Your search keyword '"Epps DE"' showing total 44 results

1. Identification and comparison of CD34-positive cells and their subpopulations from normal peripheral blood and bone marrow using multicolor flow cytometry

Author

Bender, JG, primary, Unverzagt, KL, additional, Walker, DE, additional, Lee, W, additional, Van Epps, DE, additional, Smith, DH, additional, Stewart, CC, additional, and To, LB, additional

Published

1991

2. Analysis of myelomonocytic leukemic differentiation by a cell surface marker panel including a fucose-binding lectin from Lotus tetragonolobus

Author

Elias, L and Van Epps, DE

Abstract

The fucose-binding lectin from Lotus tetragonolobus ( FBL -L) has been previously shown to bind specifically to normal cells of the myeloid and monocytic lineages. The purpose of this study was to explore the utility of fluoresceinated FBL -L as a leukemia differentiation marker in conjunction with a panel of other frequently used surface markers (Fc receptor, HLA-DR, OKM1, and antimonocyte antibody). FBL -L reacted with leukemic cells in 8/9 cases of clinically recognized acute myeloid leukemia, including myeloid blast crisis of chronic granulocytic leukemia, 3/3 cases of chronic phase chronic myelogenous leukemia, and in 2/7 cases of clinically undifferentiated acute leukemia. Correlations were noted between reactivity with FBL -L, and DR and Fc receptor expression. Among continuous cell lines, FBL -L bound with high intensity to a majority of HL-60 and U937 cells. The less well differentiated myeloblast cell lines, KG-1, KG1a , and HL-60 blast II, exhibited less FBL -L binding than HL-60 and U937. A moderate proportion of K562 cells exhibited low level binding of FBL -L. Several lymphoblastic cell lines exhibited a pattern of low intensity binding that was distinguishable from the high intensity binding pattern of the myeloblastic lines. FBL -L reactivity of U937 was enhanced by induction of differentiation with leukocyte conditioned medium, but not dimethylsulfoxide. Such treatments induced contrasting patterns of change of HL-60 and U937 when labeled with OKM1, alpha-Mono, and HLA- DR. These studies demonstrate the application of FBL -L to analysis and quantitation of myelomonocytic leukemic differentiation.

Published

1984

3. Correlation of serum opsonic activity in cystic fibrosis with colonization and disease state: measurement of opsonins to Pseudomonas aeruginosa by neutrophil superoxide anion generation

Author

Van Epps De, Florman Al, and Bender Jg

Subjects

Adult, Male, congenital, hereditary, and neonatal diseases and abnormalities, Adolescent, Cystic Fibrosis, Neutrophils, Biology, medicine.disease_cause, Cystic fibrosis, Microbiology, chemistry.chemical_compound, Superoxides, medicine, Humans, Colonization, Pseudomonas Infections, Child, Opsonin, Superoxide, Pseudomonas aeruginosa, Pseudomonas, Opsonin Proteins, medicine.disease, biology.organism_classification, digestive system diseases, respiratory tract diseases, Respiratory burst, Antibody opsonization, chemistry, Pediatrics, Perinatology and Child Health, Immunology, Female

Abstract

Serum from patients with cystic fibrosis and normal controls was used to opsonize mucoid and nonmucoid Pseudomonas aemginosa particles. Opsonic activity was then determined by measuring the production of superoxide anion (O2-) from normal neutrophils stimulated with the opsonized particles. Without any opsonization, mucoid P. aeruginosa stimulated significantly more O2- than nonmucoid P. aeruginosa. Responses to nonmucoid P. aemginosa observed with heat-inactivated serum from patients with cystic fibrosis were significantly higher (p=0.008) than those observed with heat-inactivated control sera. Comparisons made between patients who were colonized with P. aeruginosa and those who were not showed that heat activated serum from colonized patients had significantly higher levels of opsonic activity than heat inactivated serum from patients who were not colonized. These differences were observed with either mucoid or nonmucoid P. aeruginosa. A negative correlation was also observed between opsonic activity and clinical status measured by Schwachman scores of colonized patients. These data indicate that in patients colonized with P. aemginosa the deterioration of their clinical status correlated with increased opsonic activity reflected in the oxidative burst response of neutrophils.

Published

1987

4. Determination of ligand-MurB interactions by isothermal denaturation: application as a secondary assay to complement high throughput screening.

Author

Sarver RW, Rogers JM, and Epps DE

Subjects

Automation, Calorimetry, Differential Scanning, Circular Dichroism, Dose-Response Relationship, Drug, Hot Temperature, Kinetics, Ligands, Models, Chemical, Protein Binding, Protein Denaturation, Spectrometry, Fluorescence, Staphylococcus aureus metabolism, Temperature, Time Factors, Ultraviolet Rays, Biochemistry methods, Carbohydrate Dehydrogenases chemistry, Carbohydrate Dehydrogenases metabolism

Abstract

We used a temperature-jump isothermal denaturation procedure with various methods of detection to evaluate the quality of putative inhibitors of MurB discovered by high-throughput screening. Three optical methods of detection-ultraviolet hyperchromicity of absorbance, fluorescence of bound dyes, and circular dichroism-as well as differential scanning calorimetry were used to dissect the effects of two chemical compounds and a natural substrate on the enzyme. The kinetics of the denaturation process and binding of the compounds detected by quenching of flavin fluorescence were used to quantitate the dose dependencies of the ligand effects. We found that the first step in the denaturation of MurB is the rapid loss of flavin from the active site and that the two chemical inhibitors appeared to destabilize the interaction of the cofactor with the enzyme but stabilize the global unfolding. The kinetics of the denaturation process as well as the loss of flavin fluorescence on binding established that both compounds had nanomolar affinities for the enzyme. We showed that coupling of the various detection methods with isothermal denaturation yields a powerful regimen to provide analytical data for assessing inhibitor specificity for a protein target.

Published

2002

5. Prolonged production of NADPH oxidase-corrected granulocytes after gene therapy of chronic granulomatous disease.

Author

Malech HL, Maples PB, Whiting-Theobald N, Linton GF, Sekhsaria S, Vowells SJ, Li F, Miller JA, DeCarlo E, Holland SM, Leitman SF, Carter CS, Butz RE, Read EJ, Fleisher TA, Schneiderman RD, Van Epps DE, Spratt SK, Maack CA, Rokovich JA, Cohen LK, and Gallin JI

Subjects

Adolescent, Adult, Antigens, CD34, Blood Component Removal, Female, Flow Cytometry, Follow-Up Studies, Hematopoietic Stem Cell Transplantation, Humans, Male, Phosphoproteins deficiency, Phosphoproteins immunology, Retroviridae genetics, Transduction, Genetic, Genetic Therapy methods, Granulocytes enzymology, Granulomatous Disease, Chronic therapy, NADPH Oxidases biosynthesis, Phosphoproteins genetics

Abstract

Little is known about the potential for engraftment of autologous hematopoietic stem cells in human adults not subjected to myeloablative conditioning regimens. Five adult patients with the p47(phox) deficiency form of chronic granulomatous disease received intravenous infusions of autologous CD34(+) peripheral blood stem cells (PBSCs) that had been transduced ex vivo with a recombinant retrovirus encoding normal p47(phox). Although marrow conditioning was not given, functionally corrected granulocytes were detectable in peripheral blood of all five patients. Peak correction occurred 3-6 weeks after infusion and ranged from 0.004 to 0.05% of total peripheral blood granulocytes. Corrected cells were detectable for as long as 6 months after infusion in some individuals. Thus, prolonged engraftment of autologous PBSCs and continued expression of the transduced gene can occur in adults without conditioning. This trial also piloted the use of animal protein-free medium and a blood-bank-compatible closed system of gas-permeable plastic containers for culture and transduction of the PBSCs. These features enhance the safety of PBSCs directed gene therapy.

Published

1997

6. Fluorescence and site-directed mutagenesis studies of interleukin 1 beta.

Author

Epps DE, Yem AW, McGee JM, Tomich CS, Curry KA, Chosay JG, and Deibel MR

Subjects

Animals, Cells, Cultured, Cloning, Molecular, Interleukin-1 chemistry, Kinetics, Leucine, Lysine, Mice, Models, Molecular, Mutagenesis, Site-Directed, Protein Binding, Protein Conformation, Protein Folding, Protein Structure, Tertiary, Receptors, Interleukin-1 metabolism, Spectrometry, Fluorescence, Tryptophan, Interleukin-1 genetics

Abstract

The authors mutated two key residues in the sequence of the cytokine interleukin 1 beta, namely the double mutant Phe46 to Trp46 and Trp120 to Phe120 and the single point mutation Lys103 to Leu103 and measured the resulting receptor binding and biological activities. The biological and receptor binding activities of the Trp46 mutein was reduced by a factor of 12 and 25, respectively, and surprisingly, those of the Leu103 mutein, 2600 and 600-fold relative to the wild-type protein. The authors had previously showed that Lys103 was unusually reactive to a variety of derivatizing agents. Furthermore, the Trp to Phe mutation allowed us to monitor the local environment of that residue by studying its intrinsic fluorescence properties, as well as any change in the fluorescence properties of Trp120 of the Leu103 mutein. The results of these studies show that mutation of Lys103 to Leu103 produces subtle long-range changes in the micro-environment of Trp120, indicative of a key role for this residue in the folding of the entire protein.

