Your search keyword '"Ross M. Taylor"' showing total 18 results

1. Enhanced Immunoaffinity Purification of Human Neutrophil Flavocytochrome B for Structure Determination by Electron Microscopy

Author

Ross M. Taylor, Algirdas J. Jesaitis, Marcia H. Riesselman, and Susan K. Brumfield

Subjects

0301 basic medicine, Molecular model, Chemistry, Negative stain, Heterotetramer, law.invention, 03 medical and health sciences, chemistry.chemical_compound, 030104 developmental biology, 0302 clinical medicine, Membrane, Transmission electron microscopy, law, 030220 oncology & carcinogenesis, Phosphatidylcholine, Microscopy, Biophysics, Electron microscope

Abstract

Determination of the structure of human neutrophil (PMN) flavocytochrome b (Cytb) is a necessary step for the understanding of the structure-function essentials of NADPH oxidase activity. This understanding is crucial for structure-driven therapeutic approaches addressing control of inflammation and infection. Our work on purification and sample preparation of Cytb has facilitated progress toward the goal of structure determination. Here we describe exploiting immunoaffinity purification of Cytb for initial examination of its size and shape by a combination of classical and cryoelectron microscopic (EM) methods. For these evaluations, we used conventional negative-stain transmission electron microscopy (TEM) to examine both detergent-solubilized Cytb as single particles and Cytb in phosphatidylcholine reconstituted membrane vesicles as densely packed random, partially ordered, and subcrystalline arrays. In preliminary trials, we also examined single particles by cryoelectron microscopy (cryoEM) methods. We conclude that Cytb in detergent and reconstituted in membrane is a relatively compact, symmetrical protein of about 100 A in maximum dimension. The negative stain, preliminary cryoEM, and crude molecular models suggest that the protein is probably a heterotetramer of two p22phox and gp91phox subunits in both detergent micelles and membrane vesicles. This exploratory study also suggests that high-resolution 2D electron microscopic approaches may be accessible to human material collected from single donors.

Published

2019

2. Single-step immunoaffinity purification and functional reconstitution of human phagocyte flavocytochrome b

Author

Marcia H. Riesselman, James B. Burritt, Jeannie M. Gripentrog, Algirdas J. Jesaitis, Connie I. Lord, and Ross M. Taylor

Subjects

Neutrophils, Detergents, Immunology, Chromatography, Affinity, Sepharose, Cell membrane, Epitopes, chemistry.chemical_compound, Glucosides, Antibody Specificity, Superoxides, NADPH oxidase complex, Catalytic Domain, Cell Line, Tumor, Phosphatidylcholine, medicine, Humans, Immunology and Allergy, Polyacrylamide gel electrophoresis, Integral membrane protein, Phospholipids, NADPH oxidase, Chromatography, biology, Chemistry, Cell Membrane, Antibodies, Monoclonal, NADPH Oxidases, Reproducibility of Results, Membranes, Artificial, Chromatography, Agarose, Cytochrome b Group, Membrane, medicine.anatomical_structure, Solubility, Biochemistry, biology.protein, Peptides

Abstract

Human neutrophil flavocytochrome b (Cyt b) is a heterodimeric, integral membrane protein that generates high levels of superoxide in the multisubunit NADPH oxidase complex. Since Cyt b is currently isolated in limited quantities, improved methods for purification from low levels of starting membranes (from both neutrophils and other expressing cell types) are important for the analysis of structure and catalytic mechanism. In the present study, the epitope-mapped monoclonal antibody CS9 was coupled to Sepharose beads and used as an affinity matrix for single-step immunoaffinity purification of Cyt b. Following solubilization of both human neutrophil and PLB-985 membrane fractions in the nonionic detergent octylglucoside, Cyt b was absorbed on the CS9-Sepharose affinity matrix and purified protein was eluted under non-denaturing conditions with an epitope-mimicking peptide. The high efficiency of this isolation procedure allowed Cyt b to be reproducibly purified from readily obtainable levels of starting membrane fractions (9x10(8) cell equivalents of neutrophil membranes and 2x10(9) cell equivalents of PLB-985 membranes). Since Cyt b could be affinity-purified in the detergent octylglucoside, high-level functional reconstitution was carried out directly on elution fractions by simple addition of solubilized phospholipid and subsequent dialysis for detergent removal. To our knowledge, this study describes the most efficient method for generating purified, functionally-reconstituted Cyt b and should facilitate analyses that require a highly-defined NADPH oxidase system.

Published

2008

3. Characterization of Surface Structure and p47phox SH3 Domain-Mediated Conformational Changes for Human Neutrophil Flavocytochrome b

Author

Edgar Pick, Algirdas J. Jesaitis, Thomas L. Leto, Marcia H. Riesselman, Linda C. McPhail, Jeannie M. Gripentrog, Yevgeny Berdichevsky, Connie I. Lord, and Ross M. Taylor

Subjects

Enzyme complex, NADPH oxidase, biology, Protein Conformation, Chemistry, Protein subunit, Antibodies, Monoclonal, NADPH Oxidases, Cytochrome b Group, environment and public health, Biochemistry, SH3 domain, src Homology Domains, enzymes and coenzymes (carbohydrates), Epitope mapping, Protein structure, biology.protein, Humans, Binding Sites, Antibody, Binding site, Integral membrane protein, Epitope Mapping

