular biology, Yeast, chemistry.chemical_compound, Enzyme, Biosynthesis, chemistry, Cytochrome C1, Candida krusei, biology.protein, Molecular Biology, Peptide sequence, Heme
Abstract

Two forms of yeast cytochrome c synthetases with different specificities were resolved, one (synthetase I), solubilized from mitochondria or the cell debris with Triton X-100, recognizing not horse apocytochrome c but yeast apo-iso-1-cytochrome c as a substrate and the other (synthetase II) still bound with the particulate fraction from mitochondria after treatment with Triton, recognizing both horse and yeast apocytochromes c. The activity with labeled yeast apo-iso-1-cytochrome c as a substrate of cytochrome c synthetase I can be quantitatively inhibited by nonlabeled Candida krusei apocytochrome c and partially by nonlabeled tuna apocytochrome c but not by nonlabeled horse apocytochrome c indicating a specific amino acid sequence being recognized. However, an enzyme similarly solubilized from beef heart mitochondria recognized both horse apocytochrome c and yeast apo-iso-1-cytochrome c for attachment of heme. In view of the fact that the yeast synthetase II and the beef synthetase can both utilize either horse apocytochrome c or yeast apo-iso-1-cytochrome c as substrates, we suggest that these enzymes may also be involved in biosynthesis of cytochrome c1, that is, the ability to attach heme to apocytochrome c and apocytochrome c1 may have been conserved in eucaryotic cells, and that both synthetases may therefore be homologous.

Published
1985

16. A study of fine specificity of monoclonal antibodies to yeast iso-1-cytochrome c

Author

I Silvestri and H Taniuchi

Subjects
Alanine, chemistry.chemical_classification, biology, Cytochrome, Stereochemistry, medicine.drug_class, Cytochrome c, Saccharomyces cerevisiae, Cell Biology, Glutamic acid, biology.organism_classification, Monoclonal antibody, Biochemistry, Amino acid, Non-competitive inhibition, chemistry, biology.protein, medicine, Molecular Biology
Abstract

Seven monoclonal antibodies, prepared to yeast holo- or apo-iso-1-cytochrome c by the method of Kohler and Milstein (Goding, J. W. (1983) Monoclonal Antibodies: Principles and Practice, Academic Press, Orlando, FL) were characterized by cross-reaction with a panel of evolutionarily related cytochromes c, apocytochromes c, fragments and homologous and hybrid fragment complexes, inhibition, competitive inhibition, and complementation and fluorescence titration. The results have permitted us to assign the specifically recognized amino acids as follows. IgG1 monoclonals: 4-74-6, Leu-63 and/or Asn-67 and/or Asn-68; 4-128-6, Glu-93; 4-145-10, Thr-74; 2-96-12, Asp-65; 2-34-19, Lys-59; and 10-28-86, trimethyl-lysine 77. IgM monoclonal 39-14, Pro-30 and His-31. With mAb 4-128-6 substitution of glutamic acid 93 with alanine, as it occurs in Candida cytochrome c, has resulted in a decrease in affinity by a factor of 10(4). A calculation appears to show that this value is too large to be accounted for solely by the sum of energy losses due to disruption of charge neutralization and changes of hydrophobic interaction including van der Waals interaction. This and similar results with mAb 10-28-86 have led us to the idea that some new extra interatomic interaction sensitive to differences in configuration of atomic groups may be present and perturbed in the substitution. Furthermore, the assumption of the presence of such interaction can explain the striking similarity between the antigen-antibody interaction (e.g. Geysen, H. M., Meloen, R. H., and Barteling, S. J. (1984) Proc. Natl. Acad. Sci. U.S.A. 81, 3998-4002) and a model system of horse cytochrome c three-fragment complex (Juillerat, M. A., and Taniuchi, H. (1986) J. Biol. Chem. 261, 2697-2711) with respect to the high specificity of interacting residues in the interface. Thus, by analogy to the hypothesis developed in the model system (Fisher, A., and Taniuchi, H. (1988) FASEB J. 2, A1338), we hypothesize that a closed interaction loop would be formed on the basis of contacting groups including glutamic acid 93 across or within the interface between the antigen and mAb 4-128-6 and mediate delocalized interaction to generate extra binding energy.

Published
1988

17. ADDENDUM

Author

H Taniuchi, C L Cusumano, C B Anfinsen, and J L Cone

Subjects
Cell Biology, Molecular Biology, Biochemistry
Published
1968

18. A study of renaturation of reduced hen egg white lysozyme. Enzymically active intermediates formed during oxidation of the reduced protein.

Author

Acharya AS and Taniuchi H

Subjects
Amino Acid Sequence, Amino Acids analysis, Animals, Chickens, Cyanogen Bromide, Egg White, Kinetics, Oxidation-Reduction, Peptide Fragments analysis, Protein Conformation, Protein Denaturation, Spectrometry, Fluorescence, Trypsin, Viscosity, Muramidase metabolism
Abstract