Published

1997

7. Wheat germ agglutinin inhibits the C5a receptor interaction: implications for receptor microheterogeneity and ligand binding site.

Author

Johnson RJ, Simpson S, Van Epps DE, and Chenoweth DE

Subjects

Binding Sites, Chromatography, Affinity, Complement C5a metabolism, Flow Cytometry, Granulocytes ultrastructure, Humans, Ligands, Receptor, Anaphylatoxin C5a, Receptors, Complement chemistry, Receptors, Complement physiology, Wheat Germ Agglutinins metabolism, Receptors, Complement antagonists & inhibitors, Wheat Germ Agglutinins administration & dosage

Abstract

Wheat germ agglutinin (WGA) has been shown to inhibit the interaction of C5a with the C5a receptor on both polymorphonuclear neutrophils (PMNs) and the histiocytic cell line U937. The level of inhibition with isolated receptor preparations is 100%, and on intact cells 10 to 20% of the receptor population appear to retain their ability to bind C5a in the presence of WGA. In contrast, this lectin completely inhibits the C5a-mediated degranulation of PMN primary and secondary granules, suggesting that the population of C5a receptors responsible for mediating degranulation is also recognized by WGA. More than 50% of the receptors appear to be blocked before an effect on degranulation occurs. This inhibition by WGA does not appear to be due to down-regulation of C5a receptors from the cell surface, excessive aggregation of receptor sites, or interaction of WGA with the carbohydrate portion of the C5a molecule. The inhibition is reversed by N-acetylglucosamine but not by sialic acid. This effect appears to be specific for WGA because various other lectins do not inhibit the C5a receptor interaction. That the inhibition by WGA is due to direct binding of the lectin to N-acetylglucosamine residues on the C5a receptor is strongly supported by the ability of the cross-linked C5a-receptor complex to bind to and be specifically eluted from a WGA-Affigel affinity matrix. These observations are consistent with hypothesis that the population of C5a receptors on leukocytes exhibits microheterogeneity with respect to structure (carbohydrate content) and/or function.

Published

1992

8. C5a and formyl peptide receptor regulation on human monocytes.

Author

Van Epps DE, Simpson SJ, and Chenoweth DE

Subjects

Ammonium Chloride pharmacology, Calcium pharmacology, Complement C5a metabolism, Endocytosis, Humans, In Vitro Techniques, Monensin pharmacology, N-Formylmethionine Leucyl-Phenylalanine metabolism, Neutrophils physiology, Receptor, Anaphylatoxin C5a, Receptors, Formyl Peptide, Monocytes physiology, Receptors, Complement physiology, Receptors, Immunologic physiology

Abstract

Regulation of C5a and formyl-methionine-leucine-phenylalanine-lysine (fMLPL) receptors on human monocytes has been studied using fluorescein-conjugated derivatives and flow cytometry. Monocytes have receptors for each of these ligands, as evidenced by their ability to bind specifically biologically active fluorescein derivatives of these ligands. Quenching experiments showed that bound fluoresceinated C5a and fMLPL are rapidly internalized at 37 degrees C. Once internalized, monocytes are able to reexpress these receptors, returning to control levels within approximately 90 min. This contrasts with rate differences seen in polymorphonuclear neutrophils (PMNs), where fMLPL receptors return more rapidly (approximately 30 min) than do C5a receptors (approximately 100 min). Monensin inhibited the reexpression of C5a but not fMLPL receptors, suggesting that a receptor recycling process is necessary to replenish C5a receptors on the monocyte surface. Similar although less efficient inhibition of C5a receptor reexpression was observed with NH4Cl treatment. Reexpression of both C5a and fMLPL receptors was independent of extracellular Ca2+. Treatment with various agents known to stimulate monocytes and PMNs increased the expression of fMLPL receptors in both cell types but either had no effect on or reduced the level of C5a receptor expression. This would indicate that monocytes, like PMNs, have intracellular pools of preformed fMLPL receptors, available for reexpression. These studies show that, like PMNs, monocytes modulate C5a and fMLPL receptors through different mechanisms. Furthermore, monocytes are capable of reexpressing these receptors following exposure to ligand, a theoretical requirement for chemotaxis.

Published

1992

9. Site-specific chemical modification of interleukin-1 beta by acrylodan at cysteine 8 and lysine 103.

Author

Yem AW, Epps DE, Mathews WR, Guido DM, Richard KA, Staite ND, and Deibel MR Jr

Subjects

2-Naphthylamine pharmacology, Amino Acid Sequence, Animals, Cells, Cultured, Chromatography, Ion Exchange, Interleukin-1 isolation & purification, Interleukin-1 metabolism, Lymphocyte Activation, Mice, Mice, Inbred C3H, Models, Structural, Molecular Sequence Data, Peptide Mapping, Protein Conformation, Receptors, Immunologic metabolism, Receptors, Interleukin-1, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Recombinant Proteins pharmacology, Spectrometry, Mass, Fast Atom Bombardment, T-Lymphocytes drug effects, T-Lymphocytes immunology, 2-Naphthylamine analogs & derivatives, Cysteine, Interleukin-1 pharmacology, Lysine

Abstract

Acrylodan, which normally modifies cysteine residues, was employed to derivatize recombinant interleukin-1 beta (rIL-1 beta) under native conditions, using a reagent:protein ratio of 3:1. Two major covalent protein/acrylodan adducts were generated and subsequently purified by DEAE TSK 5PW ion exchange chromatography. Peptide mapping and mass spectrometry were used to locate the probe on the modified proteins. Both modified proteins carried one molecule of acrylodan each, one at Cys-8 and the other at Lys-103. Neither Cys-71 nor any of the other 13 lysine residues of rIL-1 beta was modified. Cysteine 71 is inaccessible to acrylodan, but the unusual specificity for Lys-103 could be caused by the location of that residue at the bottom of a hydrophobic pocket which might specifically bind the reagent. No double-labeled protein was detected, indicating that the introduction of the label at either site interferes with the labeling at the other. Both acrylodan-modified proteins exhibited bioactivity in the thymocyte proliferation assay at a level equivalent to that of the unmodified control protein (1.7 x 10(7) units/mg), which shows that the modification of either the Cys-8 or Lys-103 position with acrylodan does not interfere with the cellular bioactivities of the respective proteins. Furthermore, receptor binding assays yielded a Kd = 32.0 +/- 4.8 pM for the Lys-103-labeled protein, Kd = 69.5 +/- 12.7 pM for the unmodified protein, and Kd = 75.0 +/- 11.6 pM for the Cys-8-labeled protein. Thus, Cys-8 or Lys-103 modification of rIL-1 beta by acrylodan also does not interfere with the ability of the molecule to bind to its receptor. The slightly higher affinity of the Lys-103-labeled protein for the receptor suggests that the positive charge on this residue in the native molecule may interfere with IL-1 receptor binding. The two fluorescent labeled IL-1 proteins described herein should provide interesting probes for the study of IL-1/IL-1 receptor interactions.

Published

1992

10. Spectral characterization of environment-sensitive adducts of interleukin-1 beta.

Author

Epps DE, Yem AW, Fisher JF, McGee JE, Paslay JW, and Deibel MR Jr

Subjects

2-Naphthylamine pharmacology, Amino Acid Sequence, Animals, Cysteine, Humans, Interleukin-1 metabolism, Kinetics, Lysine, Mice, Protein Conformation, Receptors, Immunologic drug effects, Receptors, Immunologic metabolism, Receptors, Interleukin-1, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Spectrometry, Fluorescence, 2-Naphthylamine analogs & derivatives, Interleukin-1 chemistry

Abstract

We have determined the fluorescence properties of two covalently attached acrylodan derivatives of recombinant human interleukin-1 beta, namely the Cys-8 and Lys-103 adducts. The emission and excitation maxima indicated the presence of two operationally distinct conformers for each probe. The iodide quenching and the kinetics of fluorescence changes associated with guanidinium chloride-induced denaturation show that each covalent adduct exists both in hydrated and dehydrated environments. Furthermore, fluorescence changes associated with the binding of the adducts to a recombinant soluble murine receptor indicated that only the conformers with the label in the hydrophobic environment are competent toward the soluble murine interleukin receptor and that the hydrated and dehydrated conformers are in a dynamic equilibrium on the time scale of the binding experiments.