Abstract

The heterodimeric, integral membrane protein flavocytochrome b (Cyt b) is the catalytic core of the phagocyte NADPH oxidase and generates superoxide which plays a critical role in host defense. To better define the activation of superoxide production by this multisubunit enzyme complex, Cyt b-specific monoclonal antibodies (mAbs) and the p47phox SH3 domains (p47SH3AB) were used in the present study as probes to map surface structure and conformational dynamics in human neutrophil Cyt b. In pull-down and co-immunoprecipitation studies with detergent-solubilized Cyt b, the oxidase-inhibitory mAb CS9 was shown to share an overlapping binding site with p47SH3AB on the C-terminal region of the p22phox subunit. Similar studies demonstrated a surprising lack of overlap between the mAb 44.1 and CS9/p47SH3AB binding sites, and they indicated that the oxidase-inhibitory mAb NL7 binds a region physically separated from the p22phox C-terminal domain. Resonance energy transfer and size exclusion chromatography confirmed the above results for functionally reconstituted Cyt b and provided evidence that binding of both mAb CS9 and p47SH3AB altered the conformation of Cyt b. Further support that binding of the p47phox SH3 domains modulates the structure of Cyt b was obtained using a cell-free assay system where p47SH3AB enhanced superoxide production in the presence of a p67phox (1-212)-Rac1(Q61L) fusion protein. Taken together, this study further characterizes the structure of human neutrophil Cyt b in both detergent micelles and reconstituted membrane bilayers, and it provides evidence that the cytosolic regulatory subunit p47phox modulates the conformation of Cyt b (in addition to serving as an adapter protein) during oxidase activation.

Published

2007

4. Localization of hCAP-18 on the surface of chemoattractant-stimulated human granulocytes: analysis using two novel hCAP-18-specific monoclonal antibodies

Author

Jamal Stie, Connie I. Lord, Ross M. Taylor, Algirdas J. Jesaitis, Jeannie M. Gripentrog, James B. Burritt, and Andrew V. Jesaitis

Subjects

Neutrophils, medicine.drug_class, Immunology, Immunofluorescence, Monoclonal antibody, Epitope, Flow cytometry, Epitopes, chemistry.chemical_compound, Cathelicidins, medicine, Humans, Immunology and Allergy, Cytochalasin, Chemotactic Factors, medicine.diagnostic_test, biology, Lactoferrin, Antibodies, Monoclonal, Cell Biology, Alkaline Phosphatase, Molecular biology, N-Formylmethionine Leucyl-Phenylalanine, Blot, Protein Transport, Specific granule, chemistry, biology.protein, Epitope Mapping, Antimicrobial Cationic Peptides, Granulocytes, Protein Binding

Abstract

The well-described antimicrobial and immunoregulatory properties of human cathelicidin antimicrobial protein 18 (hCAP-18) derive in part from the ability of its proteolytic fragment, LL-37 (a.k.a. CAP-37), to associate with activated immune and epithelial cells during inflammation. We now show a stable association between hCAP-18 and the cell surface of formyl-Met-Leu-Phe (fMLF)-stimulated neutrophils using two novel hCAP-18-specific mAb, H7 and N9, which recognize a single 16-kDa band, identified by N-terminal sequencing and mass spectrometry as hCAP-18. Phage display analysis of epitope-binding sites showed that both mAb probably recognize a similar five amino acid sequence near the C terminus of the prodomain. Immunoblot analysis of degranulated neutrophil supernatants resulted in mAb recognition of the 14-kDa prodomain of hCAP-18. Subcellular fractionation of unstimulated neutrophils on density gradients showed expected cosedimentation of hCAP-18 with specific granule lactoferrin (LF). fMLF stimulation resulted in an average 25% release of specific granule hCAP-18, with ∼15% of the total cellular hCAP-18 recovered from culture media, and ∼10% and ∼75%, respectively, codistributing with plasma membrane alkaline phosphatase and specific granule LF. Surface association of hCAP-18 on fMLF-stimulated neutrophils was confirmed by immunofluorescence microscopy and flow cytometry analysis, which also suggested a significant up-regulation of surface hCAP-18 on cytochalasin B-pretreated, fully degranulated neutrophils. hCAP-18 surface association was labile to 10 mM NaOH treatment but resistant to 1 M NaCl and also partitioned into the detergent phase following Triton X-114 solubilization, possibly suggesting a stable association with one or more integral membrane proteins. We conclude that fMLF stimulation promotes redistribution of hCAP-18 to the surface of human neutrophils.

Published

2007

5. Functional Epitope on Human Neutrophil Flavocytochrome b558

Author

James B. Burritt, Charles A. Parkos, Travis D. Baughan, Danas Baniulis, John S. Mills, Algirdas J. Jesaitis, Dirk Roos, Thomas R. Foubert, Connie I. Lord, Ross M. Taylor, and Landsteiner Laboratory

Subjects

Neutrophils, Immunology, Granulomatous Disease, Chronic, Epitope, Epitopes, chemistry.chemical_compound, NADPH oxidase complex, Humans, Immunology and Allergy, Binding site, Oxidase test, Membrane Glycoproteins, NADPH oxidase, biology, Superoxide, Antibodies, Monoclonal, NADPH Oxidases, Cytochrome b Group, Phosphoproteins, Molecular biology, Peptide Fragments, rac GTP-Binding Proteins, Enzyme Activation, Protein Transport, Epitope mapping, chemistry, NADPH Oxidase 2, biology.protein, NADPH binding, Binding Sites, Antibody, Protein Binding

Abstract

mAb NL7 was raised against purified flavocytochrome b558, important in host defense and inflammation. NL7 recognized the gp91phox flavocytochrome b558 subunit by immunoblot and bound to permeabilized neutrophils and neutrophil membranes. Epitope mapping by phage display analysis indicated that NL7 binds the 498EKDVITGLK506 region of gp91phox. In a cell-free assay, NL7 inhibited in vitro activation of the NADPH oxidase in a concentration-dependent manner, and had marginal effects on the oxidase substrate Michaelis constant (Km). mAb NL7 did not inhibit translocation of p47phox, p67phox, or Rac to the plasma membrane, and bound its epitope on gp91phox independently of cytosolic factor translocation. However, after assembly of the NADPH oxidase complex, mAb NL7 bound the epitope but did not inhibit the generation of superoxide. Three-dimensional modeling of the C-terminal domain of gp91phox on a corn nitrate reductase template suggests close proximity of the NL7 epitope to the proposed NADPH binding site, but significant separation from the proposed p47phox binding sites. We conclude that the 498EKDVITGLK506 segment resides on the cytosolic surface of gp91phox and represents a region important for oxidase function, but not substrate or cytosolic component binding.