The material obtained from reduced hen egg white lysozyme after complete air oxidation at pH 8.0 and 37 degrees has yielded, by gel filtration on a Bio-Gel P-30 column, enzymically active species and an enzymically inactive form which eluted sooner than the active species but later than expected for a dimer of lysozyme. Reduced lysozyme also elutes at the same position as this inactive material. Examination of the fragments produced on CNBr cleavage of the inactive form indicates that at least 24% of the population contains incorrect disulfide bonds involving half-cystine residues 6, 30, 115, and 127. Tryptophan fluorescence and the intrinsic viscosity of the inactive form show an enlarged molecular domain with a disordered conformation. The yield of the inactive form increases as the oxidation of reduced lysozyme is accelerated using cupric ion. In the presence of 4 X 10(-5) M cupric ion, reduced lysozyme forms almost quantitatively the inactive form, which is almost completely converted to the native form by sulfhydryl-disulfide interchange catalyzed by thiol groups of either reduced lysozyme or beta-mercaptoethanol. The material trapped by alkylation of the free sulfhydryl groups with [1-14C]iodoacetic acid during the early stage of air oxidation of reduced lysozyme was fractionated by gel filtration to permit separation of the active species from the inactive form. Ion exchange chromatography of the active species yielded completely renatured lysozyme and three major enzymically active radioactive derivatives. Two of these derivatives contained approximately 2 mol of S-carboxymethylcysteine. Isolation and characterization of radioactive tryptic peptides from each of the three active forms, permitted the identification of Cys 6 and Cys 127, Cys 76 and 94, and Cys 80 as the sulfhydryl groups alkylated in these three incompletely oxidized, partially active forms. Thus, it appears that the interatomic interactions maintaining the compact three-dimensional structure of native lysozyme are operational even when one of these three native disulfide bonds between Cys 6 and Cys 127, Cys 76 and Cys 94, and Cys 64 and 80 is open.

Published
1976

22. Kinetic intermediates in the formation of ordered complexes from cytochrome c fragments. Evidence that methionine ligation is a late event in the folding process.

Author

Parr GR and Taniuchi H

Subjects
Animals, Binding Sites, Horses, Kinetics, Myocardium metabolism, Oscillometry, Protein Binding, Protein Conformation, Cytochrome c Group metabolism, Heme, Methionine
Abstract

The reactions of ferric heme-containing fragments with apofragments to form ordered complexes resembling native horse heart cytochrome c have been studied under conditions which resolve the overall process into consecutive second order and first order kinetic steps. In the initial, second order step the two fragments combine to form an intermediate complex which exhibits tryptophan 59 fluorescence quenching similar to native cytochrome c, but which has not yet achieved the native ligation state of the heme iron. The existence of first order processes following the second order step is demonstrated by absorbance changes in the Soret region. the entire absorbance change at 695 nm, relating to ligation of the sulfur atom of methionine 80 to the heme iron, is also associated with these first order processes. Thus, ligation of methionine is a late event in this self ordering of the polypeptide chains. Since the conformational energy is assumed to distinctly decrease in this late process of folding (Parr, G.R., and Taniuchi, H. (1980) J. Biol. Chem. 255, 2616-2623), it would follow that small spatial rearrangements of the polypeptide chains in the late stage of folding (as manifested by the ligation of methionine) are associated with a specific decrease in energy.

Published
1980

24. Formation of an iso-1-cytochrome c-like species containing a covalently bonded heme group from the apoprotein by a yeast cell-free system in the presence of hemin.

Author

Basile G, Di Bello C, and Taniuchi H

Subjects
Apoproteins biosynthesis, Cell-Free System, Cytochrome c Group biosynthesis, Iodine Radioisotopes, NAD, NADP, Cytochrome c Group analogs & derivatives, Cytochromes c, Heme metabolism, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins
Abstract

Incubation of the 125I-labeled apoprotein, prepared from 125I-labeled iso-1-cytochrome c, with a yeast mitochondrial fraction in the presence of hemin, NADPH, and an extract of the postmitochondrial fraction at 32 +/- 1 degree C for 30 min has resulted in formation of cytochrome c-like species in yields of up to 35%. This radioactive synthesized species contains a functional group which responds to reduction with ascorbate and oxidation with K3Fe(CN)6 in that it is resistant in the reduced form and susceptible in the oxidized form to trypsin action in a manner characteristic of native cytochrome c. The functional group cannot be removed from the protein by cold HCl-acetone or 8 M urea treatment. The reduced form of the synthesized species exhibits resistance against autoxidation and the oxidized form can be reduced also by cytochrome b2. The synthesized species exhibits the same compact hydrodynamic volume of native cytochrome c. Treatment with silver sulfate followed by incubation with dithiothreitol converts the synthesized species to the original apoprotein as judged by an increase in the hydrodynamic volume. Thus, the synthesized species is indistinguishable from the original labeled iso-1-cytochrome c by these measurements; i.e. the synthesized species consists of the apoprotein to which heme is covalently attached through the thioether bond(s). The active factor of the mitochondrial fraction is heat-labile. The synthetic activity is strongly dependent on pH with a maximum approximately at pH 7.0. Hemin (or heme) appears to be required for this synthesis. The postmitochondrial fraction is inactive by itself. However, its addition markedly increases the synthetic activity. This factor is heat-stable, soluble in 80% methanol (or 75% ethanol), and insoluble in ethyl ether or ethyl acetate. Addition of NADP(H) (or NAD(H)) also increases the synthetic activity, the reduced form being more effective than the oxidized form. The postmitochondrial factor and the pyridine nucleotides appear to enhance the effect of each other. Thus, it seems that cytochrome c or a cytochrome c-like species is formed from the apoprotein and heme (or hemin) by an enzyme, cytochrome c synthetase, present in mitochondria.

Published
1980

25. Formation of a cytochrome c-like species from horse apoprotein and hemin catalyzed by yeast mitochondrial cytochrome c synthetase.

