Your search keyword '"Narhi LO"' showing total 30 results

1. Use of In Vitro Assays to Assess Immunogenicity Risk of Antibody-Based Biotherapeutics.

Author

Joubert MK, Deshpande M, Yang J, Reynolds H, Bryson C, Fogg M, Baker MP, Herskovitz J, Goletz TJ, Zhou L, Moxness M, Flynn GC, Narhi LO, and Jawa V

Subjects

Antibodies, Monoclonal genetics, Antibodies, Monoclonal metabolism, Biosimilar Pharmaceuticals, Cell Proliferation, Cells, Cultured, Cytokines analysis, Enzyme-Linked Immunosorbent Assay, Enzyme-Linked Immunospot Assay, Glycosylation, Humans, Interferon-gamma analysis, Interleukin-2 analysis, Leukocytes, Mononuclear cytology, Leukocytes, Mononuclear metabolism, Lymphocyte Activation, Point Mutation, Risk Assessment, T-Lymphocytes cytology, T-Lymphocytes metabolism, Antibodies, Monoclonal immunology, Leukocytes, Mononuclear immunology, T-Lymphocytes immunology

Abstract

An In Vitro Comparative Immunogenicity Assessment (IVCIA) assay was evaluated as a tool for predicting the potential relative immunogenicity of biotherapeutic attributes. Peripheral blood mononuclear cells from up to 50 healthy naïve human donors were monitored up to 8 days for T-cell proliferation, the number of IL-2 or IFN-γ secreting cells, and the concentration of a panel of secreted cytokines. The response in the assay to 10 monoclonal antibodies was found to be in agreement with the clinical immunogenicity, suggesting that the assay might be applied to immunogenicity risk assessment of antibody biotherapeutic attributes. However, the response in the assay is a measure of T-cell functional activity and the alignment with clinical immunogenicity depends on several other factors. The assay was sensitive to sequence variants and could differentiate single point mutations of the same biotherapeutic. Nine mAbs that were highly aggregated by stirring induced a higher response in the assay than the original mAbs before stirring stress, in a manner that did not match the relative T-cell response of the original mAbs. In contrast, mAbs that were glycated by different sugars (galactose, glucose, and mannose) showed little to no increase in response in the assay above the response to the original mAbs before glycation treatment. The assay was also used successfully to assess similarity between multiple lots of the same mAb, both from the same manufacturer and from different manufacturers (biosimilars). A strategy for using the IVCIA assay for immunogenicity risk assessment during the entire lifespan development of biopharmaceuticals is proposed.

Published

2016

2. Highly aggregated antibody therapeutics can enhance the in vitro innate and late-stage T-cell immune responses.

Author

Joubert MK, Hokom M, Eakin C, Zhou L, Deshpande M, Baker MP, Goletz TJ, Kerwin BA, Chirmule N, Narhi LO, and Jawa V

Subjects

Antibodies immunology, Cells, Cultured, Cytokines immunology, Humans, Receptors, IgG immunology, Signal Transduction drug effects, Signal Transduction immunology, T-Lymphocytes cytology, Toll-Like Receptor 2 immunology, Toll-Like Receptor 4 immunology, Antibodies pharmacology, Immunity, Cellular drug effects, Immunity, Innate drug effects, Immunotherapy methods, T-Lymphocytes immunology

Abstract

Aggregation of biotherapeutics has the potential to induce an immunogenic response. Here, we show that aggregated therapeutic antibodies, previously generated and determined to contain a variety of attributes (Joubert, M. K., Luo, Q., Nashed-Samuel, Y., Wypych, J., and Narhi, L. O. (2011) J. Biol. Chem. 286, 25118-25133), can enhance the in vitro innate immune response of a population of naive human peripheral blood mononuclear cells. This response depended on the aggregate type, inherent immunogenicity of the monomer, and donor responsiveness, and required a high number of particles, well above that detected in marketed drug products, at least in this in vitro system. We propose a cytokine signature as a potential biomarker of the in vitro peripheral blood mononuclear cell response to aggregates. The cytokines include IL-1β, IL-6, IL-10, MCP-1, MIP-1α, MIP-1β, MMP-2, and TNF-α. IL-6 and IL-10 might have an immunosuppressive effect on the long term immune response. Aggregates made by stirring induced the highest response compared with aggregates made by other methods. Particle size in the 2-10 μm range and the retention of some folded structure were associated with an increased response. The mechanism of aggregate activation at the innate phase was found to occur through specific cell surface receptors (the toll-like receptors TLR-2 and TLR-4, FcγRs, and the complement system). The innate signal was shown to progress to an adaptive T-cell response characterized by T-cell proliferation and secretion of T-cell cytokines. Investigating the ability of aggregates to induce cytokine signatures as biomarkers of immune responses is essential for determining their risk of immunogenicity.

Published

2012

3. Classification and characterization of therapeutic antibody aggregates.

Author

Joubert MK, Luo Q, Nashed-Samuel Y, Wypych J, and Narhi LO

Subjects

Animals, Antibodies, Monoclonal, Murine-Derived therapeutic use, Catalysis, Humans, Hydrogen-Ion Concentration, Immunoglobulin G therapeutic use, Antibodies, Monoclonal, Murine-Derived chemistry, Copper chemistry, Immunoglobulin G chemistry

Abstract

A host of diverse stress techniques was applied to a monoclonal antibody (IgG(2)) to yield protein particles with varying attributes and morphologies. Aggregated solutions were evaluated for percent aggregation, particle counts, size distribution, morphology, changes in secondary and tertiary structure, surface hydrophobicity, metal content, and reversibility. Chemical modifications were also identified in a separate report (Luo, Q., Joubert, M. K., Stevenson, R., Narhi, L. O., and Wypych, J. (2011) J. Biol. Chem. 286, 25134-25144). Aggregates were categorized into seven discrete classes, based on the traits described. Several additional molecules (from the IgG(1) and IgG(2) subtypes as well as intravenous IgG) were stressed and found to be defined with the same classification system. The mechanism of protein aggregation and the type of aggregate formed depends on the nature of the stress applied. Different IgG molecules appear to aggregate by a similar mechanism under the same applied stress. Aggregates created by harsh mechanical stress showed the largest number of subvisible particles, and the class generated by thermal stress displayed the largest number of visible particles. Most classes showed a disruption of the higher order structure, with the degree of disorder depending on the stress process. Particles in all classes (except thermal stress) were at least partially reversible upon dilution in pH 5 buffer. High copper content was detected in isolated metal-catalyzed aggregates, a stress previously shown to produce immunogenic aggregates. In conclusion, protein aggregates can be a very heterogeneous population, whose qualities are the result of the type of stress that was experienced.

Published

2011

4. Chemical modifications in therapeutic protein aggregates generated under different stress conditions.

Author

Luo Q, Joubert MK, Stevenson R, Ketchem RR, Narhi LO, and Wypych J

Subjects

Animals, Hot Temperature, Humans, Immunoglobulin Fc Fragments therapeutic use, Mice, Oxidation-Reduction, Protein Conformation, Copper chemistry, Hydrogen Peroxide chemistry, Immunoglobulin Fc Fragments chemistry

Abstract

In this study, we characterized the chemical modifications in the monoclonal antibody (IgG(2)) aggregates generated under various conditions, including mechanical, chemical, and thermal stress treatment, to provide insight into the mechanism of protein aggregation and the types of aggregate produced by the different stresses. In a separate study, additional biophysical characterization was performed to arrange these aggregates into a classification system (Joubert, M. K., Luo, Q., Nashed-Samuel, Y., Wypych, J., and Narhi, L. O. (2011) J. Biol. Chem. 286, 25118-25133). Here, we report that different aggregates possessed different types and levels of chemical modification. For chemically treated samples, metal-catalyzed oxidation using copper showed site-specific oxidation of Met(246), His(304), and His(427) in the Fc portion of the antibody, which might be attributed to a putative copper-binding site. For the hydrogen peroxide-treated sample, in contrast, four solvent-exposed Met residues in the Fc portion were completely oxidized. Met and/or Trp oxidation was observed in the mechanically stressed samples, which is in agreement with the proposed model of protein interaction at the air-liquid interface. Heat treatment resulted in significant deamidation but almost no oxidation, which is consistent with thermally induced aggregates being generated by a different pathway, primarily by perturbing conformational stability. These results demonstrate that chemical modifications are present in protein aggregates; furthermore, the type, locations, and severity of the modifications depend on the specific conditions that generated the aggregates.