Published

2003

6. Full Subunit Coverage Liquid Chromatography Electrospray Ionization Mass Spectrometry (LCMS+) of an Oligomeric Membrane Protein

Author

Rodrigo Aguilera, Ross M. Taylor, William A. Cramer, Julian P. Whitelegge, and Huamin Zhang

Subjects

Cytochrome f, Chromatography, biology, Protein mass spectrometry, Chemistry, Cytochrome b6f complex, Electrospray ionization, Protein subunit, food and beverages, Tandem mass spectrometry, Mass spectrometry, biology.organism_classification, Biochemistry, Analytical Chemistry, Spinach, Molecular Biology

Abstract

Highly active cytochrome b6f complexes from spinach and the cyanobacterium Mastigocladus laminosus have been analyzed by liquid chromatography with electrospray ionization mass spectrometry (LCMS+). Both size-exclusion and reverse-phase separations were used to separate protein subunits allowing measurement of their molecular masses to an accuracy exceeding 0.01% (±3 Da at 30,000 Da). The products of petA, petB, petC, petD, petG, petL, petM, and petN were detected in complexes from both spinach and M. laminosus, while the spinach complex also contained ferredoxin-NADP+ oxidoreductase (Zhang, H., Whitelegge, J. P., and Cramer, W. A. (2001) Flavonucleotide:ferredoxin reductase is a subunit of the plant cytochrome b6f complex. J. Biol. Chem. 276, 38159–38165). While the measured masses of PetC and PetD (18935.8 and 17311.8 Da, respectively) from spinach are consistent with the published primary structure, the measured masses of cytochrome f (31934.7 Da, PetA) and cytochrome b (24886.9 Da, PetB) modestly deviate from values calculated based upon genomic sequence and known post-translational modifications. The low molecular weight protein subunits have been sequenced using tandem mass spectrometry (MSMS) without prior cleavage. Sequences derived from the MSMS spectra of these intact membrane proteins in the range of 3.2–4.2 kDa were compared with translations of genomic DNA sequence where available. Products of the spinach chloroplast genome, PetG, PetL, and PetN, all retained their initiating formylmethionine, while the nuclear encoded PetM was cleaved after import from the cytoplasm. While the sequences of PetG and PetN revealed no discrepancy with translations of the spinach chloroplast genome, Phe was detected at position 2 of PetL. The spinach chloroplast genome reports a codon for Ser at position 2 implying the presence of a DNA sequencing error or a previously undiscovered RNA editing event. Clearly, complete annotation of genomic data requires detailed expression measurements of primary structure by mass spectrometry. Full subunit coverage of an oligomeric intrinsic membrane protein complex by LCMS+ presents a new facet to intact mass proteomics.

Published

2002

7. Invariant local conformation in p22phox p.Y72H polymorphisms suggested by mass spectral analysis of crosslinked human neutrophil flavocytochrome b

Author

Ross M. Taylor, Algirdas J. Jesaitis, and Edward A. Dratz

Subjects

Neutrophils, Protein subunit, Biochemistry, Mass Spectrometry, Article, chemistry.chemical_compound, medicine, Humans, Structural motif, Integral membrane protein, Oxidase test, NADPH oxidase, Polymorphism, Genetic, biology, Superoxide, NADPH Oxidases, General Medicine, Trypsin, Cytochrome b Group, Cross-Linking Reagents, chemistry, biology.protein, P22phox, Reactive Oxygen Species, medicine.drug

Abstract

The NADPH oxidase of phagocytic leukocytes generates superoxide that plays a critical role in innate immunity and inflammatory responses. The integral membrane protein flavocytochrome b (Cyt b, a.k.a. cytochrome b(558/559)) is the catalytic core of the complex and serves as a prototype for homologs important in regulating signaling networks in a wide variety of animal and plant cells. Our analysis identifies a naturally-occurring Tyr72/His72 polymorphism (p.Y72H) in the p22(phox) subunit of Cyt b at the protein level that has been recognized at the nucleotide level (c.214T > C, formerly C242T) and implicated in cardiovascular disease. In the present study, Cyt b was isolated from human neutrophils and reacted with chemical crosslinkers for subsequent structure analysis by MALDI mass spectrometry. Following mild chemical modification of Cyt b with two pairs of isotopically-differentiated lysine crosslinkers: BS(2)G-d(0)/d(4) and BS(3)-d(0)/d(4), the reaction mixtures were digested with trypsin and purified on C(18)ZipTips to generate samples for mass analysis. MALDI analysis of tryptic digests from each of the above reactions revealed a series of masses that could be assigned to p22(phox) residues 68-85, assuming an intra-molecular crosslink between Lys71 and Lys78. In addition to the 30 ppm mass accuracy obtained with internal mass calibration, increased confidence in the assignment of the crosslinks was provided by the presence of the diagnostic mass patterns resulting from the isotopically-differentiated crosslinking reagent pairs and the Tyr72/His72 p22(phox) polymorphisms in the crosslinked peptides. This work identifies a novel, low-resolution distance constraint in p22(phox) and suggests that the medically-relevant p.Y72H polymorphism has an invariant structural motif in this region. Because position 72 in p22(phox) lies outside regions identified as interactive with other oxidase components, the structural invariance also provides additional support for maturational differences as the source of the wide variation in observed reactive oxygen species production by cells expressing p.Y72H.

