Your search keyword '"Epps DE"' showing total 181 results

1. Clinical impact of ex vivo differentiated myeloid precursors after high-dose chemotherapy and peripheral blood progenitor cell rescue

Author

Zimmerman, TM, Lee, WJ, Bender, JG, Schilling, M, Smith, SL, Van Epps, DE, and Williams, SF

Published

2000

2. Spectroscopic analysis of [Trp3]-β-casomorphin analogs Comparative structure conformation-activity studies

Author

EPPS, DE., primary, HAVEL, HA., additional, SAWYER, T.K., additional, STAPLES, D.J., additional, CHUNG, N.N., additional, SCHILLER, P.W., additional, HARTRODT, B., additional, and BARTH, A., additional

Published

2009

3. A flow cytometric method for counting very low levels of white cells in blood and blood components

Author

Vachula, M, primary, Simpson, SJ, additional, Martinson, JA, additional, Aono, FM, additional, Hutchcraft, AM, additional, Balma, DL, additional, and Epps, DE, additional

Published

1993

4. 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

5. Spectroscopic analysis of [Trp3]-β-casomorphin analogs Comparative structure conformation-activity studies.

Author

EPPS, DE., HAVEL, HA., SAWYER, T.K., STAPLES, D.J., CHUNG, N.N., SCHILLER, P.W., HARTRODT, B., and BARTH, A.

Published

1991

6. 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

7. Mediators and Modulators of Human Lymphocyte Chemotaxis

Author

van Epps De

Subjects

Human lymphocyte, Text mining, In Vitro Techniques, business.industry, Immunology, Medicine, Chemotaxis, business, Dinoprostone

Published

1983

8. Regulation of myelopoiesis

Author

James G. Bender, Van Epps De, and Stewart Cc

Subjects

Myeloid, Cellular differentiation, medicine.medical_treatment, Immunology, Bone Marrow Cells, Biology, Microbiology, Colony-Stimulating Factors, Bone Marrow, medicine, Immunology and Allergy, Animals, Humans, Progenitor cell, Growth Substances, General Veterinary, Growth factor, Macrophages, Stem Cells, Cell Differentiation, General Medicine, Hematopoietic Stem Cells, Cell biology, Hematopoiesis, Haematopoiesis, Infectious Diseases, medicine.anatomical_structure, Bone marrow, Myelopoiesis, Stem cell, Cell Division, Granulocytes

Abstract

Myeloid cells are produced by the bone marrow from stem cells and progenitor cells. This review summarizes the current understanding of how this process is regulated. Regulation of progenitor cell proliferation and differentiation occurs in microenvironments present within the bone marrow as well as on the systemic level by the release of regulators into the circulation. The regulators of central importance to myelopoiesis are growth factors necessary for the proliferation and differentiation of progenitors. These growth factors have recently been characterized and studies indicate that there is a hierarchy of factors acting upon successive differentiation stages of progenitors. Endotoxin appears to be a major modulator of myeloid growth factor production. Other inhibitors of myelopoiesis are also discussed. Regulation of myelopoiesis therefore involves a balance between growth factor production and inhibition by other factors.

Published

1987

9. 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

10. Histological characterization of human breast implant capsules.

Author

Bui JM, Perry T, Ren CD, Nofrey B, Teitelbaum S, and Van Epps DE

Subjects

Biopsy, Needle, Case-Control Studies, Female, Humans, Immunohistochemistry, Linear Models, Myofibroblasts pathology, Reference Values, Retrospective Studies, Sampling Studies, Statistics, Nonparametric, Breast Implants adverse effects, Implant Capsular Contracture pathology, Implant Capsular Contracture prevention & control, Prosthesis Design

Abstract

Background: This study investigated the relationships between histomorphological aspects of breast capsules, including capsule thickness, collagen fiber alignment, the presence of α-smooth muscle actin (α-SMA)-positive myofibroblasts, and clinical observations of capsular contracture., Methods: Breast capsule samples were collected at the time of implant removal in patients undergoing breast implant replacement or revision surgery. Capsular contracture was scored preoperatively using the Baker scale. Histological analysis included hematoxylin and eosin staining, quantitative analysis of capsule thickness, collagen fiber alignment, and immunohistochemical evaluation for α-SMA and CD68., Results: Forty-nine samples were harvested from 41 patients. A large variation in histomorphology was observed between samples, including differences in cellularity, fiber density and organization, and overall structure. Baker I capsules were significantly thinner than Baker II, III, and IV capsules. Capsule thickness positively correlated with implantation time for all capsules and for contracted capsules (Baker III and IV). Contracted capsules had significantly greater collagen fiber alignment and α-SMA-positive immunoreactivity than uncontracted capsules (Baker I and II). Capsules from textured implants had significantly less α-SMA-positive immunoreactivity than capsules from smooth implants., Conclusion: The histomorphological diversity observed between the breast capsules highlights the challenges of identifying mechanistic trends in capsular contracture. Our findings support the role of increasing capsule thickness and collagen fiber alignment, and the presence of contractile myofibroblasts in the development of contracture. These changes in capsule structure may be directly related to palpation stiffness considered in the Baker score. Approaches to disrupt these processes may aid in decreasing capsular contracture rates., Level of Evidence Iii: This journal requires that authors assign a level of evidence to each article. For a full description of these Evidence-Based Medicine ratings, please refer to the Table of Contents or the online Instructions to Authors www.springer.com/00266 .

Published

2015

11. Erratum to: Histological Characterization of Human Breast Implant Capsules.

Author

Bui JM, Perry T, Ren CD, Nofrey B, Teitelbaum S, and Van Epps DE

Published

2015

12. A novel source of viable peripheral blood mononuclear cells from leukoreduction system chambers.

Author

Dietz AB, Bulur PA, Emery RL, Winters JL, Epps DE, Zubair AC, and Vuk-Pavlović S

Subjects

Dendritic Cells cytology, Enterotoxins pharmacology, Hematopoietic Stem Cells cytology, Humans, Immunomagnetic Separation, Lipopolysaccharide Receptors analysis, Leukocyte Reduction Procedures methods, Leukocytes, Mononuclear cytology

Abstract

Background: Buffy coats are becoming less available as a source of research-grade peripheral blood mononuclear cells (PBMNCs). Therefore, alternative sources of these cells were investigated., Study Design and Methods: PBMNCs isolated from the cells retained in leukoreduction system chambers (LRSCs) and those eluted from white blood cell filters were compared. From LRSCs (1.88 +/- 0.40) x 10(9) PBMNCs (n = 13) versus (0.43 +/- 0.15) x 10(9) PBMNCs were isolated from leukofilter eluates (LFEs, n = 8; p < 0.0001)., Results: Cells from LRSCs and LFEs produced similar numbers of burst-forming unit-erythroid, colony-forming unit (CFU)-granulocyte-macrophage, and CFU-granulocyte-erythrocyte-monocyte-macrophage-megakaryocyte colonies. The percentages of cells positive for CD3, CD4, CD8, CD14, CD19, and CD56 in the PBMNCs isolated from LRSCs and LFEs were indistinguishable. Cells isolated from LRSCs expressed higher levels of CD69 and CD25 in reaction to staphylococcal enterotoxin B than the cells isolated from LFEs. The source of cells affected neither the yield and purity of immunomagnetically isolated CD3+ cells, CD14+ cells, and CD56+ cells nor the function of T cells, natural killer cells, and in vitro matured dendritic cells (DCs). DC yield from LRSC-derived CD14+ cells, however, was higher., Conclusion: LRSCs are a novel source of fully functional PBMNCs that can replace the more traditional sources of research-grade cellular products.

Published

2006

13. Specific active immunotherapy of cancer: potential and perspectives.

Author

Srinivasan R and Van Epps DE

Subjects

Antibodies, Monoclonal therapeutic use, Antigens, Neoplasm, Cancer Vaccines pharmacology, Dendritic Cells immunology, Humans, Neoplasms immunology, Cancer Vaccines therapeutic use, Immunotherapy, Active methods, Neoplasms therapy

Abstract

Extensive research over the past two decades in tumor immunology has shown that immune reactivity to tumor antigens can restrict tumor growth and/or metastasis, especially when tumor burden is low. These observations in experimental models have been translated into clinical studies involving both active and passive forms of immunotherapies. While immune responses to specific tumor antigens can be detected in patients with various types of cancers, responses to any single antigen seldom correlate directly with a clinical response to tumors; however, some clinical regressions of solid tumors have been reported with certain types of cancer vaccines. While passive immunotherapies with antibody to tumor antigens (Avastin, Herceptin, Erbitux, Rituxan, Bexxar) are being used to treat selected types of cancers, active immunotherapies may be better suited to potentially elicit a sustained immune response, particularly when administered in an adjuvant setting. This review covers the potential and issues with specific active immunotherapies (SAI) for the treatment of cancer.