Author

Veloso D, Basile G, and Taniuchi H

Subjects
Animals, Cell-Free System, Horses, Iron metabolism, Kinetics, Apoproteins metabolism, Cytochrome c Group biosynthesis, Heme metabolism, Lyases, Mitochondria enzymology, Saccharomyces cerevisiae enzymology, Transferases metabolism
Abstract

Cytochrome c synthetase in yeast mitochondria catalyzes the formation of a yeast cytochrome c-like species from the apoprotein and hemin (Basile, G., DiBello, C., and Taniuchi, H. (1980) J. Biol. Chem. 255, 7181-7191). To test the specificity of this enzyme, 125I-labeled horse apocytochrome c was incubated with the yeast mitochondrial fraction in the presence of hemin, NADPH, and an ethanol extract of the postmitochondrial fraction. A radioactive 125I-labeled cytochrome c-like species was formed in yields of up to 26%. This 125I-labeled species is indistinguishable from horse cytochrome c by ion exchange chromatography (under the conditions which allow separation of horse and yeast cytochrome c), resistance in its reduced form to digestion by trypsin, resistance against autoxidation, reduction by cytochrome b2, and generation of the apoprotein after treatment with silver sulfate and dithiothreitol. With unlabeled horse apoprotein and [59Fe]hemin, the yield of a [59Fe-labeled horse cytochrome c-like species was up to 7% with respect to the apoprotein incubated. The yield of the 59Fe-labeled species was not altered by the addition of unlabeled FeCl3. Conversely, synthesis of the 59Fe-labeled species was not detectable after incubation of yeast mitochondria with unlabeled horse apoprotein, unlabeled hemin, and 59FeCl3. The formation of both 125I- and 59Fe-labeled cytochrome c-like species was sensitive to heat. Thus, we conclude that cytochrome c synthetase catalyzes direct bonding of heme (or hemin) to the apoprotein. Since the amino acid sequences of horse and yeast cytochromes c differ considerably, cytochrome c synthetase may recognize only a limited region(s) of the apoprotein.

Published
1981

26. A kinetic study of the complementation of fragments of staphylococcal nuclease.

Author

Light A, Taniuchi H, and Chen RF

Subjects
Amino Acid Sequence, Amino Acids analysis, Calcium pharmacology, Chemical Phenomena, Chemistry, Computers, Hydrogen-Ion Concentration, Kinetics, Mathematics, Models, Chemical, Nucleic Acids, Peptide Fragments analysis, Phosphoric Diester Hydrolases analysis, Spectrometry, Fluorescence, Temperature, Thymine Nucleotides pharmacology, Tryptophan analysis, Peptide Fragments metabolism, Phosphoric Diester Hydrolases metabolism, Staphylococcus enzymology
Published
1974

27. Nuclease B. A possible precursor of nuclease A, an extracellular nuclease of Staphylococcus aureus.

Author

Davis A, Moore IB, Parker DS, and Taniuchi H

Subjects
Amino Acid Sequence, Peptide Fragments analysis, Trypsin, Enzyme Precursors metabolism, Micrococcal Nuclease biosynthesis, Staphylococcus aureus enzymology
Abstract

During purification of nuclease (redisignated as nuclease A in the present studies) from the culture media of Staphylococcus aureus strain Foggi, three enzymacally active second species (nucleases B1, B2, and B3) were isolated as a mixture by ion exchange chromatography. Examination of the amino acid sequence of these second species indicates that nucleases B1, B2, and B3 apparently contain the same sequence as that of nuclease A with an extra sequence Ser-Gln-Thr-Asp-Asx-Gly-Val-Asx-Arg-Ser-Gly-Ser-Glu-Asp-Pro-Thr-Val-Tyr-Ser linked through a peptide bond to the NH2 terminus of the nuclease A portion. In nuclease B1 the 2 residues indicated by Asx are aspartic acid, in nuclease B2 the first and the second Asx from the NH2 terminus are aspartic acid and asparagine, respectively, and in nuclease B3 both Asx are asparagine. These second species do not contain a significant amount of carbohydrate. The extra amino acid sequence appears to be flexible and does not interfere with the ordered structure and function of the nuclease A portion. The nuclease A portion was recovered, in part, from a mixture of these nuclease B species after digestion with staphylococcal protease in the presence of ligands, deoxythymidine 3',5'-diphosphate, and calcium ion. Thus, these nuclease B species may be closely related to, if not identical with, a precursor of nuclease A. Similar second species of nuclease have been found in strain V8.

Published
1977

28. Further study of the conformation of nuclease-(1-126) in relation to intrinsic enzymatic activity.

Author

Parker DS, Davis A, and Taniuchi H

Subjects
Circular Dichroism, Kinetics, Molecular Weight, Peptide Fragments metabolism, Protein Conformation, Staphylococcus aureus enzymology, Thermodynamics, Viscosity, Micrococcal Nuclease metabolism
Abstract

Nuclease-(1-126), although containing 89% of the amino acid sequence which folds to the ordered structure of nuclease A, is disordered and highly flexible (Taniuchi, H., and Anfinsen, C. B. (1969) J. Biol. Chem. 243, 4778-4786). On the other hand, Sachs et al. (Sachs, D. H., Schechter, A. N., Eastlake, A., and Anfinsen, C. B. (1974) Nature 251, 242-244) have demonstrated intrinsic enzymatic activity for nuclease-(1-126). To attempt to learn whether or not the active population of nuclease-(1-126) has the native conformation, we have examined nuclease-(1-126) with respect to enzymatic kinetics with and without the competitive inhibitor deoxythymidine 3',5'-diphosphate (pdTp), effect of temperature on enzymatic activity, binding of pdTp in the presence of Ca2+ and intrinsic viscosity, Stokes radius, CD, and response to trypsin action in the presence and absence of pdTp and Ca2+. The results indicate that the conformation of nuclease-(1-126) bound with pdTp in the presence of Ca2+ is partially constrained but still highly flexible below 30 degrees C, outside the range of thermal transition exhibited by the ordered elements of nuclease-(1-126). Thus, formation or stabilization of active site of nuclease-(1-126) by binding with ligands is not associated with cooperative folding of the entire polypeptide chain. Considering that nuclease-(1-126) does not bind to nuclease-(127-149) but does to nuclease-(111-149), the results are consistent with the idea that the specific cooperative interactions, providing extra stabilizing energy required for maintaining the polypeptide chain in the ordered state of nuclease A, may be disrupted for nuclease-(1-126) primarily due to cleavage of the peptide bond between residues 126 and 127. Then, it may be thought that binding with ligands does not compensate for this disruption.