Published

2011

5. Ion-specific modulation of protein interactions: anion-induced, reversible oligomerization of a fusion protein.

Author

Gokarn YR, Fesinmeyer RM, Saluja A, Cao S, Dankberg J, Goetze A, Remmele RL Jr, Narhi LO, and Brems DN

Subjects

Cell Adhesion Molecules chemistry, Cell Adhesion Molecules genetics, Cell Adhesion Molecules metabolism, Escherichia coli genetics, Escherichia coli metabolism, Escherichia coli Proteins chemistry, Escherichia coli Proteins genetics, Humans, Light, Peptides chemistry, Peptides genetics, Peptides metabolism, Protein Binding physiology, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Scattering, Radiation, Ultracentrifugation, Anions metabolism, Escherichia coli Proteins metabolism, Protein Interaction Domains and Motifs physiology, Protein Multimerization physiology, Recombinant Fusion Proteins metabolism

Abstract

Ions can significantly modulate the solution interactions of proteins. We aim to demonstrate that the salt-dependent reversible heptamerization of a fusion protein called peptibody A or PbA is governed by anion-specific interactions with key arginyl and lysyl residues on its peptide arms. Peptibody A, an E. coli expressed, basic (pI = 8.8), homodimer (65.2 kDa), consisted of an IgG1-Fc with two, C-terminal peptide arms linked via penta-glycine linkers. Each peptide arm was composed of two, tandem, active sequences (SEYQGLPPQGWK) separated by a spacer (GSGSATGGSGGGASSGSGSATG). PbA was monomeric in 10 mM acetate, pH 5.0 but exhibited reversible self-association upon salt addition. The sedimentation coefficient (s(w)) and hydrodynamic diameter (D(H)) versus PbA concentration isotherms in the presence of 140 mM NaCl (A5N) displayed sharp increases in s(w) and D(H), reaching plateau values of 9 s and 16 nm by 10 mg/mL PbA. The D(H) and sedimentation equilibrium data in the plateau region (>12 mg/mL) indicated the oligomeric ensemble to be monodisperse (PdI = 0.05) with a z-average molecular weight (M(z)) of 433 kDa (stoichiometry = 7). There was no evidence of reversible self-association for an IgG1-Fc molecule in A5N by itself or in a mixture containing fluorescently labeled IgG1-Fc and PbA, indicative of PbA self-assembly being mediated through its peptide arms. Self-association increased with pH, NaCl concentration, and anion size (I(-) > Br(-) > Cl(-) > F(-)) but could be inhibited using soluble Trp-, Phe-, and Leu-amide salts (Trp > Phe > Leu). We propose that in the presence of salt (i) anion binding renders PbA self-association competent by neutralizing the peptidyl arginyl and lysyl amines, (ii) self-association occurs via aromatic and hydrophobic interactions between the ..xxCTRWPWMC..xxxCTRWPWMCxx.. motifs, and (iii) at >10 mg/mL, PbA predominantly exists as heptameric clusters.

Published

2009

6. Enhanced stability of recombinant keratinocyte growth factor by mutagenesis.

Author

Hsu E, Osslund T, Nybo R, Chen BL, Kenney WC, Morris CF, Arakawa T, and Narhi LO

Subjects

Amino Acid Sequence, Animals, Calorimetry, Differential Scanning, Cell Line, Circular Dichroism, Drug Stability, Fibroblast Growth Factor 7 metabolism, Fibroblast Growth Factor 7 pharmacology, Heparin metabolism, Hot Temperature, Mice, Mitogens analysis, Molecular Sequence Data, Mutagenesis, Protein Binding, Protein Conformation, Protein Denaturation, Fibroblast Growth Factor 7 genetics, Recombinant Proteins genetics

Abstract

Native sequence keratinocyte growth factor (KGF) is fairly unstable, as manifested by the loss of the monomeric native protein accompanied by the accumulation of aggregated species during storage at moderate temperatures. Several different types of analogs were generated and the storage stability of the protein assessed. In the first type of analog one or more of the five cysteinyl residues in KGF were replaced; in the second class the N-terminal residues that included the first disulfide bond were deleted. Both of these types of analogs involved removal of the disulfide bond between cysteines 1 and 15. The third group involved mutating one of the basic amino acids located in a cluster of positive charges (involved in heparin binding) around Arg144 to a neutral or acidic amino acyl residue. Among the cysteine replacement analogs, the double mutation of Cys1 and 15 to Ser resulted in significantly increased stability without compromising the mitogenic activity, while Cys to Ser mutations at other positions were either destabilizing or had no effect. Deletion of the 15, 23 or 27 N-terminal amino acyl residues also increased the stability of the protein. The activity of the analogs was not affected by the deletion of 15 or 23 amino acids, but it was significantly decreased upon removal of the 27 N-terminal amino acyl residues. Much greater stability was achieved by mutation of the basic amino acids, especially Arg144, to Glu or Gln, but this increase in stability was accompanied by large decrease in activity. The analog with the 23 N-terminal amino acyl residues deleted represents one of the best compromises between increased stability and retention of activity.

Published

2006

7. Effect of the intermolecular disulfide bond on the conformation and stability of glial cell line-derived neurotrophic factor.

Author

Li T, Yamane H, Arakawa T, Narhi LO, and Philo J

Subjects

Amino Acid Sequence, Cell Line, Circular Dichroism, Cysteine genetics, Disulfides chemistry, Glial Cell Line-Derived Neurotrophic Factor, Heparin metabolism, Hot Temperature, Hydrogen-Ion Concentration, Mutation, Nerve Tissue Proteins genetics, Nerve Tissue Proteins metabolism, Protein Conformation, Protein Folding, Protein Structure, Secondary, Protein Structure, Tertiary, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Spectroscopy, Fourier Transform Infrared, Spectrum Analysis, Raman, Tyrosine chemistry, Nerve Growth Factors, Nerve Tissue Proteins chemistry

Abstract

Glial cell line-derived neurotrophic factor (GDNF) is a member of the TGF-beta superfamily of proteins. It exists as a covalent dimer in solution, with the 15 kDa monomers linked by an interchain disulfide bond through the Cys101 residues. Sedimentation equilibrium and velocity experiments demonstrated that, after removal of the interchain disulfide bond, GDNF remains as a non-covalent dimer and is stable at pH 7.0. To investigate the effect of the intermolecular disulfide on the structure and stability of GDNF, we compared the solution structures of the wild-type protein and a cysteine-101 to alanine (C101A) mutant using Fourier transform infrared (FTIR), FT-Raman and circular dichroism (CD) spectroscopy and sedimentation analysis. The elimination of the intermolecular disulfide bond causes only minor changes (approximately 4%) in the secondary structures of GDNF. The far- and near-UV CD spectra demonstrated that the secondary and tertiary structures were similar for both wild-type and C101A GDNF. Heparin binding and sedimentation velocity experiments also indicated that the folded structure of the wild-type and C101A GDNF are indistinguishable. The thermal stability of GDNF does not appear to be affected by the absence of the interchain disulfide bond and the biological activity of the C101A mutant is identical with that of the wild-type protein. However, small but significant changes in side chain conformations of tyrosine and aliphatic residues were observed by FT-Raman spectroscopy upon removal of the intermolecular disulfide bond, which may reflect structural changes in the area of dimeric contact. By comparing the Raman spectrum of wild-type GDNF with that of the C101A analog, we identified the conformation of the intermolecular disulfide as trans-gauche-trans geometry. These results indicate that GDNF is an active, properly folded molecule in the absence of the interchain disulfide bond.

Published

2002

8. Asn to Lys mutations at three sites which are N-glycosylated in the mammalian protein decrease the aggregation of Escherichia coli-derived erythropoietin.