Published

2006

14. Isoform-specific interactions of human apolipoprotein E to an intermediate conformation of human Alzheimer amyloid-beta peptide.

Author

Stratman NC, Castle CK, Taylor BM, Epps DE, Melchior GW, and Carter DB

Subjects

Apolipoprotein E2, Apolipoprotein E3, Apolipoprotein E4, Enzyme-Linked Immunosorbent Assay, Humans, Protein Binding, Protein Isoforms chemistry, Protein Structure, Tertiary, Amyloid beta-Peptides chemistry, Apolipoproteins E chemistry, Peptide Fragments chemistry

Abstract

Brain plaque deposits of amyloid-beta peptide (Abeta) is a pathological hallmark of Alzheimer's disease (AD) and apolipoprotein E (apoE) is thought to be involved in its deposition. One hypothesis for the role of apoE in the pathogenesis of AD is that apoE may be involved in deposition or clearance of Abeta by direct protein-to-protein interaction. Lipidated apoE4 bound preferentially to an intermediate aggregated form of Abeta and formed two- to three-fold more binding complexes than isoforms apoE2 or apoE3. The interaction was detected by a sandwich ELISA with capture antibodies specific for the N-terminus of apoE, whereas the interaction was not recognized with a C-terminal antibody. The observations indicate that the C-terminus of apoE4 interacts with the intermediate form of Abeta. The differential risk of AD related to apoE genotype may be the result of an enhanced capacity of apoE4 binding to an intermediate aggregated form of Abeta.

Published

2005

15. A slowly formed transient conformer of Abeta(1-40) is toxic to inward channels of dissociated hippocampal and cortical neurons of rats.

Author

Sun XD, Mo ZL, Taylor BM, and Epps DE

Subjects

Alzheimer Disease pathology, Alzheimer Disease physiopathology, Amyloid beta-Peptides metabolism, Animals, Calcium Channels drug effects, Calcium Channels metabolism, Cell Culture Techniques methods, Cell Separation, Cerebral Cortex drug effects, Cerebral Cortex physiopathology, Female, Hippocampus drug effects, Hippocampus physiopathology, Ion Channels drug effects, Male, Membrane Potentials drug effects, Membrane Potentials physiology, Molecular Conformation, Neurons drug effects, Neurons pathology, Patch-Clamp Techniques, Peptide Fragments metabolism, Potassium Channels drug effects, Potassium Channels metabolism, Rats, Rats, Sprague-Dawley, Reaction Time drug effects, Reaction Time physiology, Sodium Channels drug effects, Sodium Channels metabolism, Alzheimer Disease metabolism, Amyloid beta-Peptides toxicity, Cerebral Cortex metabolism, Hippocampus metabolism, Ion Channels metabolism, Neurons metabolism, Peptide Fragments toxicity

Abstract

The mechanism by which amyloid peptide (Abeta(1-40)) produces effects on neurotransmission is currently unresolved. In initial experiments, using the patch-clamp technique, we found that 11.5 microM of preaggregated Abeta(1-40) altered the hippocampal neuron resting membrane potential and inhibited action potential firing. To identify the toxic species, the effects of Abeta(1-40) on sodium (I(Na)), calcium (I(Ca)), and potassium (I(K)) currents in hippocampal neurons were examined as a function of peptide aggregation state in a specially designed miniature recording chamber. Aggregation reactions were induced by constant shaking, starting with 50 microM monomeric peptide. At 10- to 30-min intervals, the ionic currents were examined on a single neuron suspended in control saline and then in a 100-microl sample of the aggregating peptide. We found that samples of the peptide taken 60-120 min into the aggregation process contained species that exhibited maximal inhibitory effects over a broad potential range in the rank ordering of I(Na) > I(Ca). I(K) was inhibited only slightly at depolarized potentials. Inhibition of APF through blockade of these channels would inhibit normal neuronal activity and directly contribute to cognitive dysfunction. In previous studies on SH-EP cells, we showed that neither monomeric nor fibrillar peptide had significant effect on cell viability except during exposure to the 60-120 minute aggregation product when cell death was recorded. Our kinetic model demonstrated that the toxic species was a slowly formed transient conformer (activated monomer), which was the only aggregating species that passed through a maximum concentration during aggregation. This species amounted to only a small fraction of the total amount of aggregating peptide. We conclude that, for both the native neurons in the present study as well as SH-EP1 cells, the activated monomeric conformer of the peptide is the toxic species.

Published

2003

16. Spontaneous aggregation and cytotoxicity of the beta-amyloid Abeta1-40: a kinetic model.

Author

Taylor BM, Sarver RW, Fici G, Poorman RA, Lutzke BS, Molinari A, Kawabe T, Kappenman K, Buhl AE, and Epps DE

Subjects

Animals, Antibodies, Monoclonal pharmacology, Cell Line, Cell Survival drug effects, Chromatography, High Pressure Liquid, Circular Dichroism, Fluorescence Polarization, Hippocampus cytology, Humans, Kinetics, Neurons drug effects, Protein Conformation, Rats, Rats, Sprague-Dawley, Amyloid beta-Peptides chemistry, Amyloid beta-Peptides toxicity, Peptide Fragments chemistry, Peptide Fragments toxicity

Abstract

The time dependency of the spontaneous aggregation of the fibrillogenic beta-amyloid peptide, Abeta1-40, was measured by turbidity, circular dichroism, HPLC, and fluorescence polarization. The results by all methods were comparable and they were most consistent with a kinetic model where the peptide first slowly forms an activated monomeric derivative (AM), which is the only species able to initiate, by tetramerization, the formation of linear aggregates. The anti-Abeta antibody 6E10, raised against residues 1-17, at concentrations of 200-300 nM delayed significantly the aggregation of 50 microM amyloid peptide. The anti-Abeta antibody 4G8, raised against residues 17-24, was much less active in that respect, while the antibody A162, raised against the C-terminal residues 39-43 of the full-length Abeta was totally inactive at those concentrations. Concomitant with the aggregation experiments, we also measured the time dependency of the Abeta1-40-induced toxicity toward SH-EPI cells and hippocampal neurons, evaluated by SYTOX Green fluorescence, lactate dehydrogenase release, and activation of caspases. The extent of cell damage measured by all methods reached a maximum at the same time and this maximum coincided with that of the concentration of AM. According to the kinetic scheme, the latter is the only transient peptide species whose concentration passes through a maximum. Thus, it appears that the toxic species of Abeta1-40 is most likely the same transient activated monomer that is responsible for the nucleation of fibril formation. These conclusions should provide a structural basis for understanding the toxicity of Abeta1-40 in vitro and possibly in vivo.

Published

2003

17. Physical methods to determine the binding mode of putative ligands for hepatitis C virus NS3 helicase.

Author

Sarver RW, Rogers JM, Stockman BJ, Epps DE, DeZwaan J, Harris MS, and Baldwin ET

Subjects

Adenosine Triphosphate analogs & derivatives, Adenosine Triphosphate metabolism, Adenosine Triphosphate pharmacology, Calorimetry methods, Calorimetry, Differential Scanning, Circular Dichroism, Crystallography, X-Ray, DNA metabolism, Enzyme Inhibitors metabolism, Enzyme Inhibitors pharmacology, Kinetics, Ligands, Nuclear Magnetic Resonance, Biomolecular, Protein Binding, Protein Denaturation, Spectrometry, Fluorescence, Spectrophotometry, Ultraviolet, Substrate Specificity, Enzyme Inhibitors analysis, Hepacivirus enzymology, Viral Nonstructural Proteins antagonists & inhibitors, Viral Nonstructural Proteins metabolism

Abstract

Several small molecules identified by high-throughput screening (HTS) were evaluated for their ability to bind to a nonstructural protein 3 (NS3) helicase from hepatitis C virus (HCV). Equilibrium dissociation constants (K(d)'s) of the compounds for this helicase were determined using several techniques including an assay measuring the kinetics of isothermal enzyme denaturation at several concentrations of the test molecule. Effects of two nonhydrolyzable ATP analogs on helicase denaturation were measured as controls using the isothermal denaturation (ITD) assay. Two compounds, 4-(2,4-dimethylphenyl)-2,7,8-trimethyl-4,5-quinolinediamine and 2-phenyl-N-(5-piperazin-1-ylpentyl)quinazolin-4-amine, were identified from screening that inhibited the enzyme and had low micromolar dissociation constants for NS3 helicase in the ITD assay. Low micromolar affinity of the quinolinediamine to helicase was also confirmed by nuclear magnetic resonance experiments. Unfortunately, isothermal titration calorimetry (ITC) experiments indicated that a more water-soluble analog bound to the 47/23-mer oligonucleotide helicase substrate with low micromolar affinity as did the substituted quinazolinamine. There was no further interest in these templates as helicase inhibitors due to the nonspecific binding to enzyme and substrate. A combination of physical methods was required to discern the mode of action of compounds identified by HTS and remove undesirable lead templates from further consideration.