Published

1992

11. Relationship of chemotactic receptors for formyl peptide and C5a to CR1, CR3, and Fc receptors on human neutrophils.

Author

Van Epps DE, Bender JG, Simpson SJ, and Chenoweth DE

Subjects

Antibodies, Monoclonal immunology, Complement C3b immunology, Complement C3b metabolism, Flow Cytometry, Fluorescent Dyes, Humans, N-Formylmethionine Leucyl-Phenylalanine metabolism, Neutrophils metabolism, Receptors, Complement 3b, Receptors, Formyl Peptide, Complement C5a metabolism, N-Formylmethionine Leucyl-Phenylalanine analogs & derivatives, Neutrophils ultrastructure, Receptors, Complement metabolism, Receptors, Fc metabolism, Receptors, Immunologic metabolism

Abstract

The co-expression of C5a and formyl-methionine-leucine-phenylalanine-lysine (FMLPL) receptors with CR1, CR3, and Fc receptors on human neutrophils (PMN) was studied. Fluorescein-conjugated C5a (FL-C5a) and FMLPL (FL-FMLPL) were used to identify C5a and formyl peptide receptors. CR1, CR3, and Fc receptors were identified with monoclonal antibodies and a Texas red-labeled goat anti-mouse immunoglobulin second step reagent. The co-expression of chemotactic receptors with CR1, CR3, or Fc receptors was evaluated using two-color flow cytometry. A direct correlation between the degree of expression of receptors for FL-FMLPL and the expression of CR3, CR1, and Fc receptors on individual PMN was observed. In contrast, no correlation between the degree of C5a receptor expression and CR1, CR3, or Fc receptor expression was found. Similar results were obtained with PMN after up regulation of CR1, CR3, Fc, and FMLPL receptors by incubation at 37 degrees C for 10 min with or without phorbol myristate acetate. These data suggest that the expression of FMLPL, CR1, CR3, and Fc receptors are regulated in a similar manner, whereas C5a receptor expression is regulated independently. Furthermore, these data indicate that within a given population of PMN, a parallel exists between the degree of CR1, CR3, FMLPL, and Fc receptor expression on individual cells.

Published

1990

12. Enhancement of neutrophils function as a result of prior exposure to chemotactic factor.

Author

Van Epps DE and Garcia ML

Subjects

Animals, Blood Bactericidal Activity, Exudates and Transudates physiology, Guinea Pigs, Humans, Luminescent Measurements, Neutrophils drug effects, Opsonin Proteins, Receptors, Complement metabolism, Receptors, Drug physiology, Receptors, Fc metabolism, Superoxides metabolism, Chemotactic Factors pharmacology, Chemotaxis, Leukocyte, Neutrophils physiology

Abstract

Exposure of human polymorphonuclear leukocytes (PMN) to chemotactic factor, as well as the migration of PMN through a 5-mum pore-size membrane, results in a PMN population with enhanced chemiluminescence, enhanced capacity for superoxide anion production, and increased Escherichia coli bactericidal activity. The enhanced PMN response resulting from exposure to chemotactic factor was observed with several chemotactic stimuli, including a mixture of casein and autologous serum, chemotactic C5 fragment, and formyl-l-methionyl-l-leucine-l-phenylalanine (f-Met-Leu-Phe). Enhanced levels of chemiluminescence were observed with both soluble stimuli (concanavalin A and phorbol myristate acetate) as well as particulate stimuli (opsonized zymosan). Once activated by chemotactic factor, PMN retained their enhanced stimulated chemiluminescence in the absence of chemotactic factor for at least 2.5 h. Enhanced activity could not be correlated with a shift in the number of immunoglobulin (Ig)G Fc receptor positive or complement receptor positive PMN. In vivo studies with guinea pigs indicated that PMN attracted to an intraperitoneal injection of casein, like those attracted through a chemotaxis membrane in vitro in response to casein, showed markedly enhanced stimulated chemiluminescence when compared with peripheral blood PMN from the same animal. Such a mechanism to stimulated PMN function may enhance the effectiveness of PMN in host defense at inflammatory foci.

Published

1980

13. Streptolysin O inhibition of neutrophil chemotaxis and mobility: nonimmune phenomenon with species specificity.

Author

Van Epps DE and Andersen BR

Subjects

Agammaglobulinemia immunology, Animals, Cell Migration Inhibition, Cell Movement drug effects, Cholesterol pharmacology, Chromatography, Gel, Erythrocytes drug effects, Haplorhini, Hemolysis drug effects, Humans, Hypersensitivity, Delayed immunology, Immune Tolerance, Immunization, Papio, Rabbits, Sheep, Skin Tests, Species Specificity, Staining and Labeling, Streptococcus pyogenes analysis, Streptolysins toxicity, Time Factors, Chemotaxis drug effects, Neutrophils drug effects, Streptolysins pharmacology

Abstract

The effects of streptolysin O (SO) (1 to 4 hemolytic units) on the mobility of neutrophilic leukocytes from humans, baboons, sheep, and rabbits were compared. After SO treatment, chemotaxis and random mobility of human neutrophils were markedly suppressed, baboon and sheep neutrophils were partially suppressed, and rabbit neutrophils were unaffected and demonstrated normal chemotaxis and mobility. The amounts of SO used in the mobility studies caused no leukocyte lysis or trypan blue uptake by human, baboon, or sheep cells, and minimal lysis or trypan blue uptake by rabbit cells. The possible involvement of immune mediators in the observed inhibition of human neutrophils was considered and excluded by the following studies. White blood cells from humans with humoral or cellular immune deficiencies responded in a manner similar to normal human cells; supernatant solutions from SO-treated human white blood cells did not contain a chemotactic suppressor; preincubation of SO with cholesterol (an inhibitor of SO hemolytic activity) caused loss of the chemotactic suppressive effect of the toxin on human leukocytes; and leukocytes from rabbits preimmunized with SO remained refractory to chemotactic suppression.

Published

1974

14. Lectin-mediated induction of human neutrophil chemotaxis, chemokinesis, and cap formation.

Author

Kuehn C and Van Epps DE

Subjects

Binding Sites, Cell Membrane drug effects, Cell Membrane immunology, Cells, Cultured, Chemotactic Factors, Humans, Immunologic Capping, Monosaccharides pharmacology, Neutrophils immunology, Chemotaxis, Leukocyte drug effects, Lectins pharmacology, Neutrophils drug effects

Abstract

Six lectins, including concanavalin A, phytohemagglutinin P, castor bean I, wheat germ agglutinin, peanut agglutinin, and pokeweed mitogen, were studied for their ability to stimulate human neutrophil locomotion and cap formation. Five of these lectins with known monosaccharide specificities, including concanavalin A, phytohemagglutinin, P, castor bean I, wheat germ agglutinin, and peanut agglutinin, were found to stimulate human neutrophil migration in a modified Boyden assay. Pokeweed mitogen showed negligible activity in the locomotion assay as compared with other lectins. Tests were performed to determine if the observed neutrophil migration in response to lectins was directional, and it was found that concanavalin A, phytohemagglutinin P, and peanut agglutinin were both chemokinetic and chemotactic, whereas castor bean I was only chemokinetic. Wheat germ agglutinin could not be declared chemotactic or chemokinetic due to its tendency to agglutinate neutrophils. Studies with fluoresceinated lectins demonstrated that lectins which stimulate neutrophil migration also bind to neutrophil surfaces. Preincubation with specific monosaccharide ligands blocked both stimulated locomotion and fluorescence, suggesting that an available lectin-binding site was required both for lectin binding and the stimulation of migration. Additional experiments indicated that fluoresceinated concanavalin A, phytohemagglutinin P, castor bean I, wheat germ agglutinin, and peanut agglutinin all induce cap formation on the neutrophil.

Published

1980

15. Discovery of an arachidonic acid C-8 lipoxygenase in the gorgonian coral Pseudoplexaura porosa.

Author

Bundy GL, Nidy EG, Epps DE, Mizsak SA, and Wnuk RJ

Subjects

Animals, Arachidonate Lipoxygenases, Arachidonic Acids metabolism, Cnidaria, Fatty Acids analysis, Hydroxyeicosatetraenoic Acids metabolism, Magnetic Resonance Spectroscopy, Mass Spectrometry, Stereoisomerism, Leukotrienes, Lipoxygenase metabolism

Abstract

The gorgonian coral Pseudoplexaura porosa contains a lipoxygenase capable of converting exogenous arachidonic acid into (8R)-8-hydroperoxy-5,9,11,14-eicosatetraenoic acid. The (8R)- (or 8-L-) configuration in this product, opposite to that observed in previously reported 8-lipoxygenase products, was determined unambiguously by comparison of oxidative ozonolysis fragments with authentic malic acid-derived standards. Extracts from the coral contained no detectable prostaglandins (PGAs, PGBs, PGEs, or PGFs). Although arachidonic acid represents one of the most abundant of the common fatty acids found in the phospholipid and total lipid fractions of P. porosa, products ascribable to the arachidonic acid 8-lipoxygenase pathway ((8R)-8-hydroperoxy-5,9,11,14-eicosatetraenoic acid, the corresponding alcohol 8-hydroxyeicosatetraenoic acid, further transformation products) have not yet been identified in the coral extracts. The physiological significance of the 8-lipoxygenase in this species remains a matter for speculation.