Author

Narhi LO, Arakawa T, Aoki K, Wen J, Elliott S, Boone T, and Cheetham J

Subjects

Amino Acid Substitution genetics, Amino Acids genetics, Asparagine chemistry, Asparagine genetics, Binding Sites, Antibody physiology, Biological Assay, Circular Dichroism, Erythropoietin chemistry, Erythropoietin metabolism, Escherichia coli, Glycosylation, Hot Temperature, Humans, Lysine chemistry, Lysine genetics, Magnetic Resonance Spectroscopy, Mutagenesis, Site-Directed, Mutation, Protein Binding, Protein Conformation, Receptors, Erythropoietin chemistry, Temperature, Amino Acids chemistry

Abstract

Erythropoietin (EPO) derived from Escherichia coli is unstable to elevated temperature and tends to aggregate with time, making it unsuitable for high-resolution structure analysis. The mammalian EPO contains about 40% carbohydrate, which makes this protein more stable and less prone to aggregate than non-glycosylated E.coli-derived EPO, but makes it unsuitable for high-resolution analysis owing to its size and flexibility. In an attempt to decrease the aggregation of E.coli-derived EPO, the three asparagine residues at positions 24, 38 and 83 were mutated to lysine residues. In the native protein, these residues are the sites of N-linked glycosylation, which suggests that they should be located on the surface of the protein and should not be involved in interactions in the hydrophobic protein core. Therefore, the substitution of basic amino acids for these neutral asparagine residues is not expected to affect the protein structure, but should increase the isoelectric point of the protein and its net positive charge, decreasing its tendency to aggregate at or below neutral pH due to electrostatic interactions. No apparent alterations in receptor binding, as determined by both cell-surface receptor competition assay and in vitro receptor dimerization experiments, were observed when these mutations were introduced into the EPO sequence. However, this mutant protein displayed a significant increase in stability to heat treatment and to storage, relative to the wild-type molecule. This resulted in a greater number of observable cross peaks in the mutant EPO in 2D NOESY experiments. However, the mutant was similar to the wild-type in stability when urea was used as a denaturant. This indicates that the introduced mutations resulted in a decrease in aggregation with heating or with prolonged incubation at ambient temperature, without changing the conformational stability or the receptor binding affinity of the mutant protein. This approach of placing charged residues at sites where N-glycosylation occurs in vivo could be applied to other systems as well.

Published

2001

9. Parkinson's disease-associated alpha-synuclein is more fibrillogenic than beta- and gamma-synuclein and cannot cross-seed its homologs.

Author

Biere AL, Wood SJ, Wypych J, Steavenson S, Jiang Y, Anafi D, Jacobsen FW, Jarosinski MA, Wu GM, Louis JC, Martin F, Narhi LO, and Citron M

Subjects

Amino Acid Sequence, Base Sequence, Circular Dichroism, DNA Primers, Molecular Sequence Data, Nerve Tissue Proteins metabolism, Protein Folding, Sequence Homology, Amino Acid, Spectrum Analysis methods, Synucleins, alpha-Synuclein, beta-Synuclein, gamma-Synuclein, Nerve Tissue Proteins chemistry, Parkinson Disease metabolism

Abstract

Parkinson's disease (PD) is a neurodegenerative disorder that is pathologically characterized by the presence of intracytoplasmic Lewy bodies. Recently, two point mutations in alpha-synuclein were found to be associated with familial PD, but as of yet no mutations have been described in the homologous genes beta- and gamma-synuclein. alpha-Synuclein forms the major fibrillar component of Lewy bodies, but these do not stain for beta- or gamma-synuclein. This result is very surprising, given the extent of sequence conservation and the high similarity in expression and subcellular localization, in particular between alpha- and beta-synuclein. Here we compare in vitro fibrillogenesis of all three purified synucleins. We show that fresh solutions of alpha-, beta-, and gamma- synuclein show the same natively unfolded structure. While over time alpha-synuclein forms the previously described fibrils, no fibrils could be detected for beta- and gamma-synuclein under the same conditions. Most importantly, beta- and gamma-synuclein could not be cross-seeded with alpha-synuclein fibrils. However, under conditions that drastically accelerate aggregation, gamma-synuclein can form fibrils with a lag phase roughly three times longer than alpha-synuclein. These results indicate that beta- and gamma-synuclein are intrinsically less fibrillogenic than alpha-synuclein and cannot form mixed fibrils with alpha-synuclein, which may explain why they do not appear in the pathological hallmarks of PD, although they are closely related to alpha-synuclein and are also abundant in brain.

Published

2000

10. Correlation between the 1.6 A crystal structure and mutational analysis of keratinocyte growth factor.

Author

Osslund TD, Syed R, Singer E, Hsu EW, Nybo R, Chen BL, Harvey T, Arakawa T, Narhi LO, Chirino A, and Morris CF

Subjects

Amino Acid Sequence, Fibroblast Growth Factor 10, Fibroblast Growth Factor 7, Heparin metabolism, Humans, Models, Molecular, Molecular Sequence Data, Protein Structure, Secondary, Sequence Homology, Amino Acid, Temperature, Crystallography, X-Ray, DNA Mutational Analysis, Fibroblast Growth Factors, Growth Substances chemistry

Abstract

A comprehensive deletion, mutational, and structural analysis of the native recombinant keratinocyte growth factor (KGF) polypeptide has resulted in the identification of the amino acids responsible for its biological activity. One of these KGF mutants (delta23KGF-R144Q) has biological activity comparable to the native protein, and its crystal structure was determined by the multiple isomorphous replacement plus anomalous scattering method (MIRAS). The structure of KGF reveals that it folds into a beta-trefoil motif similar to other members of fibroblast growth factor (FGF) family whose structures have been resolved. This fold consists of 12 anti-parallel beta-strands in which three pairs of the strands form a six-stranded beta-barrel structure and the other three pairs of beta-strands cap the barrel with hairpin triplets forming a triangular array. KGF has 10 well-defined beta strands, which form five double-stranded anti-parallel beta-sheets. A sixth poorly defined beta-strand pair is in the loop between residues 133 and 144, and is defined by only a single hydrogen bond between the two strands. The KGF mutant has 10 additional ordered amino terminus residues (24-33) compared to the other FGF structures, which are important for biological activity. Based on mutagenesis, thermal stability, and structural data we postulate that residues TRP125, THR126, and His127 predominantly confer receptor binding specificity to KGF. Additionally, residues GLN152, GLN138, and THR42 are implicated in heparin binding. The increased thermal stability of delta23KGF-R144Q can structurally be explained by the additional formation of hydrogen bonds between the GLN side chain and a main-chain carbonyl on an adjoining loop. The correlation of the structure and biochemistry of KGF provides a framework for a rational design of this potentially important human therapeutic.

Published

1998

11. The majority of stem cell factor exists as monomer under physiological conditions. Implications for dimerization mediating biological activity.

Author

Hsu YR, Wu GM, Mendiaz EA, Syed R, Wypych J, Toso R, Mann MB, Boone TC, Narhi LO, Lu HS, and Langley KE

Subjects

Amino Acid Sequence, Chromatography, Gel, Circular Dichroism, Humans, Models, Biological, Molecular Sequence Data, Protein Binding, Proto-Oncogene Proteins c-kit chemistry, Proto-Oncogene Proteins c-kit metabolism, Recombinant Proteins, Solubility, Spectrometry, Fluorescence, Stem Cell Factor metabolism, Ultracentrifugation, Stem Cell Factor chemistry

Abstract

Soluble Escherichia coli-derived recombinant human stem cell factor (rhSCF) forms a non-covalently associated dimer. We have determined a dimer association constant (Ka) of 2-4 x 10(8) M-1, using sedimentation equilibrium and size exclusion chromatography. SCF has been shown previously to be present at concentrations of approximately 3.3 ng/ml in human serum. Based on the dimerization Ka, greater than 90% of the circulating SCF would be in the monomeric form. When 125I-rhSCF was added to human serum and the serum analyzed by size exclusion chromatography, 72-49% of rhSCF was monomer when the total SCF concentration was in the range of 10-100 ng/ml, consistent with the Ka determination. Three SCF variants, SCF(F63C), SCF (V49L,F63L), and SCF(A165C), were recombinantly expressed in Escherichia coli, purified, and characterized. The dimer Ka values, biophysical properties, and biological activities of these variants were studied. Dimerization-defective variants SCF(F63C)S-CH2CONH2 and SCF(V49L,F63L) showed substantially reduced mitogenic activity, while the activity of the Cys165-Cys165 disulfide-linked SCF(A165C) dimer was 10-fold higher than that of wild type rhSCF. The results suggest a correlation between dimerization affinity and biological activity, consistent with a model in which SCF dimerization mediates dimerization of its receptor, Kit, and subsequent signal transduction.