Published

2002

18. 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

19. The essential role of a free sulfhydryl group in blocking the cholesteryl site of cholesteryl ester transfer protein (CETP).

Author

Epps DE and Vosters AF

Subjects

Amino Acid Sequence, Anilino Naphthalenesulfonates, Binding Sites, Biological Transport, Active drug effects, Carrier Proteins antagonists & inhibitors, Cholesterol Ester Transfer Proteins, Cysteine chemistry, Ethylmaleimide pharmacology, In Vitro Techniques, Kinetics, Molecular Sequence Data, Peptide Fragments chemistry, Peptide Fragments metabolism, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Spectrometry, Fluorescence, Sulfhydryl Compounds chemistry, 2-Naphthylamine analogs & derivatives, Carrier Proteins chemistry, Carrier Proteins metabolism, Cholesterol Esters metabolism, Glycoproteins

Abstract

Cholesteryl ester transfer protein (CETP) has at least one unpaired sulfhydryl residue, which we have shown previously to be in or near the active site region. We investigated the location of this unpaired cysteine residue(s) of CETP using chemical modification with fluorescent sulfhydryl-specific reagents, limited proteolysis, and amino acid/sequence analysis. The kinetics of labeling CETP by either 2-(4'-maleimidylanilino)-naphthalene-6-sulfonic acid (MIANS) or acrylodan were followed by observing the increase in fluorescence of the bound probes. Labeling was inhibited strongly by preincubation of the CETP with either PNU-617, a competitive inhibitor of cholesteryl ester (CE) transport, and TP2 antibody. In addition, the transfer activities of the substrate CE by the modified CETP's were also inhibited but not competitively. Finally, preincubation of the native protein with N-ethylmaleimide (NEM) resulted in inhibition of activity that was dependent upon the time of exposure of the protein to the alkylating agent. These results provide further evidence that there is a cysteine residue in the active site region of CETP and ligands that either react or bind to this residue produce steric hindrance to CE transfer activity. Finally, although not conclusive, results of the protein chemistry experiments with the modified CETP suggest that the cysteine residue at position 333 is unpaired.

Published

2002

20. A competitive fluorescence assay to measure the reactivity of compounds.

Author

Epps DE and Taylor BM

Subjects

Binding, Competitive, Coumarins chemistry, Coumarins metabolism, Fluoresceins chemistry, Fluorescence, Fluorescent Dyes chemistry, Glutathione chemistry, Kinetics, Sulfhydryl Compounds chemistry, Fluoresceins metabolism, Fluorescent Dyes metabolism, Glutathione metabolism, Sulfhydryl Compounds metabolism

Abstract

A sensitive competitive method was developed for assessing the reactivity of compounds toward glutathione and toward thiols in general. The method employs the reaction of the fluorogenic reagent fluorescein-5-maleimide (FM) with glutathione (GSH) to generate a large increase in fluorescence emission. When the reaction is measured in the presence of a compound that competes with FM toward GSH, the rate constant for fluorescent product formation increases while the total amount of product formed at the end of the reaction decreases. These changes in the presence of a series of competitor concentrations allow one to calculate the rate constant of the reaction of the competitor with GSH. At 23 degrees C, pH 7.40 in PBS buffer the second-order rate constant of the FM-GSH reaction is k2 = (1.67 +/- 0.32) x 10(4) M(-1) x s(-1). Two GSH-reactive compounds were evaluated: the second-order rate constant for the reaction of PNU-27707 with GSH under our experimental conditions is k(i) = 5660 +/- 266 M(-1) x s(-1), while that of PNU-37802 is k(i) = 21,200 +/- 1600 M(-1) x s(-1). The method is easily adaptable to a high-throughput screening format., (Copyright 2001 Academic Press.)

Published

2001

21. The ligand affinity of proteins measured by isothermal denaturation kinetics.

Author

Epps DE, Sarver RW, Rogers JM, Herberg JT, and Tomich PK

Subjects

Circular Dichroism, Kinetics, Ligands, Protein Denaturation physiology, Spectrometry, Fluorescence methods, Temperature, Time Factors, Matrix Metalloproteinase 3 analysis, Nucleoside-Phosphate Kinase analysis

Abstract

An isothermal denaturation kinetic method was developed for identifying potential ligands of proteins and measuring their affinity. The method is suitable for finding ligands specific toward proteins of unknown function and for large-scale drug screening. It consists of analyzing the kinetics of isothermal denaturation of the protein-with and without the presence of potential specific ligands-as measured by long-wavelength fluorescent dyes whose quantum yield increases when bound to hydrophobic regions exposed upon unfolding of the proteins. The experimental procedure was developed using thymidylate kinase and stromelysin as target proteins. The kinetics of thermal unfolding of both of these enzymes were consistent with a pathway of two consecutive first-order rate-limiting steps. Reflecting the stabilizing effect of protein/ligand complexes, the presence of specific ligands decreased the value of the rate constants of both steps in a dose-dependent manner. The dependence of the rate constants on ligand concentration obeyed a simple binding isotherm, the analysis of which yielded an accurate equilibrium constant for ligand binding. The method was validated by comparing its results with those obtained under the same conditions by steady-state fluorescence spectroscopy, circular dichroism, and uv spectrophotometry: The corresponding rate constants were comparable for each of the analytical detection methods.

Published

2001

22. A fluorescence resonance energy transfer method for measuring the binding of inhibitors to stromelysin.

Author

Epps DE, Mitchell MA, Petzold GL, VanDrie JH, and Poorman RA

Subjects

Catalytic Domain, Kinetics, Matrix Metalloproteinase 3 chemistry, Protein Binding, Spectrometry, Fluorescence, Enzyme Inhibitors metabolism, Matrix Metalloproteinase 3 metabolism

Abstract

A sensitive fluorescence resonance energy transfer method was developed for the direct measurement of the dissociation constants of stromelysin inhibitors. The method is applied to the thiadiazole class of stromelysin inhibitors and it takes advantage of the fact that, upon binding to the active site of enzyme, the thiadiazole ring, with its absorbance centered at 320 nm, is able to quench the fluorescence of the tryptophan residues surrounding the catalytic site. The changes in fluorescence are proportional to the occupancy of the active site: Analysis of the fluorescence versus inhibitor concentration data yields dissociation constants that are in agreement with the corresponding competitive inhibitory constants measured by a catalytic rate assay. The affinity of nonthiadiazole inhibitors of stromelysin-such as hydroxamic acids and others-can be determined from the concentration-dependent displacement of a thiadiazole of known affinity. Using this displacement method, we determined the affinities of a number of structurally diverse inhibitors toward stromelysin. Since the three tryptophan residues located in the vicinity of the active site of stromelysin are conserved in gelatinase and collagenase, the method should also be applicable to inhibitors of other matrix metalloproteinases., (Copyright 1999 Academic Press.)

Published

1999

23. Determination of the affinity of drugs toward serum albumin by measurement of the quenching of the intrinsic tryptophan fluorescence of the protein.