Published
1981

29. Ordered complexes of cytochrome c fragments. Kinetics of formation of the reduced (ferrous) forms.

Author

Parr GR and Taniuchi H

Subjects
Animals, Cattle, Heme metabolism, Horses, Iron, Kinetics, Myocardium metabolism, Oxidation-Reduction, Cytochrome c Group metabolism
Abstract

The kinetics of formation of noncovalently bound ferrous complexes derived from fragments of horse heart cytochrome c have been investigated. When the reactions are initiated by combining ferrous heme fragments with an appropriate apofragment, in the presence of 50 mM imidazole, second order rate processes are observed with rate constants essentially the same as those reported with ferric heme fragments (Parr, G. R., and Taniuchi, H. (1979) J. Biol. Chem. 254, 4836-4842). An additional, probably consecutive, kinetic process is also demonstrated. If imidazole is not present in the reaction buffer, the kinetic profiles are dramatically altered. While this is partially due to aggregation (dimerization) of the ferrous heme fragments, it can nevertheless be demonstrated that the complementation reactions with apofragments are much faster than those observed with the corresponding ferric heme fragments (in the absence of imidazole). These results reflect the effect of the oxidation state of the heme iron on the folding mechanism and, thus, the manifold nature of protein folding pathways. The rate of reduction of productive ferric complexes by sodium ascorbate was investigated and biphasic reactions were found in all cases. The data indicate an equilibrium between two forms of the ferric complexes. The results of an experiment in which the complementation of ferric (1-25)H and (23-104) was carried out in the presence of sodium ascorbate indicate that the intermediate complex (Parr, G. R., and Taniuchi, H. (1980) J. Biol. Chem. 255, 8914-8918) is not reducible by ascorbate. Thus, the increase in oxidation-reduction potential occurring on formation of the productive complex from the unbound heme fragment occurs at a late stage of the overall reaction, possibly coinciding with ligation of methionine 80 to the heme iron.

Published
1981

30. On the specificity of cytochrome c synthetase in recognition of the amino acid sequence of apocytochrome c.

Author

Visco C, Taniuchi H, and Berlett BS

Subjects
Amino Acid Sequence, Animals, Cattle, Cytochromes c, Mitochondria enzymology, Mitochondria, Heart enzymology, Saccharomyces cerevisiae enzymology, Species Specificity, Substrate Specificity, Transferases isolation & purification, Apoproteins metabolism, Cytochrome c Group metabolism, Lyases, Transferases metabolism
Abstract

Two forms of yeast cytochrome c synthetases with different specificities were resolved, one (synthetase I), solubilized from mitochondria or the cell debris with Triton X-100, recognizing not horse apocytochrome c but yeast apo-iso-1-cytochrome c as a substrate and the other (synthetase II) still bound with the particulate fraction from mitochondria after treatment with Triton, recognizing both horse and yeast apocytochromes c. The activity with labeled yeast apo-iso-1-cytochrome c as a substrate of cytochrome c synthetase I can be quantitatively inhibited by nonlabeled Candida krusei apocytochrome c and partially by nonlabeled tuna apocytochrome c but not by nonlabeled horse apocytochrome c indicating a specific amino acid sequence being recognized. However, an enzyme similarly solubilized from beef heart mitochondria recognized both horse apocytochrome c and yeast apo-iso-1-cytochrome c for attachment of heme. In view of the fact that the yeast synthetase II and the beef synthetase can both utilize either horse apocytochrome c or yeast apo-iso-1-cytochrome c as substrates, we suggest that these enzymes may also be involved in biosynthesis of cytochrome c1, that is, the ability to attach heme to apocytochrome c and apocytochrome c1 may have been conserved in eucaryotic cells, and that both synthetases may therefore be homologous.

Published
1985

34. A study of roles of evolutionarily invariant proline 30 and glycine 34 of cytochrome c.

Author

Poerio E, Parr GR, and Taniuchi H

Subjects
Amino Acid Sequence, Animals, Circular Dichroism, Horses, Kinetics, Mathematics, Molecular Conformation, Myocardium enzymology, Spectrophotometry, Ultraviolet, Thermodynamics, Cytochrome c Group metabolism, Glycine analysis, Proline analysis
Abstract