Published

1997

12. Formation of an active dimer during storage of interleukin-1 receptor antagonist in aqueous solution.

Author

Chang BS, Beauvais RM, Arakawa T, Narhi LO, Dong A, Aparisio DI, and Carpenter JF

Subjects

Anilino Naphthalenesulfonates, Cell Line, Cell Survival drug effects, Chromatography, Gel, Chromatography, High Pressure Liquid, Circular Dichroism, Dimerization, Drug Stability, Fluorescent Dyes, Humans, Interleukin 1 Receptor Antagonist Protein, Interleukin-1 pharmacology, Kinetics, Melanoma, Protein Conformation, Protein Denaturation, Recombinant Proteins chemistry, Recombinant Proteins isolation & purification, Recombinant Proteins pharmacology, Sialoglycoproteins isolation & purification, Sialoglycoproteins pharmacology, Solutions, Spectroscopy, Fourier Transform Infrared, Water, Sialoglycoproteins chemistry

Abstract

The degradation products of recombinant human interleukin-1 receptor antagonist (rhIL-1ra) formed during storage at 30 degrees C in aqueous solution were characterized. Cationic exchange chromatography of the stored sample showed two major, new peaks eluting before (P1) and after (L2) the native protein, which were interconvertible. Size-exclusion chromatography and electrophoresis documented that both the P1 and L2 fractions were irreversible dimers, formed by noncovalent interactions. A competition assay with interleukin-1 indicated that on a per monomer basis the P1 and L2 dimers retained about two-thirds of the activity of the native monomer. Infrared and far-UV circular dichroism spectroscopies showed that only minor alterations in secondary structure arose upon the formation of the P1 dimer. However, alteration in the near-UV circular dichroism spectrum suggested the presence of disulfide bonds in the P1 dimer, which are absent in the native protein. Mass spectroscopy and tryptic mapping, before and after carboxymethylation, demonstrated that the P1 dimer contained an intramolecular disulfide bond between Cys-66 and Cys-69. Although conversion of native protein to the P1 dimer was irreversible in buffer alone, the native monomer could be regained by denaturing the P1 dimer with guanidine hydrochloride and renaturing it by dialysis, suggesting that the intramolecular disulfide bond does not interfere with refolding. Analysis of the time course of P1 formation during storage at 30 degrees C indicated that the process followed first-order, and not second-order, kinetics, suggesting that the rate-limiting step was not dimerization. It is proposed that a conformational change in the monomer is the rate-limiting step in the formation of the P1 dimer degradation product. Sucrose stabilized the native monomer against this process. This result can be explained by the general stabilization mechanism for this additive, which is due to its preferential exclusion from the protein surface.

Published

1996

13. In vitro methionine oxidation of Escherichia coli-derived human stem cell factor: effects on the molecular structure, biological activity, and dimerization.

Author

Hsu YR, Narhi LO, Spahr C, Langley KE, and Lu HS

Subjects

Amino Acid Sequence, Chromatography, High Pressure Liquid, Circular Dichroism, Escherichia coli genetics, Humans, Hydrogen Peroxide chemistry, Hydrogen-Ion Concentration, Iodine Radioisotopes, Kinetics, Oxidants chemistry, Oxidation-Reduction, Peptide Fragments analysis, Peptide Fragments chemistry, Protein Structure, Tertiary, Proto-Oncogene Proteins c-kit metabolism, Radioligand Assay, Recombinant Proteins analysis, Recombinant Proteins chemistry, Recombinant Proteins genetics, Spectrometry, Fluorescence, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Spectrophotometry, Ultraviolet, Stem Cell Factor analysis, Stem Cell Factor genetics, Stem Cell Factor metabolism, Thymidine metabolism, Trypsin metabolism, Tumor Cells, Cultured, Methionine chemistry, Stem Cell Factor chemistry

Abstract

The effect of oxidation of the methionine residues of Escherichia coli-derived recombinant human stem cell factor (huSCF) to methionine sulfoxide on the structure and activity of SCF was examined. Oxidation was performed using hydrogen peroxide under acidic conditions (pH 5.0). The kinetics of oxidation of the individual methionine residues was determined by quantitation of oxidized and unoxidized methionine-containing peptides, using RP-HPLC of Asp-N endoproteinase digests. The initial oxidation rates for Met159, Met-1, Met27, Met36, and Met48 were 0.11 min-1, 0.098 min-1, 0.033 min-1, 0.0063 min-1, and 0.00035 min-1, respectively, when SCF was incubated in 0.5% H2O2 at room temperature. Although oxidation of these methionines does not affect the secondary structure of SCF, the oxidation of Met36 and Met48 affects the local structure as indicated by CD and fluorescence spectroscopy. The 295-nm Trp peak in the near-UV CD is decreased upon oxidation of Met36, and lost completely following the oxidation of Met48, indicating that the Trp44 environment is becoming significantly less rigid than it is in native SCF. Consistent with this result, the fluorescence spectra revealed that Trp44 becomes more solvent exposed as the methionines are oxidized, with the hydrophobicity of the Trp44 environment decreasing significantly. The oxidations of Met36 and Met48 decrease biological activity by 40% and 60%, respectively, while increasing the dissociation rate constant of SCF dimer by two- and threefold. These results imply that the oxidation of Met36 and Met48 affects SCF dimerization and tertiary structure, and decreases biological activity.

Published

1996

14. Refolding and oxidation of recombinant human stem cell factor produced in Escherichia coli.

Author

Jones MD, Narhi LO, Chang WC, and Lu HS

Subjects

Amino Acid Sequence, Chromatography, Gel, Chromatography, High Pressure Liquid, Circular Dichroism, Cloning, Molecular, Cysteine, Disulfides, Electrophoresis, Polyacrylamide Gel, Escherichia coli, Humans, Iodoacetates, Iodoacetic Acid, Kinetics, Light, Mutagenesis, Site-Directed, Oxidation-Reduction, Peptide Fragments chemistry, Peptide Fragments isolation & purification, Peptide Mapping, Point Mutation, Protein Denaturation, Recombinant Proteins chemistry, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Scattering, Radiation, Spectrometry, Fluorescence, Spectrophotometry, Ultraviolet, Stem Cell Factor isolation & purification, Protein Folding, Protein Structure, Secondary, Protein Structure, Tertiary, Stem Cell Factor chemistry, Stem Cell Factor metabolism

Abstract

Oxidative folding of recombinant human stem cell factor (rhSCF) produced in Escherichia coli was investigated in vitro. Folding of denatured and reduced rhSCF involves at least five intermediate forms, I-1 to I-5, detectable by their differences in hydrophobicity using reverse-phase high performance liquid chromatography. Both I-1 and I-2 contain a native-like disulfide bond, Cys4-Cys89 and Cys43-Cys138, respectively, and I-3 forms a mispaired disulfide, Cys43-Cys89. These forms appear to reach steady state equilibrium and are important folding intermediates. I-1 was found to be the prominent intermediate that directly folds into native rhSCF (N); and the thermodynamically less stable I-2 favors rearrangment into I-1. I-3 may serve as an intermediate for disulfide rearrangment between I-1 and I-2. I-4 and I-5, which are disulfide-linked dimers, are in equilibrium with reduced rhSCF and other intermediates and may not play an important role in rhSCF folding. Both trifluoroacetic acid-trapped I-1 and I-2, after isolation by high performance liquid chromatography, proceed with the remaining oxidative folding process after reconstitution. Iodoacetate-trapped I-1 and I-2 contain low alpha-helical content and some tertiary structure, while I-3 and reduced rhSCF have little ordered structure. Gel filtration/light-scattering experiments indicate that reduced rhSCF and iodoacetate-trapped I-1, I-2, and I-3 exist as dimeric forms, indicating that rhSCF dimerization precedes formation of disulfide bonds. I-1, I-2, I-3, and the C43,138A analog lacking Cys43-Cys138 bond are not biologically active or exhibit significantly lower activity. The two disulfide bonds in rhSCF seem to be essential for the molecule to maintain an active conformation required for its receptor binding and biological activities.

Published

1996

15. Isolation and characterization of a disulfide-linked human stem cell factor dimer. Biochemical, biophysical, and biological comparison to the noncovalently held dimer.