Published

1986

16. Serum chemotactic inhibitory activity: heat activation of chemotactic inhibition.

Author

Epps DE and Williams RC Jr

Subjects

Absorption, Caseins metabolism, Complement C3 metabolism, Escherichia coli metabolism, Humans, In Vitro Techniques, Neutrophils metabolism, Skin Tests, Time Factors, Chemotaxis, Hot Temperature

Abstract

Serum chemotactic inhibitory activity (CIA) was studied in 46 patients with various systemic diseases, using a system consisting of normal human leukocytes as indicator cells and 10% fresh normal serum as a control chemotactic attractant. It was shown, as previously reported, that an association exists between CIA and skin test anergy. Heat treatment of sera at 56 C for 30 min increased both the incidence and the degree of chemotactic inhibition observed in these patients. The effects of heat treatment of sera containing CIA on other chemotactic attractants (C3a, bacteria-derived chemotactic factor (BF), and casein) are shown. Before heat treatment, some sera suppressed chemotaxis mediated by BF in the absence of suppression of normal serum-mediated chemotaxis, indicating the possible involvement of more than one system of inhibition. Multiple systems were further supported by data indicating that room temperature incubation resulted in a loss of CIA as measured by normal serum-mediated chemotoxis with no apparent decrease in the inhibition of BF -mediated chemotaxis. Separation of sera containing CIA by Sephadex G-200 showed chemotactic inhibitory activity to be increased in both the void volume region. Experiments showed that heat treating before separation resulted in similar increases in both peaks, implying the presence of an antagonist to CIA. Experiments demonstrating that sera containing CIA do not suppress casein-mediated chemotaxis by means of an irreversible inactivation of chemotactic factor are included along with experiments demonstrating a cellular mode of action. The possible presence of two systems of chemotactic inhibition, one acting directly upon chemotactic factors and one interacting with the responding cell, are discussed.

Published

1976

17. Characterization of human mononuclear cells using reduced pyridine nucleotide fluorescence and flow cytometry.

Author

Bender JG, Van Epps DE, and Steinkamp JA

Subjects

Antibodies, Monoclonal metabolism, Flow Cytometry, Fluorescence, Humans, Lasers, Oxidation-Reduction, Tetradecanoylphorbol Acetate pharmacology, Monocytes cytology, NADP metabolism

Abstract

Peripheral blood monocytes undergo an oxidative burst similar to that seen in neutrophils. The basis for this response appears to be an NAD(P)H oxidase that utilizes reduced NAD(P)H to form superoxide anion. We utilized the unique UV-stimulated fluorescence property of reduced pyridine nucleotides to analyze NAD(P)H utilization in monocytes. UV-stimulated fluorescence in mononuclear cell preparations indicated two populations of cells with the highly fluorescent cells having a Coulter volume consistent with that of monocytes. Dual laser analysis with monoclonal antibodies confirmed that these highly fluorescent cells are monocytes by showing them to be OKM1+, Leu DR+, and anti-monocyte 0.2+. Natural killer (NK) cells, as defined by Leu 7, were not found in this highly fluorescent population. Stimulation of mononuclear cells with phorbol myristate acetate caused a fluorescence loss indicative of NAD(P)H oxidation in monocytes but not in lymphocytes. Stimulation with suboptimal concentrations of PMA (1-5 ng/ml) resulted in a dose-dependent fluorescence loss in monocytes that occurred in an all-or-none fashion identical to the pattern observed in neutrophils. Simultaneous measurement of H2O2 production using dichlorofluorescein formation with NAD(P)H fluorescence indicates that oxidant production occurs in a graded manner. This method, then, provides a convenient way to study in single cells the metabolic events involved in depletion and replenishment of NAD(P)H during the oxidative burst and demonstrates an additional means by which to distinguish monocytes from lymphocytes using flow cytometry.

Published

1985

18. Effect of high doses of radiation on human neutrophil chemotaxis, phagocytosis and morphology.

Author

Holley TR, Van Epps DE, Harvey RL, Anderson RE, and Williams RC Jr

Subjects

Cell Nucleus radiation effects, Cell Survival, Cytological Techniques, Cytoplasm radiation effects, Dose-Response Relationship, Radiation, Humans, Microscopy, Electron, Neutrophils cytology, Staphylococcus, Trypan Blue, Chemotaxis radiation effects, Neutrophils radiation effects, Phagocytosis radiation effects, Radiation Effects

Abstract

Human neutrophils were exposed to varying amounts of ionizing radiation up to 1,000,000 rad and evaluated as to their ability to respond to chemotactic stimuli and phagocytize and kill bacteria. Striking morphologic and functional resistance to radiation was apparent. At doses up to 5,000 rad there was little or no impairment of chemotaxis. As the dosage increased to 50,000 rad, chemotaxis decreased to approximately 50% of nonirradiated control values. At very high doses of radiation (250,000 to 1,000,000 rad) neutrophils failed to respond significantly to chemotactic stimuli. Effects of radiation as measured by phagocytosis and the degree of ultrastructural change paralleled the chemotaxis results.

Published

1974

19. Abnormalities of lymphocyte locomotion in immunodeficiency disease.

Author

Van Epps DE, El-Naggar A, and Ochs HD

Subjects

Adolescent, Adult, Aged, Caseins, Chemotactic Factors, Child, Child, Preschool, Complement C5, Complement C5a, Female, Humans, Hypersensitivity, Delayed, Job Syndrome immunology, Lymphocyte Activation, Lymphocytes immunology, Male, Middle Aged, Mitosis, N-Formylmethionine Leucyl-Phenylalanine, Neutrophils immunology, Phytohemagglutinins pharmacology, Receptors, Antigen, B-Cell analysis, Chemotaxis, Leukocyte, Immunologic Deficiency Syndromes immunology

Abstract

Lymphocyte and neutrophil locomotion were studied in 23 patients with well defined, primary immunodeficiencies. These included eight patients with common variable immune deficiency, three patients with X-linked agammaglobulinaemia, two patients with the Wiskott-Aldrich syndrome, three patients with ataxia telangiectasia, three patients with immunodeficiency and normal serum immunoglobulin concentrations, one patient with immune deficiency and hyper-IgM syndrome, two patients with Job syndrome and one patient with a granulocyte adherence defect. Random and stimulated lymphocyte and neutrophil migration were evaluated. C5a and casein were used to stimulate lymphocyte migration and C5a and formyl-methionyl-leucyl-phenylalanine (f-MLP) were used to stimulate neutrophil migration. Significantly depressed lymphocyte migration in response to casein and C5a was observed in patients with common variable immune deficiency, patients with immune deficiency and normal immunoglobulin concentration, and patients with Job syndrome. No consistent defect in lymphocyte locomotion was observed in the other patients studied. Neutrophil migration in response to C5a and f-MLP was depressed in Job syndrome, the patient with a granulocyte adherence defect, one of the six patients with common variable immune deficiency and none of the remaining patients. No significant correlation of skin test reactivity and lymphocyte migration was noted, but a correlation between the degree of lymphocyte proliferation in response to phytohaemagglutinin and lymphocyte migration in response to casein was observed. The results presented indicate that aberrations in lymphocyte migration occur in several types of immunodeficiency diseases and that defects in lymphocyte and neutrophil migration can occur simultaneously or totally independent of each other.

Published

1983

20. Serum inhibitor of C5 fragment-mediated polymorphonuclear leukocyte chemotaxis associated with chronic hemodialysis.

Author

Goldblum SE, Van Epps DE, and Reed WP

Subjects

Adult, Centrifugation, Density Gradient, Chemical Precipitation, Hot Temperature, Humans, Neutrophils physiology, Time Factors, Ultrafiltration, Chemotaxis, Leukocyte, Complement C5 antagonists & inhibitors, Renal Dialysis

Abstract

Abnormal granulocyte chemotaxis has been described in chronic hemodialysis patients. In this study, sera from 53 hemodialysis patients were tested for chemotactic inhibitory activity by a modified Boyden technique. Chemotactic inhibitory activity, defined as >20% inhibition of normal granulocyte chemotaxis, was found in 45% of patients. Only sera from patients having undergone >3 mo hemodialysis displayed chemotactic inhibitory activity and retained this inhibitory activity when retested 9 mo later. Four of five patients who had initially undergone <3 mo hemodialysis and lacked serum chemotactic inhibitory activity developed inhibitory activity when tested 9 mo later. Clinical evaluation of patients with serum chemotactic inhibitory activity showed that these patients did not have a significantly increased incidence of infection, although a trend toward decreased mortality during the time of study was observed (P = 0.0721). Serum chemotactic inhibitory activity was heat stable at 56 degrees C for 30 min and concentration dependent. The major inhibitory component was found to have a sedimentation coefficient of 4S by sucrose density gradient centrifugation. The chemotactic inhibitory activity was not precipitated by 30% ammonium sulfate, but was partially precipitated by 50% ammonium sulfate. Inhibitory sera effectively suppressed neutrophil migration in response to chemotactic C5 fragment and Escherichia coli derived chemotactic factor but was least effective in a system mediated by casein. Furthermore, normal neutrophils preincubated in hemodialysis patient sera displayed normal chemotactic responsiveness indicating a lack of cell-directed inhibition. Serum fractions that contained the inhibitor were found to directly act on the chemotactic C5 fragment, reducing its chemotactic activity. This study indicates that a circulating 4S, heat-stable, factor-directed inhibitor of granulocyte chemotaxis is present in the sera of many hemodialysis patients and probably results from the hemodialysis procedure.