Author

Epps DE, Raub TJ, Caiolfa V, Chiari A, and Zamai M

Subjects

Binding Sites, Fluorescence, Humans, In Vitro Techniques, Ligands, Statistics as Topic, Serum Albumin metabolism, Spectrometry, Fluorescence methods, Tryptophan chemistry

Abstract

Binding of new chemical entities to serum proteins is an issue confronting pharmaceutical companies during development of potential therapeutic agents. Most drugs bind to the most abundant plasma protein, human serum albumin (HSA), at two major binding sites. Excepting fluorescence spectroscopy, existing methods for assaying drug binding to serum albumin are insensitive to higher-affinity compounds and can be labour-intensive, time-consuming, and usually require compound-specific assays. This led us to examine alternative ways to measure drug-albumin interaction. One method described here uses fluorescence quenching of the single tryptophan (Trp) residue in HSA excited at 295 nm to measure drug-binding affinity. Unfortunately, many compounds absorb, fluoresce, or both, in this UV wavelength region of the spectrum. Several types of binding phenomenon and spectral interference were identified by use of six structurally unrelated compounds and the equations necessary to make corrections mathematically were derived and applied to calculate binding constants accurately. The general cases were: direct quenching of Trp fluorescence by optically transparent ligands with low or high affinities; binding of optically transparent, non-fluorescent ligands to two specific sites where both sites or only one site result in Trp fluorescence quenching; and chromophores whose absorption either overlaps the Trp emission and quenches by energy transfer or absorbs light at the Trp fluorescence excitation wavelength producing absorptive screening as well as fluorescence quenching. Unless identification of the site specificity of drug binding to serum albumin is desired, quenching of the Trp fluorescence of albumin by titration with ligand is a rapid and facile method for determining the binding affinities of drugs for serum albumin.

Published

1999

24. Neutrophil precursor generation: effects of culture conditions.

Author

Martinson JA, Unverzagt K, Schaeffer A, Smith SL, Loudovaris M, Schneidkraut MJ, Bender JG, and Van Epps DE

Subjects

Antigens, CD34, Cell Differentiation drug effects, Culture Media, Cytokines pharmacology, Granulocyte Colony-Stimulating Factor pharmacology, Humans, Lewis X Antigen, Recombinant Proteins pharmacology, Cell Culture Techniques methods, Hematopoietic Stem Cells cytology, Neutrophils cytology

Abstract

The influence of feeding schedules on the expansion and differentiation of enriched PB CD34+ cells (84.9+/-14.7% purity) was studied after 12-13 days of serum-free liquid culture. CD34+ cell cultures were initiated (n=6) on day 0 (2 x 10(5) cells) in X-VIVO 10 medium containing 1% human albumin (HA) and 100 ng/ml each of rIL-3, rIL-6, rSCF, and rG-CSF. The cultures were supplemented on days 3, 6, and 9 as follows: condition 1, unfed (static culture); condition 2, 100 ng/ml rG-CSF; condition 3, split 1:2 medium + 100 ng/ml each rIL-3, rIL-6, rSCF, and rG-CSF; condition 4, split 1:2 medium + 100 ng/ml rG-CSF. The proliferative capacities (fold increase) of condition 2 (49.1+/-21.3), condition 3 (75.6+/-33.4), and condition 4 (63.1+/-23.8) cultures were significantly higher (p < 0.05) than that of the condition 1 unfed (35.5+/-14.0) cultures. Flow cytometric analysis (CD15-FITC/CD11b-PE) showed that the highest CD15+ cell purity (neutrophil precursors) was found in the condition 3 (1.18 x 10(7)+/-4.29 x 10(6)) cultures, followed by condition 4 (9.84 x 10(6)+/-3.57 x 10(6)), condition 2 (7.54 x 10(6)+/-2.06 x 10(6)), and condition 1 (4.78 x 10(6)+/-9.80 x 10(5)), respectively. The average cloning efficiency of the day 0 enriched CD34+ cells, 15.1%+/-10.3%, decreased to less than 0.2% in all of the day 12-13 cultures. These data suggest that feeding CD34+ cell cultures with rG-CSF alone, medium + rG-CSF, or medium + rIL3, rIL-6, rSCF, and rG-CSF enhances CD15+ neutrophil precursor (promyelocytes, myelocytes, metamyelocytes) production in vitro.

Published

1998

25. Ex vivo generation of dendritic cells from CD34+ cells in gas-permeable containers under serum-free conditions.

Author

Kowalkowski KL, Alzona MT, Aono FM, Van Epps DE, and Vachula M

Subjects

Antigens, CD34, Blood Component Removal, Cell Culture Techniques methods, Cell Differentiation, Culture Media, Serum-Free, Humans, Cell Culture Techniques instrumentation, Dendritic Cells cytology, Hematopoietic Stem Cells cytology

Abstract

Dendritic cells (DC) are efficient and potent APCs that can be generated ex vivo. For them to be used clinically, however, a closed culture system using serum-free medium should be used. Our goal was to differentiate DC from human blood CD34+ cells in serum-free media in a new gas-permeable culture container, PL2417. Apheresis products were collected from healthy G-CSF-mobilized donors, and CD34+ cells were selected using the Isolex immunomagnetic cell selection system. Cells were cultured in the presence of GM-CSF and tumor necrosis factor-alpha (TNF-alpha) in various serum-free media and compared with serum-containing medium in 4-well plates. One of the serum-free media was then selected and used in PL2417 containers and compared with serum-containing medium in standard flasks. The cells were evaluated at days 0, 7, and 14 for the presence of DC, which were identified morphologically after Wright-Giemsa staining by cytoplasmic processes extending from the surface of the cell. The cultures were evaluated phenotypically by flow cytometry and immunohistochemistry. The stimulatory capacity was examined in MLR. Overall, results from serum-free media and PL2417 containers were comparable results obtained under the other conditions. These data indicate that culture-deriving DC from CD34+ cells in PL2417 closed system containers using serum-free media is as effective as using standard flasks and serum-supplemented media.

Published

1998

26. Large-scale production of CD4+ T cells from HIV-1-infected donors after CD3/CD28 costimulation.

Author

Levine BL, Cotte J, Small CC, Carroll RG, Riley JL, Bernstein WB, Van Epps DE, Hardwick RA, and June CH

Subjects

Animals, CD28 Antigens immunology, CD3 Complex immunology, CD4-Positive T-Lymphocytes immunology, Cells, Cultured, Centrifugation, Density Gradient, HIV Infections immunology, Humans, Immunosorbent Techniques, Mice, Adoptive Transfer methods, CD4-Positive T-Lymphocytes pathology, HIV Infections therapy, Leukapheresis methods

Abstract

We describe a procedure for large-scale enrichment, growth, and harvesting CD4+ T cells. This method may be effective for HIV-1 immunotherapy, as the mode of stimulation, with anti-CD3 plus anti-CD28 coated beads (CD3/CD28 beads) induces a potent antiviral effect. PBMC were obtained by density gradient centrifugation of an apheresis product. Monocytes/macrophages were removed by incubating PBMC with beads coated with IgG. The cells were then magnetically depleted of B cells and CD8+ cells with mouse anti-CD20 and anti-CD8 MAbs and sheep antimouse coated beads. The remaining cells were >80% CD4+ and were transferred to gas-permeable bags containing CD3/CD28 beads and cultured in a closed system. After 14 days, the cell number increased an average of 37-fold, and cells were nearly 100% CD4+. Viral load, assessed by DNA PCR for HIV-1 gag, decreased >10-fold during culture in the absence of antiretroviral agents. Removal of CD3/CD28 beads from the cell suspension was accomplished by passing cells plus beads (3-30 x 10(9) cells in 2-12 L) over a MaxSep magnetic separator using gravity-driven flow. The cells were then concentrated to 300 ml in an automated centrifuge. This process allows safe and efficient growth of large numbers of CD4+ T cells from HIV-1+ donors.

Published

1998

27. The constituent tryptophans and bisANS as fluorescent probes of the active site and of a secondary binding site of stromelysin-1 (MMP-3).

Author

Epps DE, Poorman RA, Petzold GL, Stuchly CW, Laborde AL, and Van Drie JH

Subjects

Acrylamides, Binding Sites, Catalytic Domain, Fluorescence Polarization, Hydroxamic Acids pharmacology, Matrix Metalloproteinase 3 metabolism, Matrix Metalloproteinase Inhibitors, Models, Chemical, Phenylalanine analogs & derivatives, Phenylalanine pharmacology, Protease Inhibitors pharmacology, Protein Binding, Spectrometry, Fluorescence, Sulfonamides pharmacology, Thiophenes pharmacology, Anilino Naphthalenesulfonates, Fluorescent Dyes, Matrix Metalloproteinase 3 chemistry, Pyrazines, Tryptophan

Abstract

The active site of the catalytic domain of stromelysin-1 (matrix metalloproteinase-3, MMP-3) was probed by fluorescence quenching, lifetime, and polarization of its three intrinsic tryptophans and by the environmentally sensitive fluorescent reporter molecule bisANS. Wavelength-dependent acrylamide quenching identified three distinct emitting tryptophan species, only one of which changes its emission and fluorescence lifetime upon binding of the competitive inhibitor Batimastat. Significant changes in the tryptophan fluorescence polarization occur upon binding by any of the three hydroxamate inhibitors Batimastat, CAS108383-58-0, and Celltech CT1418, all of which bind in the P2'-P3' region of the active site. In contrast, the inhibitor CGS27023A, which is thought to bind in the P1-P1' region, does not induce any change in tryptophan fluorescence polarization. The use of the fluorescent probe bisANS revealed the existence of an auxiliary binding site extrinsic to the catalytic cleft. BisANS acts as a competitive inhibitor of stromelysin with a dissociation constant of Ki=22 microM. In addition to this binding to the active site, it also binds to the auxiliary site with a dissociation constant of 3.40+/-0.17 microM. The auxiliary site is open, hydrophobic, and near the fluorescing tryptophans. The binding of bisANS to the auxiliary site is greatly enhanced by Batimastat, but not by the other competitive inhibitors tested.