Author

Lu HS, Jones MD, Shieh JH, Mendiaz EA, Feng D, Watler P, Narhi LO, and Langley KE

Subjects

Amino Acid Sequence, Cells, Cultured, Chromatography, High Pressure Liquid, Cloning, Molecular, Colony-Forming Units Assay, Disulfides, Electrophoresis, Polyacrylamide Gel, Escherichia coli, Hematopoietic Stem Cells drug effects, Humans, Kinetics, Macromolecular Substances, Methionine, Models, Structural, Molecular Sequence Data, Peptide Fragments chemistry, Peptide Fragments isolation & purification, Peptide Mapping, Proto-Oncogene Proteins c-kit metabolism, Recombinant Proteins chemistry, Recombinant Proteins isolation & purification, Recombinant Proteins pharmacology, Stem Cell Factor isolation & purification, Stem Cell Factor pharmacology, Protein Structure, Secondary, Protein Structure, Tertiary, Stem Cell Factor chemistry

Abstract

Distinct from the noncovalently linked recombinant human stem call factor (rhSCF) dimer, we report here the isolation and identification of an SDS-nondissociable dimer produced during folding/oxidation of rhSCF. Experimental evidence using various cleavage strategies and analyses shows that the isolated dimer is composed of two rhSCF monomers covalently linked by four disulfide bonds. The cysteines are paired as in the noncovalently associated dimer except that all pairings are intermolecular rather than intramolecular. Other structural models, involving intertwining of intramolecular disulfide loops, are ruled out. The molecule behaves similarly to the noncovalently associated dimer during ion-exchange or gel permeation chromatography. However, the disulfide-linked dimer exhibits increased hydrophobicity in reverse-phase columns and in the native state does not undergo spontaneous dimer dissociation-association as seen for the noncovalent dimer. Spectroscopic analyses indicate that the disulfide-linked and noncovalently associated rhSCF dimers have grossly similar secondary and tertiary structures. In vitro, the disulfide-linked dimer exhibits approximately 3-fold higher biological activity in supporting growth of a hematopoietic cell line and stimulating hematopoietic cell colony formation from enriched human CD34+ cells. The molecule binds to the rhSCF receptor, Kit, with an efficiency only half that of the noncovalently associated dimer. Formation of intermolecular disulfides in the disulfide-linked dimer with retention of biological activity has implications for the three-dimensional structure of noncovalently held dimer and disulfide-linked dimer.

Published

1996

16. CD14: physical properties and identification of an exposed site that is protected by lipopolysaccharide.

Author

McGinley MD, Narhi LO, Kelley MJ, Davy E, Robinson J, Rohde MF, Wright SD, and Lichenstein HS

Subjects

Amino Acid Sequence, Animals, Antigens, CD isolation & purification, Antigens, Differentiation, Myelomonocytic isolation & purification, Binding Sites, CHO Cells, Chromatography, High Pressure Liquid, Circular Dichroism, Cricetinae, Humans, Lipopolysaccharide Receptors, Lipopolysaccharides isolation & purification, Mass Spectrometry, Molecular Sequence Data, Peptide Fragments chemistry, Peptide Fragments isolation & purification, Protein Conformation, Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins isolation & purification, Spectrometry, Fluorescence, Transfection, Antigens, CD chemistry, Antigens, CD metabolism, Antigens, Differentiation, Myelomonocytic chemistry, Antigens, Differentiation, Myelomonocytic metabolism, Lipopolysaccharides metabolism

Abstract

Soluble CD14 (sCD14) is a 55-kDa serum protein that binds lipopolysaccharide (LPS) and mediates LPS-dependent responses in a variety of cells. Using recombinant sCD14 expressed in Chinese hamster ovary (CHO) cells, we examined the structural characteristics of sCD14 and sCD14.LPS complexes. The circular dichroism and fluorescence spectra of the sCD14 indicate that it contains substantial beta-sheet (40%) and a well-defined tertiary structure with the tryptophan residues located in environments with different degrees of hydrophobicity and solvent exposure. The spectra of the sCD14.LPS complex are identical within experimental error to the uncomplexed sCD14. Changes in surface accessibility upon LPS binding were examined using limited proteolysis with endoproteinase Asp-N. This analysis revealed that aspartic acid residues at amino acids 57, 59, and 65 are susceptible to cleavage by Asp-N, while the same residues are protected from proteolytic cleavage in the sCD14.LPS complex. These results suggest that a region including amino acids 57 to 64 is involved in LPS binding by sCD14.

Published

1995

17. Identification of a lipopolysaccharide binding domain in CD14 between amino acids 57 and 64.

Author

Juan TS, Hailman E, Kelley MJ, Busse LA, Davy E, Empig CJ, Narhi LO, Wright SD, and Lichenstein HS

Subjects

Amino Acid Sequence, Animals, Antigens, CD isolation & purification, Antigens, Differentiation, Myelomonocytic isolation & purification, Base Sequence, Binding Sites, Cell Line, Chlorocebus aethiops, DNA Primers, Electrophoresis, Polyacrylamide Gel, Humans, Kidney, Kinetics, Lipopolysaccharide Receptors, Lipopolysaccharides pharmacology, Molecular Sequence Data, Mutagenesis, Site-Directed, Neutrophils drug effects, Peptide Fragments chemical synthesis, Recombinant Proteins chemistry, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Structure-Activity Relationship, Transfection, Antigens, CD chemistry, Antigens, CD metabolism, Antigens, Differentiation, Myelomonocytic chemistry, Antigens, Differentiation, Myelomonocytic metabolism, Lipopolysaccharides metabolism, Neutrophils physiology, Peptide Fragments pharmacology, Sequence Deletion

Abstract

CD14 is a 55-kDa glycoprotein which binds lipopolysaccharide (LPS) and enables LPS-dependent responses in a variety of cells. Recent limited proteolysis studies have implicated a region in CD14 between amino acids 57 and 64 as being involved in LPS interaction. To specifically assess the importance of this region with respect to LPS binding, we constructed a mutant sCD14 (sCD14 delta 57-64) lacking amino acids 57-64. sCD14 delta 57-64 was isolated from the serum-free conditioned medium of this cell line, and, in all assays, the purified protein failed to recognize LPS or enable LPS-dependent responses in cells. We also demonstrated that the region between amino acids 57 and 64 is required for binding of a neutralizing CD14 mAb, MEM-18. Native polyacrylamide gel electrophoresis assays were used to demonstrate that MEM-18 and LPS compete for the same binding site on CD14. These data strongly suggest that the region spanning amino acids 57-64 binds LPS and that formation of sCD14.LPS complex is required in order for sCD14-mediated responses to occur.

Published

1995

18. Studies on the structure and function of glycosylated and nonglycosylated neu differentiation factors. Similarities and differences of the alpha and beta isoforms.

Author

Lu HS, Chang D, Philo JS, Zhang K, Narhi LO, Liu N, Zhang M, Sun J, Wen J, and Yanagihara D

Subjects

3T3 Cells, Animals, CHO Cells, Circular Dichroism, Cricetinae, Escherichia coli genetics, Glycoproteins genetics, Glycoproteins metabolism, Glycosylation, Humans, Mice, Molecular Sequence Data, Molecular Weight, Neuregulins, Protein Processing, Post-Translational, Rats, Solutions, Spectrophotometry, Ultraviolet, Spectroscopy, Fourier Transform Infrared, Glycoproteins chemistry

Abstract

Comparative analyses of both glycosylated and nonglycosylated neu differentiation factor (NDF) isoforms revealed significant similarities and differences of their overall structures and functions. Biophysical analyses confirmed that all NDF isoforms are monomeric, but have an extended ellipsoidal shape in solution. All full-length NDFs are similar in secondary and tertiary structures and they contain no alpha-helix but are abundant in beta-strand structures. A small NDF fragment containing only the epidermal growth factor domain is also rich in beta-strand structures, but exhibits tertiary structure different from the long NDF forms. Monoclonal antibodies that selectively recognize epidermal growth factor domains of human NDF-alpha and -beta can specifically bind the respective NDF-alpha and -beta isoforms independent of NDF origins. Western blot analysis and quantitative binding assays further identify that an NDF preparation produced naturally from Rat1-EJ cells contains both alpha and beta isoforms in a 3 to 2 ratio. In receptor-binding competition experiments, human and rat NDF-beta isoforms have higher affinity than NDF-alpha isoforms. NDF-beta isoforms can dramatically enhance the stimulation of DNA synthesis for transfected NIH3T3 cells that overexpress HER-3 and HER-4 receptors, while NDF-alpha isoforms can only stimulate proliferation of HER-4-transfected cells with lower activity. Taken together, NDF-alpha and -beta isoforms share similar gross protein conformations but are biologically distinct.

Published

1995

19. Formation of heterodimers from three neurotrophins, nerve growth factor, neurotrophin-3, and brain-derived neurotrophic factor.