The previous studies (Juillerat, M. A., and Taniuchi, H. (1986) J. Biol. Chem. 261, 2697-2711), using a three-fragment complex (1-25)H X (28-38) X (39-104) of horse cytochrome c, have shown that invariant leucine 32 and partially invariant leucine 35, both buried in the interior, exhibit a striking difference in perturbation of binding fragment (28-38) by substitution with isoleucine. Then the idea has been proposed that the energy states of leucine 32, the Met-80-S-heme-Fe bond and other distant residues such as tryptophan 59 would be coupled to generate extra force while leucine 35 would be less important for such coupling if it were involved. In the present studies we synthesized three (28-38) analogs substituting invariant proline 30 with glycine or invariant glycine 34 with alanine or serine. Thermodynamic and kinetic studies and UV CD and biological activity measurements were carried out on binding of the analogs to complex (1-25)H X (39-104). The results with the ferric form show that perturbations of delta G, delta H, and delta S associated with formation of the intermediate complex and with the ensuing process by the Gly34----Ala or Ser substitution result in weakening the Met-80-S-heme-Fe bond formed in the latter process; in contrast, perturbation by the Pro30----Gly substitution is small. However, the biological activity is more perturbed by the Pro30----Gly substitution than by the Gly34----Ala or Ser; and in the Gly34----Ala or Ser substitution the complex appears to be more readily activated for both formation and disruption of the Met-80-S-heme-Fe bond at 20 degrees C and below than without substitution. In all cases reduction of the heme strengthens the binding of fragment (28-38). However, striking are the increases in perturbation (less negative) of both delta H and delta S for binding of fragment (28-38) to form the ground state on reduction of the heme in the Pro30----Gly, Gly34----Ala or Ser (the present studies), and Leu32----norvaline (the previous studies) substitutions. It is known that fluctuation of the atomic positions of most residues of tuna ferrocytochrome c including Pro30, Leu32, and Gly34 increases on oxidation of the heme and that these three residues are among those showing the least fluctuating atomic positions (Takano, T., and Dickerson, R.E. (1982) in Electron Transport and Oxygen Utilization (Ho, C., ed) pp. 17-26, Elsevier/North-Holland Biomedical Press, New York).(ABSTRACT TRUNCATED AT 400 WORDS)

Published
1986

35. A study on the role of evolutionarily invariant leucine 32 of cytochrome c.

Author

Juillerat MA and Taniuchi H

Subjects
Amino Acid Sequence, Animals, Chromatography, Gel, Dialysis, Horses, Mathematics, Models, Chemical, Structure-Activity Relationship, Thermodynamics, Cytochrome c Group, Leucine
Abstract

To investigate the role of evolutionarily invariant leucine 32 of horse cytochrome c, analogs of residues 28-38, (28-38), each containing a substituted amino acid at positions 32 or 35 were synthesized using Merrifield's method. Position 35 is leucine in horse cytochrome c but replaced by nonpolar amino acids in some species. The ability of the analogs to bind to the two-fragment complex of ferri- or ferro heme fragment (1-25)H and apofragment (39-104) was measured using gel filtration and equilibrium dialysis. Replacement of leucine 32 with isoleucine, for example, increased the dissociation constant by more than 400-fold for the ferrous complex. In contrast, replacement of leucine 35 with isoleucine seems to increase it only by a small degree. Since both leucine 32 and leucine 35 are completely buried within the structure, hydrophobic interaction would not explain this striking difference. However, thermodynamic analyses and absorption spectra of the ferric complex have indicated that replacement with norvaline of leucine 32 increases both delta H and delta S (more positive) associated with formation of an intermediate three-fragment complex and decreases both delta H and delta S (more negative) associated with transformation from the intermediate to the ground state, resulting in weakening the methionine 80--S--heme-Fe bond formed in the latter step. Taking the results together with the fragment exchange studies on the ferrous complex and available evidence, we suggest that the interaction involving leucine 32 would be coupled not only with the methionine 80--S--heme-Fe bond but also with the energy state of other distant residues such as tryptophan 59, generating extra energy for modulating the binding of the complex, i.e. the force of folding. In contrast, leucine 35 would be less important even if it were involved in such coupling.

Published
1986

36. Formation of a biologically active, ordered complex from two overlapping fragments of cytochrome c.

Author

Hantgan RR and Taniuchi H

Subjects
Amino Acids analysis, Animals, Apoenzymes, Binding Sites, Ethylmaleimide, Horses, Kinetics, Models, Structural, Myocardium enzymology, Peptide Fragments analysis, Protein Binding, Protein Conformation, Spectrometry, Fluorescence, Trypsin, Cytochrome c Group metabolism
Abstract

A noncovalent complex of the apoprotein (1-104) and cyanogen bromide heme fragment containing residues 1 to 65, (1-65) H, has been prepared from horse heart cytochrome c. Conditions under which the redundant portions of the ferrous complex can be removed by limited trypsin digestion have been devised. The complementing fragments have been isolated from the derived complexes and four apofragments and one heme fragment have been identified in the amino acid sequence of cytochrome c. They are (39-104), (40-104), (54-104), (56-104), and (1-53)H. The formation of an ordered ferric complex composed of one heme fragment and one apofragment for the cases (1-53)H (39-104), (1-53)H-(40-104), (1-53)H-(54-104), and (1-53)H-(56-104) has been demonstrated by the quenching of the tryptophan 59 fluorescence and the regain of biological activity in a cytochrome b2 assay. The apparent dissociation constant has been estimated as less than 3 X 10(-7) M in all the aforementioned cases. Thus, the region (between residues 38 and 57) of the amino acid sequence permissible for cleavage without disruption of the ordered structure indicated by the present in vitro experiments corresponds to that (between residues 38 and 57) evolutionally deleted in the three-dimensional structure of Pseudomonas aeruginosa cytochrome c551 discovered by Dickerson et al. (Dickerson, R.E., Timkovich, R., and Almassy, R.J. (1976) J. Mol. Biol. 100, 473-491).