Published

1979

21. Inaccessibility of tryptophan residues of recombinant human renin to quenching agents.

Author

Epps DE, Poorman R, Hui J, Carlson W, and Heinrikson R

Subjects

Acrylamide, Acrylamides pharmacology, Cesium pharmacology, Glycosylation, Humans, Iodides pharmacology, Protein Conformation, Protein Denaturation, Spectrometry, Fluorescence, Chlorides, Fluorescence, Recombinant Proteins, Renin, Tryptophan

Abstract

The fluorescence quenching of the three tryptophan residues of recombinant human renin was determined using ionic and penetrating quenchers. Tryptophans 44,200, and 312 of recombinant human renin were found to be totally inaccessible to the ionic quenchers cesium and iodide and only partially accessible to the penetrating quencher acrylamide. The renin had a fluorescence emission maximum at 325 nm which was made up of three separate components as determined by second derivative spectroscopy. These data are in accord with solvent accessibility calculations from three-dimensional models of human renin but differ from findings published previously from similar analysis of mouse submandibular gland renin (Quay, S. C., Heropoulous, A., Commes, K., Dzau, V. J. (1985) J. Biol. Chem. 260, 15055-15058), which is 68% identical in sequence to human renin.

Published

1987

22. Analysis of the bimodal chemiluminescence pattern stimulated in human neutrophils by chemotactic factors.

Author

Bender JG and Van Epps DE

Subjects

Blood Cell Count, Humans, Interleukin-8, Luminol pharmacology, Lymphocyte Activation drug effects, Neutrophils metabolism, Oxidation-Reduction drug effects, Oxygen Consumption drug effects, Peroxidase metabolism, Superoxides, Time Factors, Chemotactic Factors pharmacology, Luminescent Measurements, Neutrophils drug effects

Abstract

Chemotactic factors, which are important in attracting neutrophils to inflammatory sites, have also been shown to stimulate oxidative metabolism, resulting in increased chemiluminescence and release of superoxide anion (O2-). We observed a unique bimodal chemiluminescence pattern upon stimulation with either the complement-derived factor C5a or formyl-methionyl-leucyl-phenylalanine. A sharp peak of activity occurred within 1 to 2 min, and a second more extended peak was seen between 3 and 6 min. Enhancement of both peaks occurred when the cells were pretreated with cytochalasin B. Expression of both peaks was found to be related to cell density, and expression of the second peak was not dependent upon extracellular metabolites released during the first peak. Cells preincubated in luminol and then thoroughly washed responded with only a single peak coincident with the second peak. Together these findings indicate that the first peak is extracellular in origin, whereas the second peak is cell associated. Studies with scavengers of oxygen intermediates and inhibitors of myeloperoxidase for the oxidation of luminol, which may occur in part through the formation of HOCl as well as through a non-HOCl-mediated mechanism. Evidence for a non-HOCl-mediated mechanism comes from experiments in which luminol, myeloperoxidase, and O2- generated by xanthine-xanthine oxidase produce luminescence in the absence of chloride ion. These studies provide further insight into the sequence of events which occur during the stimulation of neutrophils with chemotactic factors and the nature of neutrophil chemiluminescence.

Published

1983

23. Human polymorphonuclear neutrophil activation with arachidonic acid.

Author

Smith RJ, Sam LM, Justen JM, Leach KL, and Epps DE

Subjects

4,4'-Diisothiocyanostilbene-2,2'-Disulfonic Acid, 4-Acetamido-4'-isothiocyanatostilbene-2,2'-disulfonic Acid analogs & derivatives, 4-Acetamido-4'-isothiocyanatostilbene-2,2'-disulfonic Acid pharmacology, Arachidonic Acid, Benzofurans, Calcium physiology, Cytochalasin B pharmacology, Cytoplasmic Granules drug effects, Exocytosis drug effects, Fatty Acids pharmacology, Fluorescence, Fluorescent Dyes, Fura-2, Humans, Neutrophils enzymology, Neutrophils metabolism, Protein Kinase C isolation & purification, Arachidonic Acids pharmacology, Neutrophils drug effects

Abstract

The capacity of arachidonic acid (AA) to stimulate granule exocytosis from human polymorphonuclear neutrophils (PMNs) was investigated. AA induced the selected extracellular release of azurophil (myeloperoxidase, lysozyme) and specific (lysozyme, vitamin B12 binding protein) granule constituents from human PMNs in a time- and concentration-dependent manner. Cytochalasin B (CB) enhanced but was not required for PMN activation with AA. Although extracellular calcium had no effect on granule exocytosis, AA did stimulate the mobilization of intracellular sequestered Ca2+ which resulted in an increase in cytosolic-free Ca2+ ([Ca2+]i) as reflected by increased fluorescence of Fura-2-treated cells. AA stimulated Ca2+/phospholipid-dependent protein kinase C (PK-C) activity in PMNs. 4,4'-Diisothiocyano-2,2'-disulphonic acid stilbene (DIDS), an anion channel blocker, caused a concentration-dependent inhibition of granule enzyme release. Activation of PMNs with AA was unaffected by the lipoxygenase/cycle-oxygenase inhibitors, 5,8,11, 14-eicosatetraynoic acid (ETYA) and benoxaprofen, a lipoxygenase inhibitor, 6, 9, deepoxy-6,9-(phenylimino) delta 6,8-prostaglandin 1(1) (piriprost potassium) or a pure cyclo-oxygenase inhibitor, flurbiprofen. These data define the properties of AA as a secretory stimulus for human PMNs.

Published

1987

24. Immunological studies of anergic patients.

Author

Van Epps DE, Frierson JA, and Williams RC

Abstract

Sixty-one patients with a variety of different illnesses were studied with respect to skin test anergy and the presence of serum chemotactic inhibitors. In initial testing, 55% of the patient tests demonstrated negative skin test responses to all six test antigens. Sera from 65% of these anergic patients were capable of suppressing the migration of normal polymorphonuclear leukocytes toward chemotactic factors. Statistical analysis of the association of anergy and chemotactic inhibitory sera resulted in a P value of <0.0005. Chemotactic inhibitory sera were also capable of suppressing monocyte chemotaxis. No association of chemotactic inhibitory activity and lymphocytotoxic antibody or suppressors of mitogen-induced lymphocyte blast transformation were noted. In addition, T-cell populations in some anergic patients were studied by the erythrocyte-binding technique. Erythrocyte-binding lymphocytes in anergic patients were significantly suppressed when compared to normal controls, but not when compared to skin test-positive patients. The data presented here indicate a close parallel between skin test anergy and the presence of serum chemotactic inhibitory activity. The exact relationship is yet undefined but may indicate the involvement of chemotactic inhibitors as immunological regulators in the host during a variety of systemic illnesses.