Published

1998

28. 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

29. Neutrophil maturation of CD34+ cells from peripheral blood and bone marrow in serum-free culture medium with PIXY321 and granulocyte-colony stimulating factor (G-CSF).

Author

Smith SL, Bender JG, Berger C, Lee WJ, Loudovaris M, Martinson JA, Opotowsky JD, Qiao X, Schneidkraut M, Sweeney P, Unverzagt KL, Van Epps DE, Williams DE, Williams SF, and Zimmerman TM

Subjects

Adult, Antigens, CD34 blood, Bone Marrow immunology, Bone Marrow Cells, Cell Differentiation drug effects, Cell Differentiation immunology, Cells, Cultured, Cellular Senescence immunology, Colony-Forming Units Assay, Culture Media, Serum-Free, Hematopoietic Stem Cells cytology, Hematopoietic Stem Cells immunology, Humans, Neutrophils cytology, Neutrophils immunology, Recombinant Fusion Proteins pharmacology, Reference Values, Antigens, CD34 analysis, Bone Marrow drug effects, Granulocyte Colony-Stimulating Factor pharmacology, Granulocyte-Macrophage Colony-Stimulating Factor pharmacology, Hematopoietic Stem Cells drug effects, Interleukin-3 pharmacology, Neutrophils drug effects

Abstract

Bone marrow (BM) or peripheral blood (PB) CD34+ cells were cultured for 12 days in serum-free culture medium containing PIXY321 (IL-3/ GM-CSF fusion protein) with or without periodic supplements of granulocyte-colony stimulating factor (G-CSF). The cultures were evaluated at day 12 for total cell proliferation (fold increase from day 0), neutrophil differentiation by flow cytometry, using dual staining with CD15-FITC and CD11b-PE, and morphology using Wright-Giemsa and granule staining. In cultures containing PIXY321 where 6000 U/ml of G-CSF was added days 0 and 6, there was no significant difference (p > or = 0.05) in cell proliferation or the percent of CD15+/CD11b+ cells when compared with cultures with PIXY321 alone. ELISA analysis showed G-CSF levels had declined by 90% after 3 days of culture. Further studies were performed to assess the benefit of supplementing lower concentrations of G-CSF (600 U/ml) at more frequent intervals. A significant increase (p < or = 0.05) in cell proliferation and percent CD15+/CD11b+ was observed when G-CSF was added on days 0, 3, 6, and 9 (every 3 days) as compared with those cultures with PIXY321 alone. CD34+ cell proliferation without G-CSF was 19.6 +/- 4.8-fold, with G-CSF added on days 0 and 6 was 28.7 +/- 6.4-fold, and with G-CSF added on days 0, 3, 6, and 9 was 45.9 +/- 10.6-fold. Percent of CD15+/CD11b+ cells was 19.0 +/- 4.6%, 38.2 +/- 7.2%, and 58.5 +/- 6.5%, respectively, in these cultures. We observed more CD15+/CD11b+ cells, myelocytes/metamyelocytes, and secondary granule staining in cultures with G-CSF added on day, 0, 3, 6, and 9 as compared with cultures with G-CSF added on days 0 and 6 or no G-CSF added. We conclude that PIXY321 and G-CSF act synergistically on the in vitro proliferation and neutrophil differentiation of BM and PB CD34+ cells and that frequent supplements of G-CSF facilitate neutrophil differentiation.

Published

1997

30. The pretransition of dipalmitoyllecithin bilayers as probed by the fluorescent pyrrolopyrimidine, U-104067.

Author

Epps DE, Wilson CL, Vosters AF, and Kézdy FJ

Subjects

1,2-Dipalmitoylphosphatidylcholine metabolism, Acrylamide, Acrylamides pharmacology, Calorimetry, Differential Scanning, Fatty Acids metabolism, Fluorescence Polarization, Fluorescent Dyes metabolism, Hydrogen-Ion Concentration, Lipid Bilayers metabolism, Liposomes metabolism, Molecular Structure, Phosphatidylcholines metabolism, Pyrimidines metabolism, Pyrrolidines metabolism, Solubility, Solvents, Spectrometry, Fluorescence, Temperature, 1,2-Dipalmitoylphosphatidylcholine chemistry, Fluorescent Dyes chemistry, Lipid Bilayers chemistry, Pyrimidines chemistry, Pyrrolidines chemistry

Abstract

The amphiphilic pyrrolopyrimidine, U-104067, is a fluorophore ideally suited to report on the relative hydrophobicities of different microenvironments. It forms stable monomolecular layers at the air/water interface with a limiting molecular area of 51.9 +/- 0.3 A2/molecule and a collapse pressure of about 18 dyn/cm. Differential scanning calorimetry of its mixed liposomes with dipalmitoyllecithin shows full solubility of the compound in the liquid disordered phase and insolubility in the solid ordered phase. In aqueous solutions, the compound binds to phospholipid bilayers with a stoichiometry of 13.2 +/- 1.2 moles of lipid per mole of U-104067, with Kd = 0.33 +/- 0.05 microM toward egg lecithin/phosphatidylserine bilayers and Kd = 1.5 +/- 0.3 microM toward pure egg lecithin bilayers. In liquid crystalline phospholipid bilayers the compound behaves as two independently emitting species, one accessible to acrylamide and the other one not. Doxyl fatty acid methyl esters quench both species and show that the average position of the fluorophore is at a depth corresponding to that of the 7th carbon of a fatty acyl chain. Dissolved in the liquid disordered (L alpha) phase of dipalmitoyllecithin at 45 degrees C, U-104067 shows a single ionizable group, pKa = 3.19 +/- 0.03 while in the solid ordered (L beta) phase it displays two ionizable groups, pKa1 = 4.99 +/- 0.10 and pKa2 = 6.96 +/- 0.13. The most unusual property of this molecule is that it is miscible with the tilted (L beta) and liquid (L alpha) phases of dipalmitoyllecithin but totally immiscible with the rippled (P beta) phase. Because of this, U-104067 is a sensitive reporter for the tilted/rippled phase transition as monitored by its fluorescence anisotropy and its quantum yield changes.

Published

1997

31. 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

32. Ex vivo expansion of frozen/thawed CD34+ cells isolated from frozen human apheresis products.

Author

Martinson JA, Loudovaris M, Smith SL, Bender JG, Vachula M, van Epps DE, Kaizer H, Ghalie RG, and McLeod BC

Subjects

Blood Component Removal methods, Cell Differentiation drug effects, Cell Division drug effects, Cells, Cultured, Colony-Forming Units Assay, Colony-Stimulating Factors, Culture Techniques methods, Female, Flow Cytometry, Hematopoietic Cell Growth Factors pharmacology, Hematopoietic Stem Cells drug effects, Humans, Neoplasms therapy, Recombinant Proteins pharmacology, Antigens, CD analysis, Antigens, CD34 analysis, Cryopreservation, Hematopoietic Stem Cells cytology, Neoplasms blood

Abstract

Human CD34+ cells purified from frozen mobilized peripheral blood apheresis products (n = 7) were studied immediately (freshly isolated) or refrozen and studied after > 30 days storage in liquid nitrogen (refrozen/thawed). The proliferation and differentiation of freshly isolated or refrozen/thawed CD34+ cells were examined after 10 days of serum-supplemented suspension culture with recombinant human hematopoietic growth factors. The proliferative capacity (fold increase) of the refrozen/thawed CD34+ cells (mean +/- SD, 54.3 +/- 34.3) was comparable to the freshly isolated CD34+ cell cultures (49.0 +/- 42.4). Two-color flow cytometry of the CD34+ cultured cell populations, fresh and refrozen/thawed, displayed typical patterns of neutrophil differentiation into CD15/CD11b neutrophil precursors. The colony-forming ability of freshly isolated and refrozen/thawed CD34+ cells showed no significant differences (p > 0.05) in the total number or type of colony-forming units (CFU-GM, CFU-M, BFU-E, CFU-GEMM) obtained. In addition, the cloning efficiencies of freshly isolated (19.5 +/- 7.6%) and refrozen/thawed CD34+ cells (21.9 +/- 12.7%) were comparable (p = 0.366). These data suggest that CD34+ cells enriched from frozen apheresis blood products can be either used immediately or stored in liquid nitrogen and thawed with minimal effect on their ability to proliferate and differentiate in liquid culture.