Published
1977

37. Synthesis of a heme fragment of horse cytochrome c which forms a productive complex with a native apofragment.

Author

Veloso D, Juillerat M, and Taniuchi H

Subjects
Amino Acid Sequence, Animals, Cytochromes c, Horses, Mitochondria enzymology, Models, Molecular, Peptide Fragments chemical synthesis, Protein Binding, Protein Conformation, Saccharomyces cerevisiae enzymology, Transferases metabolism, Apoproteins metabolism, Cytochrome c Group chemical synthesis, Cytochrome c Group metabolism, Heme metabolism, Lyases
Abstract

To investigate the amino acid sequence of apocytochrome c recognized by yeast mitochondrial cytochrome c synthetase, a labeled apofragment containing residues 1 to 25 of horse cytochrome c, N alpha-[3H]acetyl-(1-25), and an analog containing glycine in place of cysteines 14 and 17, N alpha-[3H]acetyl-[14-Gly, 17-Gly] (1-25), have been synthesized using the Merrifield's improved solid phase method (Mitchell, A. R., Ericksen , B. W., Ryabtsev , M. N., Hodges , R. S., and Merrifield, R. B. (1976) J. Am. Chem. Soc. 98, 7357-7362) and then purified to homogeneity. Upon incubation with yeast mitochondria in the presence of hemin, a radioactive species, produced from N alpha-[3H]acetyl-(1-25) and not from N alpha-acetyl-[14-Gly, 17-Gly] (1-25), formed a complex with native apofragment (23-104). This semisynthetic complex was indistinguishable from the native complex in resistance to trypsin upon reduction with ascorbate and by ion-exchange chromatography. The radioactive species, dissociated from the complex was identical with native heme fragment N alpha-acetyl-(1-25)H by reverse-phase high pressure liquid chromatography. Treatment of this radioactive heme fragment with silver sulfate and then with dithiothreitol generated the original apofragment . Thus, if it is assumed that the mitochondrial enzyme catalyzing this covalent attachment of heme to synthetic apo-N alpha-[3H]acetyl-(1-25) is a cytochrome c synthetase, the results may be interpreted as indicating that the amino acid sequence of residues 1 to 25 of horse cytochrome c would contain the principal recognition site of the enzyme.

Published
1984

38. The mechanism of stabilization of the structure of nuclease-T by binding of ligands.

Author

Taniuchi H and Bohnert JL

Subjects
Calcium, Hot Temperature, Mathematics, Nucleic Acids, Protein Binding, Protein Conformation, Staphylococcus enzymology, Thermodynamics, Thymine Nucleotides, Ligands, Phosphoric Diester Hydrolases
Abstract

The rate of unfolding of Nuclease-T at pH 8,20 degrees was determined as a function of concentration of the ligands deoxythymidine 3',5'-diphosphate (pdTp) and Ca2+ on the basis of the rate of exchange between free fragment, Nuclease-T(50-149) and labeled fragment, Nuclease-T-(50-149) incorporated in the structure of nuclease-T (Taniuchi, H. (1973) J. Biol. Chem. 248, 5164-5174). The rate constant of unfolding of unliganded Nuclease-T' was 4.6 times 10-4s-1. Those of Nuclease-T' bound with pdTp, with Ca2+, and with both pdtp and Ca2+ were 9.0 times 10-5, 1.6 times 10-4, and 2.2 times 10-5s-1, respectively. The association constants of pdTp and Ca2+ with Nuclease-T' were found to be 1.0 times 10-4 and 2.0 times 10-2 m-1, respectively. Those of pdTp with Nuclease-T' plus Ca2+ and of Ca2+ with Nuclease-T' plus pdTp were 4 times 10-5 and 1.4 times 10-4M-1, respectively. The calculation of free energy change on the basis of the association constants shows that the magnitude of negative free energy change involved in the binding of either of the two ligands increases by approximately 2 kcal when the other ligand is already bound. There is a correlation between the free energy change and the specifically coupled with the cooperative interacions operating throught the three-dimensional structure resulting in strengthening of the interactions throughtout the structure, including those with the ligands, without a large change in conformation.

Published
1975

39. Study of equilibration of the system involving two alternative, enzymically active complementing structures simultaneously formed from two overlapping fragments of staphylococcal nuclease.

Author

Taniuchi H, Parker DS, and Bohnert JL

Subjects
Amino Acid Sequence, Amino Acids analysis, Binding Sites, Calcium, Kinetics, Ligands, Mathematics, Nucleotides, Cyclic, Peptide Fragments metabolism, Protein Binding, Protein Conformation, Temperature, Thymine Nucleotides, Micrococcal Nuclease metabolism
Abstract