Author

Arakawa T, Haniu M, Narhi LO, Miller JA, Talvenheimo J, Philo JS, Chute HT, Matheson C, Carnahan J, and Louis JC

Subjects

3T3 Cells, Animals, Biological Assay, Brain-Derived Neurotrophic Factor, CHO Cells, Chickens, Chromatography, Ion Exchange, Circular Dichroism, Cricetinae, Electrophoresis, Polyacrylamide Gel, Ganglia, Spinal drug effects, Ganglia, Spinal physiology, Guanidine, Guanidines, Humans, Macromolecular Substances, Mice, Nerve Growth Factors biosynthesis, Nerve Growth Factors isolation & purification, Nerve Tissue Proteins biosynthesis, Nerve Tissue Proteins isolation & purification, Neurotrophin 3, Phosphorylation, Protein Denaturation, Receptor, Ciliary Neurotrophic Factor, Receptors, Nerve Growth Factor biosynthesis, Receptors, Nerve Growth Factor metabolism, Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins isolation & purification, Transfection, Nerve Growth Factors chemistry, Nerve Tissue Proteins chemistry, Protein Conformation, Protein Folding

Abstract

Three neurotrophic factors, brain-derived neurotrophic factor (BDNF), neurotrophin-3 (NT-3), and nerve growth factor (NGF) form noncovalent homodimers in solution. Since they are highly homologous proteins, it seemed probable that two monomers of these proteins might associate together to form a heterodimer. This was tested by denaturing the two different proteins together in 6 M guanidine HCl and refolding them in phosphate-buffered saline. When the refolded mixture of BDNF and NT-3 was subjected to Mono S cation exchange chromatography, a new peak was observed eluting between NT-3 and BDNF, which accounted for about 30% of the protein used. This new protein species migrated as a single band upon native gel electrophoresis with mobility between that of the NT-3 homodimer and the BDNF homodimer, indicating that a complex had been formed. Sedimentation equilibrium data show that the dissociation constant of this heterodimer is < 3 x 10(-10) M. The heterodimer was stable upon incubation at 37 degrees C in phosphate-buffered saline over 11 days. Having determined that the heterodimer is highly stable, it was subjected to various biological assays. Autophosphorylation assay using TrkB receptor showed that the heterodimer is indistinguishable from the BDNF or NT-3 homodimer in the ability to induce phosphorylation of the receptor. It was also indistinguishable from the homodimers in the neurotrophic activity using chick dorsal root ganglion explant. In the sympathetic neuron survival assay, the heterodimer behaved more similarly to NT-3, whereas in the dopamine uptake assay, it was intermediate between the two homodimers. In addition, the heterodimer was shown to be retrogradely transported in the dorsal root ganglion neurons. A heterodimer between NGF and BDNF is formed but much less effectively than the NT-3.BDNF heterodimer, and it is not stable even at 4 degrees C. These results indicate that BDNF and NT-3 have an intersubunit contact surface for dimerization resembling each other's but different from the contact surface of NGF.

Published

1994

20. Sites of iodination in recombinant human brain-derived neurotrophic factor and its effect on neurotrophic activity.

Author

Rosenfeld R, Philo JS, Haniu M, Stoney K, Rohde MF, Wu GM, Narhi LO, Wong C, Boone T, and Hawkins NN

Subjects

Amino Acid Sequence, Animals, Binding Sites, Brain-Derived Neurotrophic Factor, Chickens, Chromatography, High Pressure Liquid, Circular Dichroism, Ganglia drug effects, Ganglia ultrastructure, Humans, Macromolecular Substances, Mass Spectrometry, Molecular Sequence Data, Nerve Tissue Proteins chemistry, Nerve Tissue Proteins pharmacology, Pepsin A metabolism, Peptide Mapping, Protein Conformation, Recombinant Proteins metabolism, Sodium Iodide metabolism, Structure-Activity Relationship, Tyrosine metabolism, Ultracentrifugation, Iodine metabolism, Nerve Tissue Proteins metabolism

Abstract

Recombinant human brain-derived neurotrophic factor (BDNF) is now under extensive investigation because of its potential clinical applications. Radioactively labeled proteins are usually required to study receptor binding and pharmacokinetic properties of proteins. This study was undertaken to see if iodination affects the biological and conformational properties of a recombinant BDNF. BDNF was iodinated using a stoichiometric amount of nonradioactive cold NaI to minimize multiple iodinations. Of the four tyrosines present in BDNF--Tyr-52, Tyr-54, Tyr-63, and Tyr-86--only Tyr-63 and Tyr-86 were iodinated under the experimental conditions used. Iodination of Tyr-63 resulted in modification without alteration of the biological activity, whereas iodination of Tyr-86 resulted in a molecule with highly compromised biological activity. Similar inactivation was observed if both Tyr-63 and Tyr-86 were iodinated. These modified proteins exhibited conformation and dimerization apparently identical to those of the native protein, as demonstrated by analytical ultracentrifugation, gel filtration, light scattering, and circular dichroism. From these results, we concluded that Tyr-52 and Tyr-54 are not accessible to the reagent and are probably buried in the hydrophobic core, whereas Tyr-63 and Tyr-86 are exposed on the surface of the molecule; of the two exposed residues, only Tyr-86 contributes to the biological activity.

Published

1993

21. Recombinant human erythropoietin (rHuEPO): cross-linking with disuccinimidyl esters and identification of the interfacing domains in EPO.

Author

Haniu M, Narhi LO, Arakawa T, Elliott S, and Rohde MF

Subjects

Amino Acid Sequence, Animals, CHO Cells, Circular Dichroism, Cricetinae, Electrophoresis, Polyacrylamide Gel, Escherichia coli, Glycosylation, Humans, Macromolecular Substances, Molecular Sequence Data, Peptide Fragments chemistry, Peptide Mapping, Protein Conformation, Protein Structure, Secondary, Cross-Linking Reagents, Erythropoietin chemistry, Recombinant Proteins chemistry

Abstract

Several amino groups of recombinant human erythropoietin are selectively cross-linked by specific cross-linkers including disuccinimidyl suberate or dithiobis(succinimidyl propionate). Intramolecular cross-linkings are obtained without significant change of the protein conformation using appropriate concentrations (0.2 mM) of the cross-linkers, which possess an 11-12-A length of a spacer between two reacting groups. Intramolecularly cross-linked peptides obtained suggest that several amino groups in erythropoietin (EPO) are positioned at a distance of near 12 A in the solution state. These interfacing amino groups include Lys 20-Lys 154, Lys 45-Lys 140, Lys 52-Lys 154, Lys 52-Lys 140, and Ala 1-Lys 116. A comparison of the cross-linking results between nonglycosylated EPO and glycosylated EPO suggests that both proteins retain high similarity regarding protein conformation. These results fit a structural model similar to that of human growth hormone, in which four alpha-helical bundles and a long stretch of beta-sheet structure are involved in the active protein.

Published

1993

22. Comparison of the biophysical characteristics of human brain-derived neurotrophic factor, neurotrophin-3, and nerve growth factor.

Author

Narhi LO, Rosenfeld R, Talvenheimo J, Prestrelski SJ, Arakawa T, Lary JW, Kolvenbach CG, Hecht R, Boone T, and Miller JA

Subjects

Amino Acid Sequence, Animals, Brain-Derived Neurotrophic Factor, CHO Cells, Circular Dichroism, Cricetinae, Humans, Molecular Sequence Data, Nerve Growth Factors genetics, Nerve Tissue Proteins genetics, Neurotrophin 3, Protein Conformation, Recombinant Proteins chemistry, Sequence Homology, Amino Acid, Spectrum Analysis, Nerve Growth Factors chemistry, Nerve Tissue Proteins chemistry

Abstract

The structural properties of human brain-derived neurotrophic factor (BDNF) and neurotrophin-3 (NT-3) were studied using sedimentation equilibrium and circular dichroism (CD), fluorescence and Fourier-transform infrared spectroscopies, and compared with those of human nerve growth factor (NGF). Both the far UV CD and infrared spectra indicate that these three proteins have similar, but not identical, secondary structures which contain primarily beta-sheet and irregular structures. NGF appears to contain the most beta-sheet while NT-3 contains a small fraction of alpha-helix. The near UV CD spectra appear to indicate that the three proteins contain disulfide bonds in similar environments, suggesting a resemblance in tertiary structure. The fluorescent tryptophans found in the molecules are relatively solvent exposed, while Trp102 found only in NT-3 is possibly quenched. The fluorescent Trp(s) in NGF are significantly quenched relative to those in the other two neurotrophic factors. Both NT-3 and BDNF have very hydrophilic surfaces at neutral pH, as indicated by a low binding affinity to a hydrophobic probe, anilinonaphthalenesulfonate. Sedimentation equilibrium showed that BDNF, NT-3, and NGF exist as strongly associated dimers in phosphate-buffered saline, pH 7.1. Fits of the observed fringe displacements to various association models suggested that the BDNF, NT-3, and NGF samples contain, in addition to the principal dimeric species, some oligomers, and that NT-3 contains a small fraction of incompetent monomer.