Published

1997

33. Large-scale selection of CD34+ peripheral blood progenitors and expansion of neutrophil precursors for clinical applications.

Author

Zimmerman TM, Bender JG, Lee WJ, Loudovaris M, Qiao X, Schilling M, Smith SL, Unverzagt K, Van Epps DE, Blake M, Williams DF, and Williams SF

Subjects

Adult, Cell Separation, Cells, Cultured, Flow Cytometry, Granulocyte-Macrophage Colony-Stimulating Factor, Humans, Interleukin-3, Neutropenia therapy, Neutrophils immunology, Recombinant Fusion Proteins, Stem Cells immunology, Antigens, CD34 analysis, Hematopoiesis, Neutrophils cytology, Stem Cells cytology

Abstract

Hematopoietic recovery after high-dose chemotherapy is characterized by an obligate period of neutropenia of approximately 8-10 days. It is postulated that if a pool of neutrophil precursors and progenitors were expanded in vitro and reinfused, the duration of neutropenia may be substantially shortened by these cells capable of providing mature neutrophils within days of reinfusion. In this study, peripheral blood progenitor cell products were obtained from six normal donors mobilized with rhG-CSF and two patients mobilized with cyclophosphamide and rhG-CSF. CD34+ cells were isolated using the Isolex immunomagnetic bead method. A mean of 8.26 x 10(7) CD34+ cells with a mean purity of 74.5% were seeded at a concentration of 1 x 10(5)/ml into a 12 day stroma-free liquid culture using gas-permeable bags. A serum-free growth medium supplemented with PIXY321 was used. On day 7, there was a mean cellular expansion of fourfold, at which time the cells were resuspended at the initial concentration, yielding a mean culture volume of 3L (1-6 L). On day 12, there was an additional mean fold cellular expansion of 10 x, achieving an overall mean fold expansion of 41 +/- 16. Cellular characterization of the expanded cells revealed predominantly neutrophil precursors by morphology (mean 70.1%) and flow cytometric analysis. A mean of 52.3% of the expanded cells expressed CD15. Immunohistochemical staining revealed a mean of 7.1% CD41a+ megakaryocytic progenitors in the final cultured cell product. Detectable CD34+ cells were maintained only in those cultures initiated with greater than 90% CD34+ cells. Colony-forming units-granulocyte-macrophage (CFU-GM) were maintained in the 12 day culture at a level similar to the preculture number, whereas CFU mixed were depleted in all samples. On day 0, there were few CFU clusters (colonies containing fewer than 50 cells) identified, but by day 12, a mean total of 8.3 x 10(6) CFU clusters were identified. On day 12, the expanded cells were harvested and pooled using the Fenwal CS3000 Plus blood cell separator and resuspended in Plasma-Lyte-A with 1% human serum albumin. The mean harvest recovery of expanded progenitors was 91%, with a mean viability of 86%.

Published

1996

34. Infusion of ovine C5a into sheep mimics the inflammatory response of hemodialysis.

Author

Johnson RJ, Burhop KE, and Van Epps DE

Subjects

Amino Acid Sequence, Animals, Blood Pressure, Complement C5a metabolism, Fluorescein-5-isothiocyanate, Fluorescent Dyes, Humans, Kinetics, Leukocyte Count, Molecular Sequence Data, Neutropenia chemically induced, Neutrophils physiology, Respiratory Burst, Sequence Homology, Sheep, Tetradecanoylphorbol Acetate pharmacology, Complement C5a administration & dosage, Disease Models, Animal, Inflammation chemically induced, Renal Dialysis

Abstract

Previous studies in our group have explored the inflammatory response in sheep to dialysis with a variety of different hemodialysis membranes. In the present study we investigated the potential role of C5a in mediating inflammatory responses that have been attributed to complement activation in the extracorporeal setting. Sheep C5a was infused into sheep in a manner that simulated exposure to this anaphylatoxin during dialysis. C5a infusion into sheep was shown to produce a dose-dependent neutropenia that was quantitatively and temporally identical to the response of sheep undergoing dialysis with complement-activating membranes. The two lowest doses used (0.25 and 0.50 micrograms/kg), which resulted in concentrations below the detectable limits of current assays (10 ng/ml), produced significant neutropenia (21.8% and 78.1%, respectively). The ability of the neutrophils (PMNs) to bind fluorescein isothiocyanate-C5a or initiate a respiratory burst in response to phorbol myristate acetate were also affected in a dose-dependent manner. In contrast, C5a alone was not able to produce significant release of lactoferrin, a specific granule constituent, suggesting that degranulation of PMN-specific and primary granules requires secondary stimuli. The production of thromboxane A2 and thromboxane's consequent cardiopulmonary effect of increasing mean pulmonary artery pressure were both observed in a dose-dependent fashion. However, larger amounts of C5a were required to elicit these latter responses as compared with the PMN activities. These results suggest that C5a may be a primary mediator of complement-dependent events that occur during extracorporeal therapies such as hemodialysis, and they also suggest that very little complement activation is necessary to activate leukocytes, whereas higher thresholds are required to produce cardiopulmonary responses.

Published

1996

35. Immunocytochemistry and flow cytometry evaluation of human megakaryocytes in fresh samples and cultures of CD34+ cells.

Author

Qiao X, Loudovaris M, Unverzagt K, Walker DE, Smith SL, Martinson J, Schilling M, Lee W, Williams SF, Van Epps DE, Cohen I, and Bender JG

Subjects

Adult, Blood Component Removal, Bone Marrow Cells, Cells, Cultured, Evaluation Studies as Topic, Humans, Leukocytes, Mononuclear cytology, Leukocytes, Mononuclear immunology, Antigens, CD34 immunology, Flow Cytometry methods, Immunoenzyme Techniques, Megakaryocytes immunology

Abstract

Adhering platelets on the cell surface can give misleading results when doing flow cytometry analysis of platelet/megakaryocyte-specific glycoprotein (GP) antigens to enumerate megakaryocytes (MK) in mobilized peripheral blood (PB), apheresis products, or normal bone marrow (BM). For adequate quantification and characterization of human MK, we examined samples with parallel flow cytometry and immunocytochemistry. MK expression of GP IIb/IIIa (CD41a), GP Ib (CD42b), GP IIIa (CD61), CD45, CD33, and CD11b, and their light scatter properties were evaluated. Fresh samples of low density mononuclear cells (MNC) or purified CD34+ cells contained 10-45% of platelet-coated cells. Platelet-coated cells decreased dramatically after several days of incubation in a serum-free medium supplemented with stem cell factor, IL-3, IL-6, and/or GM-CSF. Between d 9-12, flow cytometry detected a distinct CD41a+ MK population, 8.3 +/- 1.3% in BM CD34 cell cultures (n = 7) and 13.1 +/- 2.1% in PB CD34 cell cultures (n = 14), comparable to immunocytochemistry data (7.8 +/- 1.9% and 16.4 +/- 2.6%, respectively). CD41a stained a higher proportion of MK than CD42b or CD61, while CD42b+ or CD61+ cells contained more morphologically mature MK than CD41a+ cells in cultures containing aplastic serum. When fluorescence emission of CD41a was plotted against forward-light scatter (FSC), subpopulations of small and large MK were observed. Such subpopulations overlapped in CD41a intensity and side-light scatter (SSC) property. Most MK co-expressed CD45 (98.8% positive) but not CD33 (80.7% negative) or CD11b (88.9% negative). Our data indicate that flow cytometry can be used effectively to identify MK. However, caution should be taken with samples containing adherent platelets.

Published

1996

36. Kinetics and inhibition of lipid exchange catalyzed by plasma cholesteryl ester transfer protein (lipid transfer protein).