Quantitative complementation of two overlapping fragments of staphylococcal nuclease, Nuclease-(1-126) (residues 1 to 126) and Nuclease-T-(50-149) (residues 50 to 149), simultaneously forms in 1 min, two alternative, enzymically active ordered structures (types I and II) resembling nuclease (149 residues) (Taniuchi, H., and Anfinsen, C.B. (1971) J. Biol. Chem. 246, 2291-2301). We determined the ratio of type I to type II complex formed from the two fragments as a function of time, temperature, and the presence or absence of the ligands thymidine 3',5'-diphosphate and calcium ion. The ratio of type I to type II complex was determined on the basis of the quantities of their derived complexes obtained after each experiment by removing the redundant amino acid sequences by limited digestion with trypsin in the presence of ligands. The quantity of the derived complexes was estimated by quantitative determination of the component fragments separated by gel filtration. The ratio of type I to type II complex formed in 2 min after mixing the two fragments was approximately 0.3 and appears to be independent of temperature and the presence or absence of ligands. The equilibrium of the system of type I and II complexes is attained through unfolding and folding. The ratios of type I to type II complex at the apparent equilibrium state of the system at 6 and 23 degrees were approximately 1.1 and 2.4, respectively. The observations indicate that the rate of unfolding of type II complex is greater than that of type I complex at 6 degrees and increases more than that of type I complex with increasing temperature. Thus, the change of the complementing structure from type I complex with increasing temperature. Thus, the change of the complementing structure from type I to type II causes a decrease in the activation free energy, an increase in the activation enthalpy, and thereby an increase in the activation entropy of unfolding. Since the unfolded states with which type I and II complexes are in equilibrium are the same, the distribution of the population of type I and II complexes at the equilibrium state will be determined on the basis of the respective decreases in Gibbs standard free energy from the unfolded state to type I and II complexes. On this basis type I complex has a lower energy by deltaG0 = -0.05 and -0.51 kcal mol-1 at 6 and 23 degrees, respectively, than type II complex. Nevertheless, at the initial complementation the population of type I complex formed is approximately one-third that of type II complex at both 6 and 23 degrees. That is, the probability (rate) of folding is not related to the decrease in energy from the unfolded to the folded state. Using van't Hoff's equation deltaH = 7.5 kcal mol-1 and then deltaS degrees = 27 cal deg-1 mol-1 from type II to type I complex.

Published
1977

40. Evidence for formation of two thioether bonds to link heme to apocytochrome c by partially purified cytochrome c synthetase.

Author

Taniuchi H, Basile G, Taniuchi M, and Veloso D

Subjects
Cytochromes c, Octoxynol, Polyethylene Glycols, Saccharomyces cerevisiae enzymology, Solubility, Cytochrome c Group metabolism, Heme metabolism, Lyases, Sulfides metabolism, Transferases metabolism
Abstract

Cytochrome c synthetase has been solubilized from yeast mitochondria using Triton X-100 and fractionated with ammonium sulfate. Use of this partially purified enzyme has permitted us to isolate a quantity of iso-1-cytochrome c formed from 125I-labeled apocytochrome c and hemin in the presence of a NADPH-generating system. Visible absorption spectra (pH 8.0 or 5.0) including alpha, beta, and Soret bands and their molar absorption coefficients of this enzymatically synthesized cytochrome c in the oxidized and reduced states are the same, within experimental error, as those of native cytochrome c. Pyridine ferrohemochrome (pH 13) of the synthesized species also exhibits the same alpha and beta bands as those of iso-l-cytochrome c and similar to those reported for heme peptides of cytochrome c. If only one or no thioether bond were formed between the two vinyl side groups of heme and the cysteine residues of apocytochrome c, all these alpha and beta bands would have shifted to red (Pettigrew, G. W., Leaver, J. L., Meyer, T. E., and Ryle, T. E. (1975) Biochem J. 147, 291-302). Thus, two thioether bonds appear to be formed to link heme to apocytochrome c by cytochrome c synthetase, completing information of the three-dimensional structure of cytochrome c.

Published
1983

42. Evidence of a compact structure for kinetic intermediates in the folding of a fragment complex of tuna cytochrome c.

Author

Parr GR and Taniuchi H

Subjects
Amino Acid Sequence, Animals, Circular Dichroism, Kinetics, Myocardium, Protein Conformation, Spectrometry, Fluorescence, Tuna, Cytochrome c Group metabolism
Abstract

A noncovalently bound, ordered complex consisting of fragments (1-25)H and (14-103) derived from tuna cytochrome c has been prepared and characterized. The equilibrium properties of this complex are indistinguishable from those of the corresponding complex, (1-25)H X (23-104), of horse cytochrome c. The tuna species possesses a second tryptophan residue (at position 33 of the amino acid sequence and replacing the histidine residue of the horse protein) whose fluorescence is also essentially fully quenched in the native form and in the complex. It is found that for the tuna complex, the fluorescence of both tryptophans is fully quenched during the second order phase of the reaction mechanism. This provides evidence for the compact nature of the intermediate complexes formed at this stage of the complementation process (Parr, G. R., and Taniuchi, H. (1982) J. Biol. Chem. 257, 10103-10111). The observed second order rate constant for the tuna fragments is reduced by a factor of two from that for the horse fragments. During the first order kinetic phase corresponding to the transition from the intermediate complexes to the native complex, qualitative as well as quantitative differences are also observed between the tuna and the horse species. The kinetics of complementation of the "hybrid" complexes is also reported. This exchangeability of both the heme fragment and the apofragment of the complex between these two species indicates close similarity of the folding mechanism. Nonetheless, the results also serve to highlight the subtle effects exerted on the folding process by a relatively small number of changes (17%) in the amino acid sequence.

Published
1983

43. Intramolecular flip between two alternative forms of complex formed from a heme fragment and apoprotein of horse cytochrome c.