Published

2011

8. Immunoaffinity Purification of Human Phagocyte Flavocytochrome b and Analysis of Conformational Dynamics

Author

Algirdas J. Jesaitis and Ross M. Taylor

Subjects

chemistry.chemical_classification, Reactive oxygen species, Enzyme complex, NADPH oxidase, biology, Phagocyte, Cytochrome b, Superoxide, enzymes and coenzymes (carbohydrates), chemistry.chemical_compound, medicine.anatomical_structure, chemistry, Biochemistry, NADPH oxidase complex, biology.protein, medicine, Integral membrane protein

Abstract

The heterodimeric integral membrane protein flavocytochrome b (Cyt b) is the catalytic core of the phagocyte NADPH oxidase, an enzyme complex that initiates a cascade of reactive oxygen species critical for the elimination of infectious agents. Many fundamental questions remain concerning the structure and catalytic mechanism of Cyt b, largely because of the inability to isolate this protein in quantities required for both biochemical analysis and meaningful attempts at high-resolution structure determination. In order to facilitate the direct analysis of Cyt b, the following method describes a rapid and efficient procedure for the immunoaffinity purification of Cyt b (under nondenaturing conditions) from neutrophil membrane fractions. The protocol presented here contains a number of steps that have been optimized and improved since the original description of this Cyt b isolation method. In order to address questions concerning the mechanism of superoxide generation by the NADPH oxidase complex, methods are additionally presented for analysis of conformational dynamics of immunoaffinity-purified Cyt b by resonance energy transfer.

Published

2007

9. Analysis of human phagocyte flavocytochrome b(558) by mass spectrometry

Author

James B. Burritt, Connie I. Lord, Marcia H. Riesselman, Edward A. Dratz, Brian Bothner, Gilda F. Linton, Thomas E. Angel, Algirdas J. Jesaitis, Jeannie M. Gripentrog, Harry L. Malech, Danas Baniulis, Ross M. Taylor, and Walid S. Maaty

Subjects

Glycosylation, Neutrophils, Protein subunit, Population, Molecular Sequence Data, Peptide, Mass spectrometry, Biochemistry, chemistry.chemical_compound, Phagocytosis, Superoxides, Humans, Trypsin, Amino Acid Sequence, education, Molecular Biology, Integral membrane protein, chemistry.chemical_classification, Chryseobacterium, education.field_of_study, NADPH oxidase, Membrane Glycoproteins, biology, NADPH Oxidases, Cell Biology, Cytochrome b Group, Recombinant Proteins, Transmembrane domain, Mannosyl-Glycoprotein Endo-beta-N-Acetylglucosaminidase, chemistry, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, NADPH Oxidase 2, biology.protein

Abstract

The catalytic core of the phagocyte NADPH oxidase is a heterodimeric integral membrane protein (flavocytochrome b (Cyt b)) that generates superoxide and initiates a cascade of reactive oxygen species critical for the host inflammatory response. In order to facilitate structural characterization, the present study reports the first direct analysis of human phagocyte Cyt b by matrix-assisted laser desorption/ionization and nanoelectrospray mass spectrometry. Mass analysis of in-gel tryptic digest samples provided 73% total sequence coverage of the gp91(phox) subunit, including three of the six proposed transmembrane domains. Similar analysis of the p22(phox) subunit provided 72% total sequence coverage, including assignment of the hydrophobic N-terminal region and residues that are polymorphic in the human population. To initiate mass analysis of Cyt b post-translational modifications, the isolated gp91(phox) subunit was subject to sequential in-gel digestion with Flavobacterium meningosepticum peptide N-glycosidase F and trypsin, with matrix-assisted laser desorption/ionization and liquid chromatography-mass spectrometry/mass spectrometry used to demonstrate that Asn-132, -149, and -240 are genuinely modified by N-linked glycans in human neutrophils. Since the PLB-985 cell line represents an important model system for analysis of the NADPH oxidase, methods were developed for the purification of Cyt b from PLB-985 membrane fractions in order to confirm the appropriate modification of N-linked glycosylation sites on the recombinant gp91(phox) subunit. This study reports extensive sequence coverage of the integral membrane protein Cyt b by mass spectrometry and provides analytical methods that will be useful for evaluating posttranslational modifications involved in the regulation of superoxide production.

Published

2006

10. Evaluation of two anti-gp91phox antibodies as immunoprobes for Nox family proteins: mAb 54.1 recognizes recombinant full-length Nox2, Nox3 and the C-terminal domains of Nox1-4 and cross-reacts with GRP 58

Author

Yoko Nakano, Botond Banfi, William M. Nauseef, James B. Burritt, Guangjie Cheng, David Lambeth, Danas Baniulis, Algirdas J. Jesaitis, and Ross M. Taylor

Subjects

medicine.drug_class, Protein subunit, Immunoblotting, Molecular Sequence Data, Biophysics, Protein Disulfide-Isomerases, Sequence alignment, Monoclonal antibody, Transfection, Biochemistry, Epitope, Analytical Chemistry, law.invention, Cell Line, Epitopes, law, medicine, Escherichia coli, Humans, Electrophoresis, Gel, Two-Dimensional, Amino Acid Sequence, Cloning, Molecular, Molecular Biology, Peptide sequence, Heat-Shock Proteins, Membrane Glycoproteins, biology, Chemistry, NOX4, Antibodies, Monoclonal, Membrane Proteins, NADPH Oxidases, Chromatography, Agarose, Molecular biology, Molecular Probes, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, NADPH Oxidase 2, Recombinant DNA, biology.protein, Antibody, Sequence Alignment