Published

1974

25. Decreased T lymphocyte migration in patients with malignancy mediated by a suppressor cell population.

Author

Hesse DG, Cole DJ, Van Epps DE, and Williams RC Jr

Subjects

Adolescent, Adult, Aged, Caseins pharmacology, Cell Movement, Concanavalin A physiology, Female, Humans, Immunity, Cellular, Male, Middle Aged, T-Lymphocytes immunology, Chemotaxis, Leukocyte, Lymphokines, Neoplasms immunology, T-Lymphocytes, Regulatory immunology

Abstract

The migration and concentration of lymphocytes at sites of antigenic challenge are an integral part of the expression of delayed cutaneous hypersensitivity, as well as of tumor and graft rejection. In this study, we have analyzed the migration of T lymphocytes from patients with malignancy. We used casein and concanavalin A (Con A)-stimulated mononuclear cell supernatants to stimulate T cell locomotion. Peripheral blood T lymphocytes from 30 patients with established malignancy, 10 patients with indolent malignancy or benign tumor, and 42 normal adult controls were tested. Data are expressed as a migration index (MI), which represents the difference in micrometers between the distance migrated in response to a stimulus and the distance migrated in response to media alone. We observed a marked depression in casein-stimulated T lymphocyte migration in patients with established malignancy (mean MI +/- 1 SD = 17.0 +/- 9 microns) as compared with normal adult controls (mean MI +/- 1 SD = 35.3 +/- 10 microns). Similar results were observed with migration in response to Con A supernatants. T cells from patients with established malignancy had a mean MI of 5.8 +/- 4 microns to Con A supernatants as compared with 24.5 +/- 5 for controls. This depressed migration was apparent both in the distance that cells migrated and in the number of cells that migrated into the membrane. Of 10 patients with indolent malignancy or benign tumor, T cell migration in 8 was not significantly decreased as compared with controls. When we mixed equal concentrations of normal control T lymphocytes with T lymphocytes from patients with cancer and added the mixture directly to the upper compartment of the chemotaxis chamber, the response of the normal T cells to casein was inhibited by an average of 48%. We observed inhibition of this migration of normal cells when we added as little as 10% of patient cells to normal cells. When we mixed normal control T lymphocytes from different donors and added them directly to the upper compartment of the chemotaxis chamber, T lymphocyte migration in response to casein was not significantly altered. If T cells from patients with cancer were cultured overnight, the suppressive effect on lymphocyte locomotion was lost. Our results indicate that there is a population of T lymphocytes in patients with cancer that suppress normal T lymphocyte migration. This suppressor activity may partially explain the subversion of immunosurveillance in established neoplastic states, as well as the defective inflammatory reaction to intradermal injection of antigen observed in many patients with malignancy.

Published

1984

26. Rapid separation of lipid classes in high yield and purity using bonded phase columns.

Author

Kaluzny MA, Duncan LA, Merritt MV, and Epps DE

Subjects

Cholesterol Esters isolation & purification, Chromatography, High Pressure Liquid methods, Chromatography, Thin Layer methods, Fatty Acids, Nonesterified isolation & purification, Phospholipids isolation & purification, Triglycerides isolation & purification, Lipids isolation & purification

Abstract

A method utilizing aminopropyl bonded phase (Bond Elut) columns has been developed to separate lipid mixtures into individual classes in high yield and purity. Up to ten lipid mixtures can be processed in 1 hr and the columns are reusable after suitable washing. Although the method was developed with standard lipid mixtures, it was shown that it is also applicable to biological extracts. Due to the rapidity and high yields (greater than 95%) of this procedure, it is superior to preparative HPLC or TLC, or other chromatographic methods for the separation of lipid mixtures for subsequent analysis.

Published

1985

27. Correlation of serum opsonic activity in cystic fibrosis with colonization and disease state: measurement of opsonins to Pseudomonas aeruginosa by neutrophil superoxide anion generation.

Author

Bender JG, Florman AL, and Van Epps DE

Subjects

Adolescent, Adult, Child, Cystic Fibrosis complications, Female, Humans, Male, Opsonin Proteins analysis, Pseudomonas Infections complications, Cystic Fibrosis immunology, Neutrophils immunology, Opsonin Proteins immunology, Pseudomonas Infections immunology, Pseudomonas aeruginosa immunology, Superoxides metabolism

Abstract

Serum from patients with cystic fibrosis and normal controls was used to opsonize mucoid and nonmucoid Pseudomonas aeruginosa particles. Opsonic activity was then determined by measuring the production of superoxide anion (O2-) from normal neutrophils stimulated with the opsonized particles. Without any opsonization, mucoid P. aeruginosa stimulated significantly more O2- than nonmucoid P. aeruginosa. Responses to nonmucoid P. aeruginosa observed with heat-inactivated serum from patients with cystic fibrosis were significantly higher (p = 0.008) than those observed with heat-inactivated control sera. Comparisons made between patients who were colonized with P. aeruginosa and those who were not showed that heat activated serum from colonized patients had significantly higher levels of opsonic activity than heat inactivated serum from patients who were not colonized. These differences were observed with either mucoid or nonmucoid P. aeruginosa. A negative correlation was also observed between opsonic activity and clinical status measured by Schwachman scores of colonized patients. These data indicate that in patients colonized with P. aeruginosa the deterioration of their clinical status correlated with increased opsonic activity reflected in the oxidative burst response of neutrophils.

Published

1987

28. Diet induced atherogenic hyperlipoproteinaemia and liver injury in cynomolgus macaques.

Author

Hunt CE, Diani AR, Brown PK, Kaluzny MA, and Epps DE

Subjects

Animals, Cholangitis etiology, Coronary Vessels pathology, Fatty Acids blood, Hyperlipoproteinemias pathology, Lipids blood, Lipoproteins blood, Liver pathology, Liver Diseases pathology, Macaca fascicularis, Male, Diet, Atherogenic, Hyperlipoproteinemias etiology, Liver Diseases etiology

Abstract

This study was conducted to determine the efficacy of an experimental anti-atherosclerosis drug in the adult male cynomolgus monkey. A semipurified diet containing 0.5% cholesterol and 25.5% butter was fed to groups of 20, each, drug and placebo-treated animals for 18 months. Similar liver and arterial changes were present in both groups. However, we report here tissue changes seen in animals given placebo only, with plasma lipid and lipoprotein values of placebo-treated animals compared to those in animals fed nonatherogenic commercial ration. Animals fed atherogenic diet had enlarged livers (mean 3.9% b.w.), and all had evidence of hepatocellular lipid accumulation which was often marked and diffuse. Cholangitis was common including mononuclear cell infiltration, bile ductule proliferation and portal tract fibrosis. Five animals had severe portal fibrosis with bands of connective tissue extending into and around lobules (bridging fibrosis). All animals fed atherogenic diet developed hypercholesterolemia (greater than 600 mg/dl) which was the result of a three-fold increase in five cholesterol and cholesterol ester. Oleic acid was increased and linoleic acid was reduced in plasma phospholipids and cholesterol esters. Plasma lipoprotein distribution was altered with a marked increase in low density lipoproteins, increased very low density lipoproteins and decreased high density lipoproteins. These changes were undoubtedly caused by diet, i.e., high in cholesterol and saturated fat and limiting in linoleic acid. It is probable that diet-induced liver injury would affect the pathogenesis of atherosclerosis in this model since the liver is central in the synthesis and metabolism of lipoproteins.

Published

1986

29. Cyanamide mediated syntheses under plausible primitive earth conditions. V. The synthesis of phosphatidic acids.

Author

Epps DE, Sherwood E, Eichberg J, and Oró J

Subjects

Imidazoles, Phospholipids chemical synthesis, Temperature, Cyanamide, Cyanides, Phosphatidic Acids chemical synthesis

Abstract

A mixture of ammonium palmitate, 14C-sn-glycero-1(3)-phosphate, cyanimide and imidazole when heated for several hours formed significant quantities of phospholipids. These reaction products were shown by chromatographic, chemical and enzymatic procedures to be monopalmitoylglycerophosphate (MPGP), dipalmitoylglycerophosphate (DPGP) and monopalmitoyl cyclic glycerophosphate (cMPGP). A portion of the MPGP and DPGP possessed the same steric configuration as naturally occurring lysophosphatidic acid and phosphatidic acid. The yield of total phospholipid was maximal at temperatures between 60 degrees and 90 degrees after 8 h. When ratios of reactants were varied, up to 45% of radioactive glycerophosphate was converted into phospholipids. The average proportions of individual phosphatidic acids were: 60% MPGP, 27% DPGP and 13% cMPGP. Evidence was obtained for a synergistic relationship between cyanamide and imidazole in promoting the formation of phosphatidic acids. These results suggest that phosphatidic acids, which are essential precursors for the biochemical synthesis of more complex membrane phospholipids, could have been produced on the primitive Earth.

Published

1978

30. Suppression of leukocyte chemotaxis by human IgA myeloma components.

Author

Van Epps DE and Williams RC Jr

Subjects

Caseins, Dithiothreitol, Hot Temperature, Humans, Immunoglobulin A, Secretory pharmacology, Immunoglobulin G, Models, Biological, Monocytes physiology, Myeloma Proteins, Neutrophils physiology, Pepsin A, Receptors, Drug, Structure-Activity Relationship, Waldenstrom Macroglobulinemia blood, Chemotaxis, Leukocyte, Immunoglobulin A analysis

Abstract

Sera from patients with IgA myeloma suppressed polymorphonuclear leukocyte (PMN) chemotaxis, while generally little or no suppression was observed with sera from patients with IgG myeloma or Waldenstrom's macroglobulinemia. Chemotactic inhibitory activity was not limited to a single chemotactic factor and was equivalent when C5a, bacterial factor, casein, or normal serum were used as chemotactic attractants. No association was noted between the degree of inhibitory activity and the IgA subclass or light chain type. Chemotactic inhibitory activity was found to be directly associated with isolated IgA M components, and similar chemotactic suppression was noted with purified preparations of normal human colostral IgA. By comparison, IgA preparations were most effective in suppressing PMN chemotaxis and had a much lesser effect on monocyte chemotaxis. The mode of IgA chemotactic inhibition was cellular and at least partially reversible after a 37degreesC incubation in the absence of IgA. Some inhibition of PMN random mobility was noted with certain IgA preparations, although such effects did not parallel the degree of chemotactic inhibition. Fractionation of IgA myeloma sera and IgA M components by sucrose density gradient centrifugation showed multiple peaks of inhibitory activity in 10 to 13S fractions. The majority of IgA inhibitory activity was lost after pepsin digestion or sulfhydryl reduction and alkylation of isolated M components. When isolated IgA M components were fractionated on Sephadex G-200, inhibitory activity was associated with the exclusion volume and was abolished by reduction and alkylation procedures which resulted in a conversion of polymeric IgA to monomeric IgA.