Author

Epps DE, Greenlee KA, Harris JS, Thomas EW, Castle CK, Fisher JF, Hozak RR, Marschke CK, Melchior GW, and Kézdy FJ

Subjects

Animals, Carrier Proteins blood, Catalysis, Cholesterol pharmacology, Cholesterol Ester Transfer Proteins, Humans, Kinetics, Lipoproteins, HDL metabolism, Macaca fascicularis, Phosphatidylcholine-Sterol O-Acyltransferase antagonists & inhibitors, Carrier Proteins antagonists & inhibitors, Cholesterol analogs & derivatives, Glycoproteins, Lipid Metabolism

Abstract

The cholesteryl ester transfer protein-catalyzed cholesteryl ester transfer is inhibited by two compounds identified by a large-scale screening of cholesterol backbone-containing molecules. Kinetic analysis shows that U-95,594, an amino steroid, inhibits competitively the cholesteryl ester transfer protein-catalyzed transfer of both cholesteryl esters and triglycerides, as well from high-density lipoproteins as from synthetic microemulsions. In contrast, U-617, an organomercurial derivative of cholesterol, inhibits competitively the transfer of cholesteryl ester from either donor but is without any effect on triglyceride transfer. In addition to the rapid, competitive inhibition of cholesteryl ester transfer, U-617 also slowly and reversibly reacts with cholesteryl ester transfer protein to produce an additional 10-fold decrease in cholesteryl ester transfer activity but, again, without effect on triglyceride transfer.

Published

1995

37. Method for measuring the activities of cholesteryl ester transfer protein (lipid transfer protein).

Author

Epps DE, Harris JS, Greenlee KA, Fisher JF, Marschke CK, Castle CK, Ulrich RG, Moll TS, Melchior GW, and Kézdy FJ

Subjects

Boron Compounds, Cholesterol Ester Transfer Proteins, Emulsions, Fluorescence, Fluorescent Dyes, Humans, Kinetics, Sensitivity and Specificity, Carrier Proteins analysis, Cholesterol Esters, Glycoproteins, Spectrometry, Fluorescence

Abstract

A continuous recording fluorescence assay was developed for cholesteryl ester transfer protein (CETP). The assay measures the increase in fluorescence accompanying the relocation of fluorescent lipids, cholesteryl esters and triglycerides, from a donor emulsion to an acceptor emulsion. In the absence of CETP, the quantum yields of the fluorescent lipids is low because their high concentrations in the donor emulsions result in self-quenching. CETP catalyzes the redistribution of the fluorescent lipids from the donor to the acceptor emulsions and fluorescence increases substantially. Efficient sonication and incorporation of apolipoproteins from human HDL into the emulsions significantly increased the transfer rates. Under optimal conditions, the redistribution of fluorescent compounds reaches equilibrium within < 30 min and the kinetics of this process are consistent with a simple, first-order reaction pathway. The redistribution kinetics support a mechanism of adsorption --> exchange --> desorption --> diffusion.

Published

1995

38. A general, wide-rage spectrofluorometric method for measuring the site-specific affinities of drugs toward human serum albumin.

Author

Epps DE, Raub TJ, and Kézdy FJ

Subjects

Binding Sites, Binding, Competitive, Dansyl Compounds chemistry, Fluorescent Dyes, HIV Protease Inhibitors chemistry, Humans, Least-Squares Analysis, Warfarin chemistry, Dansyl Compounds pharmacokinetics, HIV Protease Inhibitors pharmacokinetics, Serum Albumin chemistry, Spectrometry, Fluorescence methods, Warfarin pharmacokinetics

Abstract

Binding of drugs to serum albumin is one of the most important pharmacokinetic determinants and the design of drugs should take advantage of this property. In the present work, the fluorescent ligands Warfarin and dansylsulfonamide were used as probes of IIA site of human albumin and dansylsarcosine as the probe of the IIIA site. From the changes in fluorescence upon binding at 37 degrees C, pH 7.4, the following dissociation constants were determined: Warfarin, 3.43 +/- 0.69 microM; dansylsulfonamide, 7.57 +/- 0.88 microM; and dansylsarcosine, 6.06 +/- 1.09 microM. Nonfluorescent ligands displace these probes competitively and the type of probe displaced identifies the site specificity of the ligands. Nonlinear least-squares analysis of the decrease in fluorescence accompanying the displacement yields the stoichiometry and the dissociation constant may also be estimated rapidly from displacement at a single competitor concentration. The method yields reliable Kd values for at least the range of 0.2 to 100 microM. Representative dissociation constants for the IIA site-specific ligands are as follows: phenylbutazone, 1.9 +/- 0.3 microM; U-99,499, 1.8 +/- 0.2 microM; U-96,988, 5.3 +/- 1.5 microM; and U-105,665, 42 +/- 7 microM. For the IIIA site we find the following Kd values: oxazepam, 27.7 +/- 2.1 microM; diazepam, 7.7 +/- 1.0 microM; and ibuprofen, 2.7 +/- 1.2 microM. The method is eminently suitable for large-scale screening.

Published

1995

39. Evidence for transbilayer, tail-to-tail cholesterol dimers in dipalmitoylglycerophosphocholine liposomes.

Author

Harris JS, Epps DE, Davio SR, and Kézdy FJ

Subjects

Calorimetry, Differential Scanning, Thermodynamics, 1,2-Dipalmitoylphosphatidylcholine chemistry, Cholesterol chemistry, Liposomes

Abstract

The behavior of multilamellar liposomes of 2,3-dipalmitoyl-sn-glycero-1-phosphocholine (DPPC) was studied by differential scanning calorimetry (DSC) in the presence of < or = 5 mol % of the amphiphilic solutes methyl oleate, cholesterol, pregnenolone, and dehydroandrosterone. The DSC thermograms indicate that the solutes are miscible only with the liquid-disordered (Id) phase, and not with the solid-ordered (so) phase. The slopes of the Tm vs solute concentration curves confirm this conclusion: It appears that the so-1d phase transition of DPPC, which corresponds to the melting of the phospholipid chains, can be treated as a simple melting process and, thus, could be used as a cryoscopic system. In that case, its melting point depression constant, Kf, can be calculated a priori from the experimentally measured heat of fusion per gram of DPPC, lf, and the temperature of the phase transition of pure DPPC, T(o), by the equation Kf = RTo2/(1000lf) = 12.3 +/- 0.9 K g M-1 cm3. With methyl oleate as the solute, the Tm vs methyl oleate concentration plot is linear, and from the slope we calculate Kf = 12.9 +/- 0.8 K g M-1 cm3. Thus, methyl oleate appears to form an ideal cryoscopic system with dipalmitoyllecithin liposomes: It is fully miscible with the 1d phase but is apparently insoluble in the s(o) phase. Pregnenolone and dehydroandrosterone also form ideal cryoscopic systems with dipalmitoyllecithin liposomes: The Tm vs solute concentration plots are linear and yield the correct MWs for these solutes.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1995

40. Tirilazad mesylate protects stored erythrocytes against osmotic fragility.

Author

Epps DE, Knechtel TJ, Bacznskyj O, Decker D, Guido DM, Buxser SE, Mathews WR, Buffenbarger SL, Lutzke BS, and McCall JM

Subjects

Dinoprost metabolism, Erythrocyte Membrane drug effects, Hemolysis drug effects, Humans, In Vitro Techniques, Time Factors, Vitamin E blood, Antioxidants, Blood Preservation methods, Osmotic Fragility drug effects, Pregnatrienes pharmacology

Abstract

The hypoosmotic lysis curve of freshly collected human erythrocytes is consistent with a single Gaussian error function with a mean of 46.5 +/- 0.25 mM NaCl and a standard deviation of 5.0 +/- 0.4 mM NaCl. After extended storage of RBCs under standard blood bank conditions the lysis curve conforms to the sum of two error functions instead of a possible shift in the mean and a broadening of a single error function. Thus, two distinct sub-populations with different fragilities are present instead of a single, broadly distributed population. One population is identical to the freshly collected erythrocytes, whereas the other population consists of osmotically fragile cells. The rate of generation of the new, osmotically fragile, population of cells was used to probe the hypothesis that lipid peroxidation is responsible for the induction of membrane fragility. If it is so, then the antioxidant, tirilazad mesylate (U-74,006f), should protect against this degradation of stored erythrocytes. We found that tirilazad mesylate, at 17 microM (1.5 mol% with respect to membrane lecithin), retards significantly the formation of the osmotically fragile RBCs. Concomitantly, the concentration of free hemoglobin which accumulates during storage is markedly reduced by the drug. Since the presence of the drug also decreases the amount of F2-isoprostanes formed during the storage period, an antioxidant mechanism must be operative. These results demonstrate that tirilazad mesylate significantly decreases the number of fragile erythrocytes formed during storage in the blood bank.