Published

1993

23. Folding and oxidation of recombinant human granulocyte colony stimulating factor produced in Escherichia coli. Characterization of the disulfide-reduced intermediates and cysteine----serine analogs.

Author

Lu HS, Clogston CL, Narhi LO, Merewether LA, Pearl WR, and Boone TC

Subjects

Chromatography, High Pressure Liquid, Circular Dichroism, Copper chemistry, Copper Sulfate, Cysteine, Escherichia coli genetics, Fluorescence Polarization, Granulocyte Colony-Stimulating Factor genetics, Humans, Kinetics, Oxidation-Reduction, Protein Conformation, Receptors, Granulocyte Colony-Stimulating Factor, Recombinant Proteins chemistry, Recombinant Proteins genetics, Serine, Spectrophotometry, Ultraviolet, Granulocyte Colony-Stimulating Factor chemistry

Abstract

The folding and oxidation of recombinant human granulocyte colony-stimulating factor solubilized from Escherichia coli inclusion bodies was investigated. During the folding process, two intermediates, I1 and I2, were detected by kinetic studies using high performance liquid chromatography. I1 exists transiently and disappears quickly with the concomitant formation of I2. In contrast, I2 requires a longer time to fold into the final oxidized form, N. CuSO4 catalysis increases the folding rate of I2 from I1, while CuSO4 and elevated temperature (37 degrees C) have a dramatic effect on the folding rate of N from I2. These observations suggest the following sequential oxidative folding pathway. [sequence: see text] Peptide map analysis of the iodoacetate-labeled intermediates revealed that I1 represents the fully reduced granulocyte colony-stimulating factor containing 5 free cysteines; I2 is the partially oxidized species containing a single Cys36-Cys42 disulfide bond; and N, the final folded form, has two disulfide bonds. The physicochemical properties and biological activities of I1, I2, N, and several Cys----Ser analogs made by site-directed mutagenesis were further investigated. In guanidine hydrochloride-induced denaturation studies, the disulfide-reduced intermediates and the analogs missing either of the disulfide bonds are conformationally less stable than those of the wild type molecule or the analog with the free Cys at position 17 changed to Ser. Recombinant human granulocyte colony stimulating factor lacking either disulfide bond or both has overall secondary and tertiary structures different from those of the wild type molecule and exhibits lower biological activity. These studies show that disulfide bond formation is crucial for maintaining the molecule in a properly folded and biologically active form.

Published

1992

24. Cloning and characterization of a gene encoding extracellular metalloprotease from Streptomyces lividans.

Author

Lichenstein HS, Busse LA, Smith GA, Narhi LO, McGinley MO, Rohde MF, Katzowitz JL, and Zukowski MM

Subjects

Amino Acid Sequence, Base Sequence, Cloning, Molecular, DNA, Bacterial, Electrophoresis, Polyacrylamide Gel, Genomic Library, Hydrogen-Ion Concentration, Metalloendopeptidases metabolism, Molecular Sequence Data, Restriction Mapping, Sequence Alignment, Streptomyces enzymology, Temperature, Bacterial Proteins, Genes, Bacterial, Metalloendopeptidases genetics, Streptomyces genetics

Abstract

The prt gene, encoding a protease (Prt) from Streptomyces lividans TK24, was cloned and sequenced. An S. lividans host with plasmid-borne prt secreted 200 micrograms/ml of a 22-kDa Prt into the culture medium. Prt is classified as a metalloprotease since its activity is significantly inhibited by 1,10-phenanthroline or EDTA. The region upstream from prt codes for an incomplete open reading frame (ORF) oriented opposite to prt. This ORF has a strong similarity to a gene family (lysR) whose members regulate the transcription of structural genes required for either biosynthesis or degradation.

Published

1992

25. Solution structure and dynamics of epidermal growth factor and transforming growth factor alpha.

Author

Prestrelski SJ, Arakawa T, Wu CS, O'Neal KD, Westcott KR, and Narhi LO

Subjects

Circular Dichroism, Fourier Analysis, Humans, Oxidation-Reduction, Protein Conformation, Recombinant Proteins chemistry, Solutions, Spectrophotometry, Infrared, Epidermal Growth Factor chemistry, Transforming Growth Factor alpha chemistry

Abstract

Circular dichroism (CD) and Fourier transform infrared spectroscopic studies have shown that the secondary structure of transforming growth factor alpha (TGF-alpha) is very similar to that of epidermal growth factor (EGF). The infrared spectra revealed a minor difference between the two proteins, in particular in the beta-sheet structure. A large difference was observed with CD between the two proteins in the apparent conformation each adopts when the disulfide bonds are reduced. Reduced TGF-alpha showed a distinct alpha-helical conformation only at a high trifluoroethanol concentration, whereas reduced EGF assumed an alpha-helical conformation in the absence of trifluoroethanol. This indicates that these two proteins adopt different secondary structures in the absence of disulfide bonds, although they assume similar folding structures in their presence. These data suggest that the disulfide bonds to a large degree dictate the conformation of these two proteins. Additionally, differences in the dynamic behavior between EGF and TGF-alpha were also observed. Infrared experiments showed that the hydrogen-deuterium exchange rate is much higher for TGF-alpha than for EGF, indicating that TGF-alpha is a more flexible molecule. The rate of reduction of the disulfide bonds by dithiothreitol was also faster for TGF-alpha. Therefore, it can be concluded that although EGF and TGF-alpha have a similar overall conformation, TGF-alpha is a more flexible molecule than EGF.

Published

1992

26. The effect of carbohydrate on the structure and stability of erythropoietin.

Author

Narhi LO, Arakawa T, Aoki KH, Elmore R, Rohde MF, Boone T, and Strickland TW

Subjects

Animals, CHO Cells, Circular Dichroism, Cloning, Molecular, Cricetinae, Erythropoietin chemistry, Erythropoietin genetics, Escherichia coli genetics, Guanidine, Guanidines pharmacology, Hydrogen-Ion Concentration, Protein Conformation, Protein Denaturation, Temperature, Carbohydrate Metabolism, Erythropoietin metabolism

Abstract

Erythropoietin is a glycoprotein hormone that stimulates the maturation of late erythroid progenitor cells. It has three N-linked and one O-linked carbohydrates which play an important role in the biosynthesis and biological activities of the protein. To determine the role the carbohydrate might have in maintaining the conformational stability of the protein, the protein expressed in mammalian cells (fully glycosylated), the asialo mammalian-expressed protein, and the protein expressed in Escherichia coli (no carbohydrate) were compared for their stability to guanidine HCl, pH, and temperature. Circular dichroism was used to follow protein unfolding. Both the intact and asialo mammalian-expressed proteins unfolded with a cooperative transition in guanidine HCl, with a midpoint at 1.75 M guanidine HCl. The E. coli-expressed material unfolded with a midpoint of 1.2 M guanidine HCl, and a delta G of unfolding which was 1.4 kcal/mol less than that of the two glycosylated molecules. The E. coli-derived protein was also significantly less stable to pH-induced conformational changes, showing a cooperative transition in 35% glycerol with a midpoint at pH 4.4, while both the intact and asialo mammalian-expressed molecules had a transition midpoint of pH 3.75 in the absence of glycerol, and approximately pH 3 in the presence of 35% glycerol. The E. coli-expressed molecule unfolded and precipitated upon heating to 44 degrees C, while the asialo and intact mammalian-expressed proteins remained soluble, with a Tm of 56 degrees C. From these experiments, the carbohydrate appears to play a critical role in stabilizing the erythropoietin molecule to denaturing conditions, and this increased stability does not depend on the presence of sialic acid.

Published

1991

27. Glycosylated and unglycosylated recombinant-derived human stem cell factors are dimeric and have extensive regular secondary structure.