Abstract

Progress in the study of Nox protein expression has been impeded because of the paucity of immunological probes. The large subunit of human phagocyte flavocytochrome b558 (Cytb), gp91phox, is also the prototype member of the recently discovered family of NADPH oxidase (Nox) proteins. In this study, we have evaluated the use of two anti-gp91phox monoclonal antibodies, 54.1 and CL5, as immunoprobes for Nox family proteins. Sequence alignment of gp91phox with Nox1, Nox3 and Nox4 identified regions of the Nox proteins that correspond to the gp91phox epitopes recognized by mAb 54.1 and CL5. Antibody 54.1 produced positive immunoblots of recombinant C-terminal fragments of these homologous proteins expressed in E. coli. Furthermore, only mAb 54.1 recognized full-length murine and human Nox3 expressed in HEK-293 cells, in immunoblots of alkali-stripped or detergent-solubilized membranes. 54.1 recognized Nox3 expression-specific proteins with Mr 30,000, 50,000, 65,000 and 88,000 for the murine protein and Mr of 38,000-58,000, 90,000, 100,000-130,000 and a broad species of higher than 160,000 for the human protein. We conclude that mAb 54.1 can serve as a probe of Nox3 and possibly other Nox proteins, if precautions are taken to remove GRP 58 and other crossreactive membrane-associated or detergent-insoluble proteins from the sample to be probed.

Published

2005

11. Unusual polyclonal anti-gp91 peptide antibody interactions with X-linked chronic granulomatous disease-derived human neutrophils are not from compensatory expression of Nox proteins 1, 3, or 4

Author

Ross M. Taylor, Paul G. Heyworth, Karl-Eric Magnusson, Vladas A. Bumelis, James B. Burritt, William M. Nauseef, Algirdas J. Jesaitis, Danas Baniulis, and Mary C. Dinauer

Subjects

Male, Heterozygote, Phagocyte, Protein family, Neutrophils, Peptide, Biology, Granulomatous Disease, Chronic, Antibodies, Antigen-Antibody Reactions, Epitopes, Chronic granulomatous disease, Affinity chromatography, medicine, Humans, Amino Acid Sequence, Gene, chemistry.chemical_classification, Membrane Glycoproteins, Membrane Proteins, NADPH Oxidases, Hematology, General Medicine, medicine.disease, Cytochrome b Group, Molecular biology, medicine.anatomical_structure, chemistry, Polyclonal antibodies, NADPH Oxidase 4, NADPH Oxidase 2, biology.protein, NADPH Oxidase 1, Female, Antibody, Peptides

Abstract

polyclonal anti-gp91 phox peptide antibody interactions with X-linked chronic granulomatous disease-derived human neutrophils are not from compensatory expression of Nox proteins 1, 3, or 4. Eur J Haematol 2005: 74: 241-249. � Blackwell Munksgaard 2005. Abstract: To obtain topological information about human phagocyte flavocytochrome b558 (Cytb), rabbit anti-peptide antibodies were raised against synthetic peptides mimicking gp91 phox regions: 1-9 (MGN), 30- 44 (YRV), 150-159 (ESY), 156-166 (ARK), 247-257 (KIS-1, KIS-2). Following affinity purification on immobilized peptide matrices, all antibodies but not prebleed controls recognized purified detergent-sol- ubilized Cytb by enzyme-linked immunosorbent assay (ELISA). Affin- ity-purified antibodies recognizing KIS, ARK and ESY but not YRV, MGN or prebleed IgG specifically detected gp91 phox in immunoblot analysis. Antibodies recognizing MGN, ESY, ARK and KIS but not YRV or the prebleed IgG fraction labeled intact normal neutrophils. Surprisingly, all antibodies, with the exception of YRV and pre-immune IgG controls, bound both normal and Cytb-negative neutrophils from the obligate heterozygous mother of a patient with X-linked chronic granulomatous disease (X-CGD) and all neutrophils from another pa- tient lacking the gp91 phox gene. Further immunochemical examination of membrane fractions derived from nine genetically unrelated patients with X-CGD, using an antibody that recognizes other Nox protein family members, suggests that the unusual reactivity observed does not reflect the compensatory expression of gp91 phox homologs Nox1, 3 or 4. These results suggest that an unusual surface reactivity exists on neu- trophils derived from X-linked chronic granulomatous disease patients that most likely extends to normal neutrophils as well. The study

Published

2005

12. Site-specific inhibitors of NADPH oxidase activity and structural probes of flavocytochrome b: characterization of six monoclonal antibodies to the p22phox subunit

Author

Mary C. Dinauer, James B. Burritt, Ross M. Taylor, Danas Baniulis, Connie I. Lord, Charles A. Parkos, Thomas R. Foubert, and Algirdas J. Jesaitis

Subjects

Models, Molecular, Enzyme complex, Phage display, medicine.drug_class, viruses, Protein subunit, Immunology, Detergents, Molecular Sequence Data, Monoclonal antibody, Epitope, Mice, Inovirus, Antibody Specificity, Peptide Library, Catalytic Domain, Membrane Transport Modulators, medicine, Fluorescence Resonance Energy Transfer, Immunology and Allergy, Animals, Humans, Amino Acid Sequence, Binding site, Enzyme Inhibitors, Oxidase test, NADPH oxidase, biology, Chemistry, NADPH Dehydrogenase, Antibodies, Monoclonal, Membrane Transport Proteins, NADPH Oxidases, Cytochrome b Group, Flow Cytometry, Phosphoproteins, Molecular biology, Protein Subunits, Biochemistry, Solubility, biology.protein, Binding Sites, Antibody, Epitope Mapping