Author

Juillerat MA and Taniuchi H

Subjects
Animals, Cytochromes c, Horses, Kinetics, Models, Molecular, Myocardium metabolism, Peptide Fragments isolation & purification, Protein Binding, Protein Conformation, Thermodynamics, Apoproteins metabolism, Cytochrome c Group metabolism, Heme metabolism
Abstract

The previous studies have shown that (a) noncovalent interactions of the ferro-heme fragment of residues 1-38 and apoprotein (1-104) of horse cytochrome c simultaneously and specifically form two isomeric complexes, types I and II resembling the native protein (the redundant residues flexibly protruding from the ordered structure); (b) the type II form but not type I appears to bind to CO; and (c) residues 39-55 are more flexible for type II form than type I (Parr, G. R., and Taniuchi, H. (1981) J. Biol. Chem. 256, 125-132). In the present study, we investigated 1) kinetics and thermodynamics of interconversion between type I and II forms of complex ferro-(1-38)-H.(1-104); 2) the properties of the CO binding population; 3) the rate of dissociation of complexes ferri- and ferro-(1-38)-H.(39-104) (mimicking type II form); and 4) thermal transition of the 695-nm absorption band and biological activity of complexes. The results indicate (a) interconversion between type I and II forms of complex ferro-(1-38)-H.(1-104) occurs without going through dissociation (t1/2 less than or equal to 12 min at 10 degrees C) and is associated with delta H (= -7.2 +/- 3.7 kcal/mol at 10 degrees C) favoring type I form and delta S (= 23 +/- 13 e.u. at 10 degrees C) favoring type II; (b) the CO-binding population correlates with type II; and (c) change from the ferrous to the ferric state of heme appears to perturb the thermodynamic relationship between type I and II forms. Interpreting the results and available evidence, we suggest that "intramolecular" flip between ferro-type I and ferro-type II forms would establish the Boltzmann distribution of these two distinctly different energy states, type I form having more strengthened interatomic interactions and type II more pronounced internal motion.

Published
1987

44. A study of fine specificity of monoclonal antibodies to yeast iso-1-cytochrome c.

Author

Silvestri I and Taniuchi H

Subjects
Amino Acid Sequence, Animals, Antibody Specificity, Cross Reactions, Enzyme-Linked Immunosorbent Assay, Molecular Sequence Data, Protein Conformation, Species Specificity, Antibodies, Monoclonal immunology, Cytochrome c Group immunology, Isoenzymes immunology, Saccharomyces cerevisiae enzymology
Abstract

Seven monoclonal antibodies, prepared to yeast holo- or apo-iso-1-cytochrome c by the method of Köhler and Milstein (Goding, J. W. (1983) Monoclonal Antibodies: Principles and Practice, Academic Press, Orlando, FL) were characterized by cross-reaction with a panel of evolutionarily related cytochromes c, apocytochromes c, fragments and homologous and hybrid fragment complexes, inhibition, competitive inhibition, and complementation and fluorescence titration. The results have permitted us to assign the specifically recognized amino acids as follows. IgG1 monoclonals: 4-74-6, Leu-63 and/or Asn-67 and/or Asn-68; 4-128-6, Glu-93; 4-145-10, Thr-74; 2-96-12, Asp-65; 2-34-19, Lys-59; and 10-28-86, trimethyl-lysine 77. IgM monoclonal 39-14, Pro-30 and His-31. With mAb 4-128-6 substitution of glutamic acid 93 with alanine, as it occurs in Candida cytochrome c, has resulted in a decrease in affinity by a factor of 10(4). A calculation appears to show that this value is too large to be accounted for solely by the sum of energy losses due to disruption of charge neutralization and changes of hydrophobic interaction including van der Waals interaction. This and similar results with mAb 10-28-86 have led us to the idea that some new extra interatomic interaction sensitive to differences in configuration of atomic groups may be present and perturbed in the substitution. Furthermore, the assumption of the presence of such interaction can explain the striking similarity between the antigen-antibody interaction (e.g. Geysen, H. M., Meloen, R. H., and Barteling, S. J. (1984) Proc. Natl. Acad. Sci. U.S.A. 81, 3998-4002) and a model system of horse cytochrome c three-fragment complex (Juillerat, M. A., and Taniuchi, H. (1986) J. Biol. Chem. 261, 2697-2711) with respect to the high specificity of interacting residues in the interface. Thus, by analogy to the hypothesis developed in the model system (Fisher, A., and Taniuchi, H. (1988) FASEB J. 2, A1338), we hypothesize that a closed interaction loop would be formed on the basis of contacting groups including glutamic acid 93 across or within the interface between the antigen and mAb 4-128-6 and mediate delocalized interaction to generate extra binding energy.

Published
1988

47. Characterization of a nuclease produced by Staphylococcus aureus.

Author

Heins JN, Suriano JR, Taniuchi H, and Anfinsen CB

Subjects
Amino Acids analysis, Calcium Chloride, Chemical Phenomena, Chemistry, Physical, Ultracentrifugation, Deoxyribonucleases metabolism, Ribonucleases metabolism, Staphylococcus enzymology
Published
1967

48. The large scale preparation of an extracellular nuclease of Staphylococcus aureus.

Author

Morávek L, Anfinsen CB, Cone JL, and Taniuchi H

Subjects
Adsorption, Chemical Phenomena, Chemistry, Chromatography, Gel, Chromatography, Ion Exchange, Culture Media, Ion Exchange, Methods, Phosphates, Cellulose, Deoxyribonucleases isolation & purification, Ribonucleases isolation & purification, Staphylococcus enzymology
Published
1969

50. ENZYMATIC FORMATION OF CATECHOL FROM ANTHRANILIC ACID.

Author

TANIUCHI H, HATANAKA M, KUNO S, HAYAISHI O, NAKAJIMA M, and KURIHARA N

Subjects
Catechols, Levulinic Acids, ortho-Aminobenzoates, Benzene, Benzoates, Carbon Isotopes, Glycols, Kynurenic Acid, Metabolism, Mixed Function Oxygenases, NAD, NADP, Oxidoreductases, Pseudomonas, Research, Salicylic Acid, Tryptophan
Published
1964

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