Author

Arakawa T, Yphantis DA, Lary JW, Narhi LO, Lu HS, Prestrelski SJ, Clogston CL, Zsebo KM, Mendiaz EA, and Wypych J

Subjects

Circular Dichroism, Electrophoresis, Polyacrylamide Gel, Glycoside Hydrolases metabolism, Glycosylation, Hematopoietic Cell Growth Factors chemistry, Humans, Molecular Weight, Protein Conformation, Recombinant Proteins metabolism, Solubility, Spectrometry, Fluorescence, Spectrophotometry, Infrared, Stem Cell Factor, Hematopoietic Cell Growth Factors metabolism, Stem Cells metabolism

Abstract

We have recently described the identification, isolation, and characterization of a factor, termed stem cell factor (SCF), which acts on primitive hematopoietic progenitors of the marrow. A soluble form of the factor was isolated from the conditioned medium of a rat cell line (Zsebo, K. M., Wypych, J., McNiece, I. K., Lu, H. S., Smith, K. A., Karkare, S. B., Sachdev, R. K., Yuschenkoff, V. N., Birkett, N. C., Williams, L. R., Satyagal, V. N., Tung, W., Bosselman, R. A., Mendiaz, E. A., and Langley, K. E. (1990) Cell 63, 195-201) and rat and human cDNAs have been cloned (Martin, F. H., Suggs, S. V., Langley, K. E., Lu, H. S., Ting, J., Okino, K. H., Morris, C. F., McNiece, I. K., Jacobsen, F. W., Mendiaz, E. A., Birkett, N. C., Smith, K. A., Johnson, M. J., Parker, V. P., Flores, J. C., Patel, A. C., Fisher, E. F., Erjavec, H. O., Herrera, C. J., Wypych, J., Sachdev, R. K., Pope, J. A., Leslie, I., Wen, D., Lin, C.-H., Cupples, R. L., and Zsebo, K. M. (1990) Cell 63, 203-211). The cDNAs encode amino acids C-terminal to those found in the isolated natural form, including a putative transmembrane domain. This paper describes the structural characterization of soluble forms of recombinant human SCF purified from Escherichia coli (unglycosylated) and from Chinese hamster ovary (CHO) cells (glycosylated). Fluorescence emission spectra indicate that the single Trp residue is present in a hydrophobic environment. Circular dichroism and infrared spectroscopy indicate considerable secondary structure, including both alpha-helix and beta-sheet. Molecular weight determinations by sedimentation equilibrium show that the molecules are dimeric (noncovalently associated), and gel filtration analyses are consistent with this conclusion. The CHO cell-derived SCF is about 30% carbohydrate by weight, with both N-linked and O-linked sugar. The presence or absence of the carbohydrate does not influence the results of the various structural analyses.

Published

1991

28. Characterization of a catalytically self-sufficient 119,000-dalton cytochrome P-450 monooxygenase induced by barbiturates in Bacillus megaterium.

Author

Narhi LO and Fulco AJ

Subjects

Amino Acid Sequence, Amino Acids analysis, Antibodies immunology, Cytochrome P-450 Enzyme System, Electrophoresis, Polyacrylamide Gel, Fatty Acids metabolism, Flavins analysis, Hydroxylation, Kinetics, Molecular Weight, NADH Dehydrogenase analysis, NADP pharmacology, Oxygenases analysis, Oxygenases immunology, Spectrophotometry, Substrate Specificity, Bacillus megaterium enzymology, Barbiturates pharmacology, Oxygenases isolation & purification

Abstract

A unique cytochrome P-450-dependent fatty acid monooxygenase from Bacillus megaterium ATCC 14581 is strongly induced by phenobarbital (Narhi, L. O., and Fulco, A. J. (1982) J. Biol. Chem. 257, 2147-2150) and many other barbiturates (Kim, B.-H., and Fulco, A. J. (1983) Biochem. Biophys. Res. Commun. 116, 843-850). This monooxygenase has now been purified to homogeneity from pentobarbital-induced bacteria as a single polypeptide with a molecular weight of 119,000 +/- 5,000 daltons. In the presence of NADPH and O2, it can catalyze the oxygenation of long chain fatty acids without the aid of any other protein. The enzyme has a catalytic center activity of 4,600 nmol of fatty acid oxygenated per nmol of P-450 (the highest activity yet reported for a P-450-dependent monooxygenase) and also functions as a highly active cytochrome c reductase in the presence of NADPH. The purified holoenzyme is a soluble protein containing 40 mol % hydrophobic amino acid residues and 1 mol each of FAD and FMN/mol of heme. It is isolated and purified in the low spin form but is converted to the high spin form in the presence of long chain fatty acids. The enzyme, which catalyzes the omega-2 hydroxylation of saturated fatty acids and the hydroxylation and epoxidation of unsaturated fatty acids has its highest affinity (Km = 2 +/- 1 microM) for the C15 and C16 chain lengths.

Published

1986

29. Identification and characterization of two functional domains in cytochrome P-450BM-3, a catalytically self-sufficient monooxygenase induced by barbiturates in Bacillus megaterium.

Author

Narhi LO and Fulco AJ

Subjects

Amino Acid Sequence, Bacillus megaterium drug effects, Cytochrome P-450 Enzyme System isolation & purification, Enzyme Induction, Macromolecular Substances, Mixed Function Oxygenases isolation & purification, Molecular Weight, NADPH-Ferrihemoprotein Reductase, Peptide Fragments analysis, Trypsin, Bacillus megaterium enzymology, Bacterial Proteins, Cytochrome P-450 Enzyme System biosynthesis, Mixed Function Oxygenases biosynthesis, Phenobarbital pharmacology

Abstract

In a previous publication (Narhi, L. O. and Fulco, A. J. (1986) J. Biol. Chem. 261, 7160-7169) we described the characterization of a soluble 119,000-dalton P-450 cytochrome (P-450BM-3) that was induced by barbiturates in Bacillus megaterium. This single polypeptide contained 1 mol each of FAD and FMN/mol of heme and, in the presence of NADPH and O2, catalyzed the oxygenation of long-chain fatty acids without the aid of any other protein. We have now utilized limited trypsin proteolysis in the presence of substrate to cleave P-450BM-3 into two polypeptides (domains) of about 66,000 and 55,000 daltons. The 66-kDa domain contains both FAD and FMN but no heme, reduces cytochrome c in the presence of NADPH, and is derived from the C-terminal portion of P-450BM-3. The 55-kDa domain is actually a mixture of three discrete peptides (T-I, T-II, and T-III) separable by high performance liquid chromatography. All three contain heme and show a P-450 absorption peak in the presence of CO and dithionite. The major component, T-I (Mr = 55 kDa), binds fatty acid substrate and has an N-terminal amino acid sequence identical to that of intact P-450BM-3, an indication that this domain constitutes the N-terminal portion of the 119-kDa protein. T-II (54 kDa) is the same as T-I except that it is missing the first nine N-terminal amino acids and does not bind substrate. T-III (Mr = 53.5 kDa) has lost the first 15 N-terminal residues and does not bind substrate. Since trypsin digestion of P-450BM-3 carried out in the absence of substrate yields T-II and T-III but no T-I, it appears that 1 or more residues of the first nine N-terminal amino acids of this protein are intimately involved in substrate binding. Although both the heme- and flavin-containing tryptic peptides retain their original half-reactions, fatty acid monooxygenase activity cannot be reconstituted after proteolysis, and the two domains, once separated, show no affinity for each other. In most respects, the reductase domain of P-450BM-3 more closely resembles the mammalian microsomal P-450 reductases than it does any known bacterial protein.

Published

1987

30. Phenobarbital induction of a soluble cytochrome P-450-dependent fatty acid monooxygenase in Bacillus megaterium.

Author

Narhi LO and Fulco AJ

Subjects

Bacillus megaterium drug effects, Cytochrome P-450 CYP4A, Enzyme Induction, Kinetics, Mixed Function Oxygenases, Bacillus megaterium enzymology, Cytochrome P-450 Enzyme System metabolism, Phenobarbital pharmacology

Abstract

A soluble, cytochrome P-450-dependent fatty acid hydroxylase-epoxidase isolated from Bacillus megaterium ATCC 14581 can be induced about 28-fold by the addition of phenobarbital (8 mM) to the growth medium. Phenobarbital is not a substrate for the enzyme nor does it activate the monooxygenase in the cell-free system. The level of the P-450-dependent monooxygenase activity in cultures harvested during the early stationary phase of growth increased linearly with phenobarbital concentration up to its solubility limit (8 mM) at 35 degrees C. The time course of induction during culture growth in the presence of 4 mM phenobarbital showed an interesting dichotomy. The specific content of cytochrome P-450 increased until the early stationary phase of growth and then leveled off. P-450-dependent monooxygenase activity, however, continued to increase rapidly to midstationary phase and then decreased just as rapidly after this time. At maximum specific activity, a turnover number of about 2,450 was obtained for palmitoleate hydroxylation-epoxidation by the cytochrome P-450 system.

Published

1982