Abstract

The integral membrane protein flavocytochrome b (Cyt b) is the catalytic core of the human phagocyte NADPH oxidase, an enzyme complex that initiates a cascade of reactive oxygen species important in the elimination of infectious agents. This study reports the generation and characterization of six mAbs (NS1, NS2, NS5, CS6, CS8, and CS9) that recognize the p22phox subunit of the Cyt b heterodimer. Each of the mAbs specifically detected p22phox by Western blot analysis but did not react with intact neutrophils in FACS studies. Phage display mapping identified core epitope regions recognized by mAbs NS2, NS5, CS6, CS8, and CS9. Fluorescence resonance energy transfer experiments indicated that mAbs CS6 and CS8 efficiently compete with Cascade Blue-labeled mAb 44.1 (a previously characterized, p22phox-specific mAb) for binding to Cyt b, supporting phage display results suggesting that all three Abs recognize a common region of p22phox. Energy transfer experiments also suggested the spatial proximity of the mAb CS9 and mAb NS1 binding sites to the mAb 44.1 epitope, while indicating a more distant proximity between the mAb NS5 and mAb 44.1 epitopes. Cell-free oxidase assays demonstrated the ability of mAb CS9 to markedly inhibit superoxide production in a concentration-dependent manner, with more moderate levels of inhibition observed for mAbs NS1, NS5, CS6, and CS8. A combination of computational predictions, available experimental data, and results obtained with the mAbs reported in this study was used to generate a novel topology model of p22phox.

Published

2004

13. Anionic amphiphile and phospholipid-induced conformational changes in human neutrophil flavocytochrome b observed by fluorescence resonance energy transfer

Author

Ross M. Taylor, James B. Burritt, Algirdas J. Jesaitis, Thomas R. Foubert, Linda C. McPhail, and Danas Baniulis

Subjects

Anions, Neutrophils, Protein Conformation, Biophysics, Phospholipid, Biochemistry, Fluorescence, chemistry.chemical_compound, Epitopes, Surface-Active Agents, Organophosphorus Compounds, NADPH oxidase complex, Fluorescence Resonance Energy Transfer, Organometallic Compounds, Humans, Phospholipids, Diacylglycerol kinase, Phosphatidylethanolamine, Quenching (fluorescence), Arachidonic Acid, Superoxide, Structure, Antibodies, Monoclonal, NADPH Oxidases, Sodium Dodecyl Sulfate, Cell Biology, Phosphatidylserine, Phosphatidic acid, Cytochrome b Group, Precipitin Tests, chemistry, Flavocytochrome b, Amphiphile

Abstract

The integral membrane protein flavocytochrome b (Cyt b) comprises the catalytic core of the human phagocyte NADPH oxidase complex and serves to initiate a cascade of reactive oxygen species that participate in the elimination of infectious agents. Superoxide production by the NADPH oxidase complex has been shown to be specifically regulated by the enzymatic generation of lipid second messengers following phagocyte activation. In the present study, a Cyt b-specific monoclonal antibody (mAb 44.1) was labeled with Cascade Blue (CCB) and used in resonance energy transfer (RET) studies probing the effects of a panel of lipid species on the structure of Cyt b. The binding of CCB-mAb 44.1 to immunoaffinity-purified Cyt b was both highly specific and resulted in significant quenching of the steady state donor fluorescence. Titration of the CCB-mAb 44.1:Cyt b complex with the anionic amphiphile lithium dodecyl sulfate (LDS) resulted in a saturable relaxation of fluorescence quenching due to conformational changes in Cyt b at concentrations of the amphiphile required for maximum rates of superoxide production by Cyt b in cell-free assays. Similar results were observed for the anionic amphiphile arachidonic acid (AA), although no relaxation of fluorescence quenching was observed for arachidonate methyl ester (AA-ME). Saturable relaxation of fluorescence quenching was also observed with the anionic, 18:1 phospholipids phosphatidic acid (DOPA) and phosphatidylserine (DOPS), while no relaxation was observed upon addition of the neutral 18:1 lipids phosphatidylcholine (DOPC), phosphatidylethanolamine (DOPE) or diacylglycerol (DAG) at similar levels. Further examination of a variety of phosphatidic acid (PA) species demonstrated DOPA to both potently induce conformational changes in Cyt b and to cause more dramatic conformational changes than PA species with shorter, saturated acyl chains. The data presented in this study support the hypothesis that second messenger lipids, such as AA and PA, directly bind to flavocytochrome b and modulate conformational states relevant to the activation of superoxide production.

Published

2003

14. Cascade blue as a donor for resonance energy transfer studies of heme-containing proteins

Author

James B. Burritt, Jan Sunner, Algirdas J. Jesaitis, Ross M. Taylor, Thomas R. Foubert, and Baiwei Lin

Subjects

Hemeproteins, Quenching (fluorescence), Magnetic Resonance Spectroscopy, biology, Cytochrome c, Electrospray ionization, Biophysics, Cytochrome c Group, Cell Biology, Photochemistry, Biochemistry, Fluorescence, chemistry.chemical_compound, Förster resonance energy transfer, Organophosphorus Compounds, Spectrometry, Fluorescence, chemistry, biology.protein, Organometallic Compounds, Animals, Denaturation (biochemistry), Azide, Molecular Biology, Heme, Fluorescent Dyes