Published

1976

31. In vivo neutrophil emigration in response to interleukin-1 and tumor necrosis factor-alpha.

Author

Mason MJ and Van Epps DE

Subjects

Animals, Cell Movement drug effects, Complement C5 pharmacology, Complement C5a, Mice, Mice, Inbred C3H, N-Formylmethionine Leucyl-Phenylalanine analogs & derivatives, N-Formylmethionine Leucyl-Phenylalanine pharmacology, Neutrophils physiology, Interleukin-1 pharmacology, Neutrophils drug effects, Tumor Necrosis Factor-alpha pharmacology

Abstract

The migration of polymorphonuclear leukocytes (PMN) in response to recombinant interleukin-1 (IL-1), tumor necrosis factor-alpha (TNF), C5a, and f-met-leu-phe-lys (FMLPL) in vivo was studied using a mouse subcutaneous sponge implantation model. In this model sponges were implanted in C3H/OUJ mice, and 2 days later they were injected with the test sample. After varying times, sponges were removed and digested with collagenase, and total cell counts and differentials were enumerated. IL-1 was found to stimulate a significant influx of PMN, which peaked at 6 hr and declined to near baseline levels by 24 hr. This response was dose-dependent, with the greatest response observed when 5 units of IL-1 were injected. When the IL-1 concentration was increased to 10 U, the total number of PMN migrating into the sponge was decreased, compared with that observed with 5 U of IL-1. The overall number of PMN migrating into the sponge 6 hr after injecting 5 U of IL-1 averaged 269% of the number of PMN migrating randomly into the sponge. No difference in the total number of macrophages or lymphocytes in control or IL-1-injected sponges was observed in this time frame. Heat treatment of the IL-1 at 90 degrees C for 30 min ablated the response. Similar studies with TNF and C5a showed that both of these agents also stimulated an influx of PMN that peaked 6 hr postinjection. In contrast, FMLPL did not stimulate a PMN response. When IL-1 and TNF were injected simultaneously, an additive response was observed. These data indicate that IL-1, TNF, and C5a can all stimulate a PMN response in vivo and support the hypothesis that these substances are actively involved in the mobilization of PMN to inflammatory sites in vivo.

Published

1989

32. Inhibition of formylmethionyl-leucyl-phenylalanine-stimulated neutrophil chemiluminescence by human immunoglobulin A paraproteins.

Author

Van Epps DE and Brown SL

Subjects

Alkylation, Luminescent Measurements, N-Formylmethionine antagonists & inhibitors, N-Formylmethionine Leucyl-Phenylalanine, Oxidation-Reduction, Paraproteins, Peptide Fragments analysis, Structure-Activity Relationship, Chemotaxis, Leukocyte drug effects, Immunoglobulin A immunology, Methionine analogs & derivatives, N-Formylmethionine analogs & derivatives, Neutrophils physiology, Oligopeptides antagonists & inhibitors

Abstract

Immunoglobulin A (IgA) paraproteins from patients with myeloma have been shown to inhibit human neutrophil chemotaxis to C5a, casein, and chemotactic factors produced by Escherichia coli. This study demonstrates that these paraproteins also inhibit neutrophil chemotaxis in response to the synthetic peptide formylmethionyl-leucyl-phenylalanine (f-MLP). Furthermore, the neutrophil chemiluminescence response stimulated by f-MLP was markedly suppressed by the presence of IgA paraprotein. Maximal inhibition of chemiluminescence was observed when the paraprotein was present during the chemiluminescence response. The inhibitory activity was substantially reduced by removal of the Fc region of IgA or by conversion of polymeric IgA to monomeric IgA by limited reduction and alkylation. Additional experiments showed that these IgA paraproteins inhibited C5a but not phorbol myristate acetate-stimulated chemiluminescence. These observations are constant with the hypothesis that polymeric forms of IgA bind to human neutrophils and interfere with the binding of chemotactic factor to its receptor or the consequent receptor-mediated oxidative burst or both.

Published

1981

33. Leukocyte C5a receptor modulation during hemodialysis.

Author

Lewis SL, Van Epps DE, and Chenoweth DE

Subjects

Female, Flow Cytometry, Humans, In Vitro Techniques, Kidney Failure, Chronic therapy, Leukocyte Count, Male, Middle Aged, Receptor, Anaphylatoxin C5a, Receptors, IgG, Receptors, Immunologic analysis, Complement C5 metabolism, Kidney Failure, Chronic blood, Leukocytes metabolism, Receptors, Complement metabolism, Renal Dialysis

Abstract

Exposure of blood to hemodialysis (HD) membranes results in the activation of the complement system. In this study, flow cytometry was used to analyze the binding of fluoresceinated chemotactic factors (C5a, f-Met-Leu-Phe-Lys [fMLPL], and casein) and aggregated IgG to PMN and monocytes isolated from normal whole blood following passage through a hemodialyzer. Analysis of ligand binding by these PMN and monocytes showed no difference in the binding of casein, fMLPL, or aggregated IgG throughout the 45 minute procedure. In contrast, a progressive decrease in the binding of C5a by PMN and monocytes occurred. By 45 minutes, the average percentage of PMN binding C5a had dropped from 95 to 61% and monocytes from 73 to 40%. In additional studies, blood samples were obtained from chronic renal failure patients undergoing hemodialysis at four different time intervals during dialysis. Total white blood cell (WBC) counts showed that the mean WBC count at 30 minutes dropped to 60.9% of the predialysis WBC count, and rebounded to 133.8% by two hours and 128.2% by four hours. Analysis of the binding of C5a, casein, fMLPL, or aggregated IgG by PMN or monocytes from HD patients indicated there were no significant differences at the four time intervals studied. When blood samples from normal subjects or chronic hemodialysis patients were incubated in vitro with dialysis membrane fibers, a loss of identifiable C5a receptors was observed on PMN from normal blood, while PMN from HD patients showed no significant change in the percentage of C5a-receptor-positive cells.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1987

34. A model for the regulation of myelopoiesis by specific factors.

Author

Bender JG, Van Epps DE, and Stewart CC

Subjects

Animals, Cell Differentiation, Cell Division, Cells, Cultured, Models, Biological, Bone Marrow Cells, Hematopoiesis, Hematopoietic Stem Cells cytology

Abstract

Hematopoietic cells originate from stem cells that generate progenitor cells programmed to differentiate along specific cell lineages. Recently, a number of factors have been identified that are involved in regulating the proliferation of myeloid lineage cells. We propose a model in which a hierarchy of specific factors acts sequentially during defined stages of maturation to regulate myelopoiesis. The role of these factors as competence or progression factors in causing cells to enter and traverse the cell cycle is discussed. Experimental evidence supports the model.

Published

1986

35. Modulation of neutrophil-reduced pyridine nucleotide content following stimulation with phorbol myristate acetate and chemotactic factors.

Author

Van Epps DE, Bender JG, Steinkamp JA, and Chenoweth DE

Subjects

Complement C5 pharmacology, Complement C5a, Cytochalasin B pharmacology, Dose-Response Relationship, Drug, Granulomatous Disease, Chronic blood, Humans, N-Formylmethionine Leucyl-Phenylalanine pharmacology, Neutrophils drug effects, Oxidation-Reduction, Superoxides metabolism, Tetradecanoylphorbol Acetate pharmacology, NADP metabolism, Neutrophils physiology

Abstract

Modulation of NAD(P)H in human neutrophils (PMN) following stimulation with phorbol myristate acetate (PMA) or chemotactic factors was determined by flow cytometry. Stimulation of PMN with 1 microgram/ml of PMA results in a time-dependent decrease in fluorescence, attributable to the oxidation of NAD(P)H. The decrease in fluorescence did not occur with PMN from a patient with chronic granulomatous disease (CGD) and was observed in only half of PMN from the mother of the patient. Loss of fluorescence in normal PMN was maximal following 7-15 min of stimulation with PMA. Simultaneous measurement of PMA-stimulated NAD(P)H oxidation and H2O2 production showed that NAD(P)H oxidation occurred as an all-or-none response while H2O2 production showed a graded response. These data suggest that with PMA stimulation, a threshold exists beyond which constitutive NAD(P)+ reduction is suppressed and complete oxidation of NAD(P)H occurs, while H2O2 production is proportional to the concentration of PMA. PMA-stimulated oxidation of NAD(P)H was reversible, and fluorescence returned to the initial level or higher after 40-60 min. Oxidation of NAD(P)H also occurred when cytochalasin B-treated PMN were stimulated with 25 nM C5a or 100 nM formyl-methionyl-leucyl-phenylalanine (f-MLP), but occurred more rapidly, peaking at 1 to 3 min. Fluorescence also returned by 5-6 min. This response to C5a and f-MLP was graded and proportional to the concentration of chemotactic factor used. Comparative studies showed that the cytochalasin-B treatment was essential for measurement of NAD(P)H oxidation, in response to C5a and F-MLP.