Abstract

Cascade Blue acetyl azide is an amine reactive compound with spectral properties ideally suited for fluorescence resonance energy transfer (FRET) studies in which heme prosthetic groups serve as acceptors. To demonstrate utility of the Cascade Blue–heme spectroscopic ruler, cytochrome c was employed as a test case to calibrate distance measurements obtained from FRET analysis. Following modification, stoichiometrically labeled cytochrome c was digested with trypsin and derivatized fragments were analyzed by matrix-assisted laser desorption/ionization and electrospray ionization mass spectrometry to identify Lys25 as the predominant site of covalent modification. FRET analysis on derivatized protein demonstrated nearly complete quenching of Cascade Blue fluorescence, indicating the labeled lysine residue to reside within 30 A of the heme prosthetic group. Sodium dodecyl sulfate (SDS) denaturation resulted in an approximately 28% recovery of fluorescence, demonstrating the utility of this donor–acceptor pair for evaluating distance changes of ∼30–90 A. Modeling the Cascade Blue donor molecule onto Lys25 of a cytochrome c NMR structure confirmed a distance of ≤30 A from the heme acceptor, as determined by FRET analysis. Further modeling of the SDS-denatured state as an extended chain suggested a maximum separation distance of ∼45 A, also consistent with results derived from FRET analysis.

Published

2002

15. Identification of a spectrally stable proteolytic fragment of human neutrophil flavocytochrome b composed of the NH2-terminal regions of gp91(phox) and p22(phox)

Author

Ross M. Taylor, James B. Burritt, Thomas R. Foubert, Justin B. Bleazard, Jeannie M. Gripentrog, Algirdas J. Jesaitis, and Danas Baniulis

Subjects

Silver Staining, Glycosylation, Time Factors, Neutrophils, Octoxynol, Size-exclusion chromatography, Detergents, Immunoblotting, Heme, Alkylation, Biochemistry, Absorbance, chemistry.chemical_compound, Humans, Amino Acids, Molecular Biology, Chromatography, High Pressure Liquid, Gel electrophoresis, Membrane Glycoproteins, biology, Chemistry, Cell Membrane, NADPH Dehydrogenase, Membrane Transport Proteins, NADPH Oxidases, Cell Biology, Cytochrome b Group, Phosphoproteins, Molecular biology, Protein Structure, Tertiary, Electrophoresis, NADPH Oxidase 2, biology.protein, Electrophoresis, Polyacrylamide Gel, P22phox, Digestion, Protein Binding

Abstract

A heme-bearing polypeptide core of human neutrophil flavocytochrome b(558) was isolated by applying high performance, size exclusion, liquid chromatography to partially purified Triton X-100-solubilized flavocytochrome b that had been exposed to endoproteinase Glu-C for 1 h. The fragment was composed of two polypeptides of 60-66 and 17 kDa by SDS-polyacrylamide gel electrophoresis and retained a native heme absorbance spectrum that was stable for several days when stored at 4 degrees C in detergent-containing buffer. These properties suggested that the majority of the flavocytochrome b heme environment remained intact. Continued digestion up to 4.5 h yielded several heme-associated fragments that were variable in composition between experiments. Digestion beyond 4.5 h resulted in a gradual loss of recoverable heme. N-Linked deglycosylation and reduction and alkylation of the 1-h digestion fragment did not affect the electrophoretic mobility of the 17-kDa fragment but reduced the 60-66-kDa fragment to 39 kDa. Sequence and immunoblot analyses identified the fragments as the NH(2)-terminal 320-363 amino acid residues of gp91(phox) and the NH(2)-terminal 169-171 amino acid residues of p22(phox). These findings provide direct evidence that the primarily hydrophobic NH(2)-terminal regions of flavocytochrome b are responsible for heme ligation.

Published

2001

16. Folded state of the integral membrane colicin E1 immunity protein in solvents of mixed polarity

Author

Stanislav D. Zakharov, and Mark E. Girvin, J. Bernard Heymann, William A. Cramer, and Ross M. Taylor

Subjects

Circular dichroism, Protein Folding, Molecular Sequence Data, Colicins, Biochemistry, Protein Structure, Secondary, Protein structure, Escherichia coli, Amino Acid Sequence, Cysteine, Integral membrane protein, Nuclear Magnetic Resonance, Biomolecular, Sequence Homology, Amino Acid, Chemistry, Circular Dichroism, Methanol, Peripheral membrane protein, Cell Membrane, Membrane Proteins, Water, Transmembrane protein, Protein tertiary structure, Recombinant Proteins, Molecular Weight, Crystallography, Membrane, Solubility, Colicin, Solvents, Chloroform

Abstract

The colicin E1 immunity protein (ImmE1), a 13.2-kDa hydrophobic integral membrane protein localized in the Escherichia coli cytoplasmic membrane, protects the cell from the lethal, channel-forming activity of the bacteriocin, colicin E1. Utilizing its solubility in organic solvents, ImmE1 was purified by 1-butanol extraction of isolated membranes, followed by gel filtration and ion-exchange chromatography in a chloroform/methanol/H(2)O (4:4:1) solvent system. Circular dichroism analysis indicated that the alpha-helical content of ImmE1 is approximately 80% in 1-butanol or 2,2,2-trifluoroethanol, consistent with a previous membrane-folding model with three extended hydrophobic transmembrane helical domains, H1-H3. Each of these extended hydrophobic domains contains a centrally located single Cys residue that could be used as a probe of protein structure. The presence of tertiary structure of purified ImmE1 in a solvent of mixed polarity, chloroform/methanol/H(2)O (4:4:1) was demonstrated by (i) the constraints on Tyr residues shown by the amplitude of near-UV circular dichroism spectra in the wavelength interval, 270-285 nm; (ii) the correlation between the near-UV Tyr CD spectrum of single and double Cys-to-X mutants of the Imm protein and their in vivo activity; (iii) the upfield shift of methyl groups in a 1D NMR spectrum, a 2D- HSQC NMR spectrum of ImmE1 in the mixed polarity solvent mixture, and a broadening and disappearance of the indole (1)H proton resonance from Trp94 in H3 by a spin label attached to Cys16 in the H2 hydrophobic domain; (iv) near-UV circular dichroism spectra with a prominent ellipticity band centered at 290 nm from a single Trp inserted into the extended hydrophobic domains. It was concluded that the colicin E1 immunity protein adopts a folded conformation in chloroform/methanol/H(2)O (4:4:1) that is stabilized by helix-helix interactions. Analysis of the probable membrane folding topology indicated that several Tyr residues in the bilayer region of the three transmembrane helices could contribute to the near-UV CD spectrum through helix-helix interactions.

Published

2000

17. Structural changes are induced in human neutrophil cytochrome b by NADPH oxidase activators, LDS, SDS, and arachidonate: intermolecular resonance energy transfer between trisulfopyrenyl-wheat germ agglutinin and cytochrome b558

Author

James B. Burritt, Thomas R. Foubert, Algirdas J. Jesaitis, and Ross M. Taylor

Subjects

NADPH oxidase activator, Cytochrome, Neutrophils, Protein Conformation, Wheat Germ Agglutinins, Cytochrome b, Biophysics, Enzyme Activators, Enzyme-Linked Immunosorbent Assay, Heme, Biochemistry, Structural change, Humans, Cytochrome c oxidase, Oxidase test, Arachidonic Acid, NADPH oxidase, Quenching (fluorescence), biology, Chemistry, NADPH Oxidases, Sodium Dodecyl Sulfate, Cytochrome P450 reductase, Cell Biology, Cytochrome b Group, Wheat germ agglutinin, B vitamins, Spectrometry, Fluorescence, Energy Transfer, biology.protein, Protein Binding

Abstract

Anionic amphiphiles such as sodium- and lithium dodecyl sulfate (SDS, LDS), or arachidonate (AA) initiate NADPH oxidase and proton channel activation in cell-free systems and intact neutrophils. To investigate whether these amphiphiles exert allosteric effects on cytochrome b, trisulfopyrenyl-labeled wheat germ agglutinin (Cascade Blue-wheat germ agglutinin, CCB-WGA) was used as an extrinsic fluorescence donor for resonance energy transfer (RET) to the intrinsic heme acceptors of detergent-solubilized cytochrome b. In solution, cytochrome b complexed with the CCB-WGA causing a rapid, saturable, carbohydrate-dependent quenching of up to approximately 55% of the steady-state fluorescence. Subsequent additions of SDS, LDS, or AA to typical cell-free oxidase assay concentrations completely relaxed the fluorescence quenching. The relaxation effects were specific, and not caused by dissociation of the CCB-WGA-cytochrome b complex or alterations in the spectral properties of the chromophores. In contrast, addition of the oxidase antagonist, arachidonate methyl ester, caused an opposite effect and was able to partially reverse the activator-induced relaxation. We conclude that the activators induce a cytochrome b conformation wherein the proximity or orientation between the hemes and the extrinsic CCB fluorescence donors has undergone a significant change. These events may be linked to NADPH oxidase assembly and activation or proton channel induction.

18. Single-step immunoaffinity purification and characterization of dodecylmaltoside-solubilized human neutrophil flavocytochrome b

Author

Thomas R. Foubert, Connie I. Lord, Ross M. Taylor, James B. Burritt, Kim Clawson Stone, Algirdas J. Jesaitis, Meagan A Snodgrass, Jeannie M. Gripentrog, and Danas Baniulis

Subjects

Neutrophils, Size-exclusion chromatography, Population, Biophysics, Dodecylmaltoside, Heme, Immunoaffinity, Mass spectrometry, Biochemistry, chemistry.chemical_compound, Affinity chromatography, Glucosides, Enzyme Stability, Transferase, Humans, education, Integral membrane protein, Purification, education.field_of_study, Chromatography, NADPH Dehydrogenase, Membrane Transport Proteins, NADPH Oxidases, Blood Proteins, Cell Biology, Cytochrome b Group, Phosphoproteins, Protein Subunits, Membrane, chemistry, Flavocytochrome b, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization

Abstract

Flavocytochrome b (Cyt b) is a heterodimeric, integral membrane protein that serves as the central component of an electron transferase system employed by phagocytes for elimination of bacterial and fungal pathogens. This report describes a rapid and efficient single-step purification of Cyt b from human neutrophil plasma membranes by solubilization in the nonionic detergent dodecylmaltoside (DDM) and immunoaffinity chromatography. A similar procedure for isolation of Cyt b directly from intact neutrophils by a combination of heparin and immunoaffinity chromatography is also presented. The stability of Cyt b was enhanced in DDM relative to previously employed solubilizing agents as determined by both monitoring the heme spectrum in crude membrane extracts and assaying resistance to proteolytic degradation following purification. Gel filtration chromatography and dynamic light scattering indicated that DDM maintains a predominantly monodisperse population of Cyt b following immunoaffinity purification. The high degree of purity obtained with this isolation procedure allowed for direct determination of a 2:1 heme to protein stoichiometry, confirming previous structural models. Analysis of the isolated heterodimer by matrix-assisted laser desorption/ionization (MALDI) mass spectrometry allowed for accurate mass determination of p22phox as indicated by the gene sequence. Affinity-purified Cyt b was functionally reconstituted into artificial bilayers and demonstrated that catalytic activity of the protein was efficiently retained throughout the purification procedure.