Published

1985

36. Cyanamide mediated synthesis under plausible primitive earth conditions. VI. The synthesis of glycerol and glycerophosphates.

Author

Epps DE, Nooner DW, Eichberg J, Sherwood E, and Oró J

Subjects

Biological Evolution, Chemical Phenomena, Chemistry, Cyanamide pharmacology, Cyanides pharmacology, Glycerol chemical synthesis, Glycerophosphates chemical synthesis

Abstract

The formation of glycerol occurs when a solution of DL-glyceraldehyde is heated in the presence of hydrogen sulfide at room temperature. DL-glyceraldehyde and dihydroxyacetone treated with hydrazine, as well as DL-glyceraldehyde incubated with formaldehyde are also partially converted to glycerol. The yields of the above reactions are from approximately 1% to about 3%. The formation of glycerophosphates occurs when glycerol is heated with ammonium dihydrogen phosphate and either urea or cyanamide. The yield of glycerophosphates is about 30%, most of which is sn-glycero-1 (3)-phosphate. These findings indicate that glycerol and sn-glycero-3-phosphate, which are moieties of glycerolipids, could have been formed under conditions which may have prevailed on the primitive Earth.

Published

1979

37. Cyanamide mediated syntheses under plausible primitive earth conditions. IV. The synthesis of acylglycerols.

Author

Eichberg J, Sherwood E, Epps DE, and Oró J

Subjects

Chemical Phenomena, Chemistry, Diglycerides, Hot Temperature, Imidazoles, Kinetics, Palmitates, Triglycerides, Glycerides, Glycerol

Abstract

The synthesis of palmitoylglycerols in good yields occurs when a solution of glycerol, ammonium palmitate, cyanamide and imidazole is dried and heated at ambient humidity at temperatures ranging from 60 degrees--100 degrees C for 16 h. Much less product is formed in the absence of either or both cyanamide or imidazole. This work suggests that acylglycerols could have been synthesized on the primitive Earth under plausible prebiotic conditions which were similar but not identical to those which have been shown to condense deoxynucleotides into oligodeoxynucleotides and amino acids into peptides.

Published

1977

38. Inhibition of permeability-dependent Ca2+ release from mitochondria by N-acylethanolamines, a class of lipids synthesized in ischemic heart tissue.

Author

Epps DE, Palmer JW, Schmid HH, and Pfeiffer DR

Subjects

Animals, Biological Transport, Active drug effects, Endocannabinoids, Ethanolamines metabolism, Intracellular Membranes metabolism, Kinetics, Male, Mitochondria, Heart drug effects, Mitochondria, Liver drug effects, Oleic Acids, Permeability, Rats, Rats, Inbred Strains, Structure-Activity Relationship, Tissue Distribution, Calcium metabolism, Ethanolamines pharmacology, Mitochondria, Heart metabolism, Mitochondria, Liver metabolism

Published

1982

39. Use of a rapid and highly sensitive fluorescamine-based procedure for the assay of plasma lipoproteins.

Author

Funk GM, Hunt CE, Epps DE, and Brown PK

Subjects

Colorimetry methods, Fluorescamine, Humans, Iodine Radioisotopes, Lipoproteins, HDL blood, Lipoproteins, LDL blood, Lipoproteins, VLDL blood, Male, Reference Values, Spectrometry, Fluorescence methods, Lipoproteins blood

Abstract

A rapid and sensitive method for determining protein concentrations using fluorescamine has been characterized for use in the analysis of intact lipoproteins. It was shown that there is no interference with the assay due to the presence of lipid-associated turbidity or primary amine content. The assay was shown to be sensitive to as little as 0.3 microgram of lipoprotein and to yield similar results when compared to the Lowry method.

Published

1986

40. Age-dependent variations in polymorphonuclear leukocyte chemiluminescence.

Author

Van Epps DE, Goodwin JS, and Murphy S

Subjects

Adolescent, Adult, Age Factors, Aged, Child, Preschool, Hemolysis, Humans, Infant, Infant, Newborn, Kinetics, Luminescent Measurements, Phagocytosis, Fetal Blood immunology, Neutrophils immunology

Abstract

Polymorphonuclear leukocytes from 46 adults (age 18 to 35), 19 adults (age 70 to 91), 10 children (age 1 to 3), and 22 neonates (cord blood samples) were tested for their chemiluminescence response to opsonized zymosan. Results indicated that both cord blood leukocytes and those from individuals over 70 were significantly lower (P less than 0.05) in their chemiluminescence response. Furthermore, when the latter group was divided into two subsets, one containing subjects over 80 years of age and the other containing subjects between 70 and 80 years of age, those over 80 showed a chemiluminescence response significantly lower (P less than 0.05) than those between 70 and 80. The kinetics of the chemiluminescence response was similar with all samples except the neonatal cells, where the response appeared to peak and subside more slowly. These data demonstrate that polymorphonuclear leukocyte chemiluminescence is depressed in the very young and the very old.

Published

1978

41. Isolation of streptolysin O by preparative polyacrylamide gel electrophoresis.

Author

Van Epps DE and Andersen BR

Subjects

Chromatography, Chromatography, Gel, Electrophoresis, Polyacrylamide Gel, Streptolysins isolation & purification

Abstract

Streptolysin O giving a single band by Ouchterlony and acrylamide gel analysis has been isolated by ammonium sulfate precipitation, Sephadex gel filtration chromatography, and preparative polyacrylamide gel electrophoresis.

Published

1973

42. Streptolysin O: sedimentation coefficient and molecular weight determinations.

Author

Van Epps DE and Andersen BR

Subjects

Centrifugation, Density Gradient, Chromatography, Gel, Ultracentrifugation, Molecular Weight, Streptolysins analysis

Abstract

The sedimentation coefficient of streptolysin O as determined by sucrose density gradient ultracentrifugation is 3.7S. An approximate molecular weight of 60,500 was calculated from the sedimentation velocity, and a similar value was obtained by Sephadex gel filtration. There was no measurable difference in the sedimentation coefficient of streptolysin O in either the active or reversibly inactive forms, indicating that there were at most only minor conformational differences between the two forms.

Published

1969

43. Suppression of chemotatic activity of human neutrophils by streptolysin O.

Author

Andersen BR and Van Epps DE

Subjects

Antistreptolysin blood, Antistreptolysin pharmacology, Chromatography, Gel, Electrophoresis, Hemolysis, Hot Temperature, Humans, Neutrophils immunology, Neutrophils physiology, Oxidation-Reduction, Streptococcus pyogenes analysis, Streptolysins antagonists & inhibitors, Streptolysins isolation & purification, Time Factors, Chemotaxis drug effects, Neutrophils drug effects, Streptolysins pharmacology

Published

1972

44. Streptolysin O II. Relationship of Sulfyhdryl Groups to Activity.

Author

Van Epps DE and Andersen BR

Abstract

Streptolysin O (SO), a group A streptococcal toxin, exists in two forms, a reduced active state and an oxidized reversibly inactive state. Activity is measured by red blood cell hemolysis. SO is a labile toxin, and, with time, activity is irreversibly lost. The rate of activity loss is slowed by incubation with 0.1 m 2-mercaptoethanol or 0.01 m ethylenediaminetetraacetic acid (EDTA). The effect of EDTA can be reversed by excess MgSO(4). Reversibly oxidized SO is activated by cleavage of disulfide bonds. When the free sulfhydryl groups of the active SO are alkylated with iodoacetamide, complete and irreversible loss of activity results. Periodate (0.01 m) oxidation also causes complete loss of activity which may be due to oxidation of sulfhydryl groups. SO in the active form reacts with Fe(2+), Cu(2+), Ca(2+), and Mg(2+), causing loss of activity in various degrees depending on the ions and the concentration used. Ferric and cupric ions are most effective and cause loss of activity at concentrations on the order of 10(-4)m. The reversibly oxidized form of SO is not influenced by exposure to cupric ions (0.01 m), indicating that the reaction is only with the active form of SO, probably involving the free sulfhydryl groups. These groups may be responsible for the direct binding of the toxin to the target membrane or for the maintenance of the proper conformation for activity.

Published

1971