Published

1994

41. Kinetic evaluation of lipophilic inhibitors of lipid peroxidation in DLPC liposomes.

Author

Horan KL, Lutzke BS, Cazers AR, McCall JM, and Epps DE

Subjects

Amidines chemistry, Azo Compounds chemistry, Chromans chemistry, Chromatography, High Pressure Liquid, Free Radical Scavengers, Free Radicals, Kinetics, Linoleic Acid, Mass Spectrometry, Nitriles chemistry, Piperazines chemistry, Pregnatrienes chemistry, Antioxidants chemistry, Linoleic Acids chemistry, Lipid Peroxidation, Liposomes chemistry, Phosphatidylcholines chemistry

Abstract

The authors have developed a kinetic method that allows one to obtain relative reactivity constants for lipophilic antioxidants in free radical systems. Two experimental model systems were developed: (a) a methanolic solution using AMVN as the free radical initiator and linoleic acid as the substrate, and (b) a multilamellar vesicle system composed of dilinoleoylphosphatidylcholine and AAPH as the substrate and the initiator, respectively. The use of these two systems allows researchers not only to determine the intrinsic reactivity of a potential antioxidant, but also to evaluate its potency in a membranous system where the contribution of the physical properties of the antioxidant to the inhibition of lipid peroxidation is important. These results show that all antioxidants tested acted in these systems as free radical scavengers, and they validate the synergism between intrinsic scavenging ability and membrane affinity and/or membrane-modifying physical properties in the inhibition of lipid peroxidation.

Published

1994

42. Des-Lys58-beta 2m and native beta 2m in rheumatoid arthritis serum and synovial fluid.

Author

Williams RC Jr, Malone CC, Nissen MH, Aono FM, Vachula M, and Van Epps DE

Subjects

Amino Acid Sequence, Animals, Antibody Formation, Arthritis, Rheumatoid immunology, Chemotaxis, Leukocyte immunology, Humans, Lupus Erythematosus, Systemic blood, Mice, Molecular Sequence Data, Neutrophils immunology, Rabbits, Spondylitis, Ankylosing blood, Synovial Fluid chemistry, Synovial Fluid immunology, Arthritis, Rheumatoid blood, Receptors, Immunologic analysis, beta 2-Microglobulin analysis

Abstract

Objective: Levels of beta 2-microglobulin and modified beta 2-microglobulin (Des-Lys58-beta 2m) were measured in serum and synovial fluids from patients with rheumatoid arthritis (RA) and other inflammatory joint disorders using rabbit antisera prepared against the beta 2m peptide VEHSDLSFS encompassing residues 49-57 and absorbed with the C-terminal beta 2m peptide (87-97) LSQPKIVKWDR: These antisera which did not react with native beta 2m were employed to quantitate Des-Lys58-beta 2m in serum and SF. Native beta 2m was measured using a direct ELISA method., Results: Removal of serum rheumatoid factor by adsorption to monomeric IgG columns did not change serum levels of beta 2m or Des-Lys58-beta 2m. Native beta 2m was found in all of 20 RA sera, but only rarely in SLE sera. No serum beta 2m was found in 20 patients with ankylosing spondylitis or 25 normal controls. Significant elevations of Des-Lys58-beta 2m were found in 80% of 21 SF from RA patients and in 43% of 41 SF from other subjects with various forms of inflammatory arthritis. In RA and other disorders such as gout or pseudogout, levels of Des-Lys58-beta 2m were higher in synovial fluid than in serum during an acute episode of synovitis. Both native beta 2m and Des-Lys58-beta 2m showed minimal neutrophil and T cell chemotactic activity., Conclusion: Des-Lys58-beta 2m present in many inflammatory SF may contribute to the inflammatory reaction in many forms of connective tissue disease by its known amplification of T cell cytotoxicity.

Published

1994

43. Characterization of the steady-state and dynamic fluorescence properties of the potential-sensitive dye bis-(1,3-dibutylbarbituric acid)trimethine oxonol (Dibac4(3)) in model systems and cells.

Author

Epps DE, Wolfe ML, and Groppi V

Subjects

Animals, Cattle, Cell Line, Chemical Phenomena, Chemistry, Physical, Kinetics, Lipid Bilayers chemistry, Membrane Potentials, Models, Chemical, Muscle, Smooth metabolism, Potassium Channels metabolism, Rats, Serum Albumin, Bovine chemistry, Spectrometry, Fluorescence, Barbiturates chemistry, Fluorescent Dyes chemistry, Isoxazoles chemistry

Abstract

The steady-state and dynamic fluorescence properties of the membrane potential-sensitive bis-oxonol dye Dibac4(3) were characterized in vitro using model ligand systems and in vivo in A10 smooth muscle cells by fluorescence microscopy in conjunction with the ACAS imaging system. In the latter system the dye responds to potassium ion-induced jumps in membrane potential with changes in its fluorescence intensity, which follow pseudo-first-order kinetics. The relationship between the magnitude of the changes and the corresponding rate constants excludes the possibility that a simple, one-step equilibrium between extracellular and cytoplasmic dye would be sufficient to account for this phenomenon. The necessity of invoking an additional step suggested that the redistribution of the free dye between the cytoplasm and the exocellular medium is rapid and that the slow step associated with the fluorescence changes may be the interaction of the dye with proteins in the cytoplasm, along the lines proposed by Bräuner et al. (Biochim. Biophys. Acta 771 (1984), 208, 216). The interaction of the dye with BSA and with egg lecithin SUVs was studied as a model for the in vivo phenomenon. The dependence of fluorescence intensity changes on the concentrations of the reagents shows the formation of a reversible dye/albumin complex with a 2/1-stoichiometry, with Kd = 0.03 +/- 0.01 microM and a reversible adsorption to the SUVs with Kd 0.45 +/- 0.08 microM. The fluorescence lifetime of the dye in solution, < 100 ps, results in a high solution steady-state anisotropy. The latter decreases considerably upon binding to BSA, SUVs and A10 cells concomitant with a large increase in the lifetime. With such a short lifetime of the free dye, selective gating of the excitation source or the photodetector should eliminate the high background of the unbound dye and thereby enhance the sensitivity of the system.

Published

1994

44. Harvesting, characterization, and culture of CD34+ cells from human bone marrow, peripheral blood, and cord blood.

Author

Van Epps DE, Bender J, Lee W, Schilling M, Smith A, Smith S, Unverzagt K, Law P, and Burgess J

Subjects

Adult, Antibodies, Monoclonal immunology, Antigens, CD analysis, Antigens, CD34, Cell Differentiation drug effects, Cells, Cultured, Colony-Forming Units Assay, Culture Techniques methods, Cyclophosphamide pharmacology, Etoposide pharmacology, Flow Cytometry, Granulocyte Colony-Stimulating Factor pharmacology, Hematopoiesis drug effects, Hematopoietic Cell Growth Factors pharmacology, Humans, Immunomagnetic Separation, Infant, Newborn, Neoplasms blood, Neoplasms therapy, Antigens, CD immunology, Blood Cells, Bone Marrow Cells, Cell Separation methods, Fetal Blood cytology, Hematopoietic Stem Cells drug effects, Hematopoietic Stem Cells immunology

Abstract

Stem and progenitor cells from a variety of sources including bone marrow, cord blood, and peripheral blood have been used for transplantation. This study compares CD34 cells from all three sources. Flow cytometry analysis of CD34 cells in multiple samples of normal peripheral blood and patient peripheral blood mobilized with chemotherapy (cyclophosphamide/VP16), chemotherapy plus granulocyte colony stimulating factor (G-CSF), and G-CSF alone were compared to bone marrow and cord blood. Although the relative distribution of CD34 percentages in each preparation of cells varied widely, on average the percentage of CD34 cells in these different preparations was 0.15%, 0.6%, 2%, 0.45%, 1.68%, and 0.83% respectively. CD34 subset analysis was performed on these cell preparations using multicolor flow cytometry and antibodies to CD33, CD13, CD45RA, CD19, CD71, and CD38. The major differences observed were that bone marrow CD34 cells contain high percentages of CD19+ cells not found in significant quantity in the other cell preparations and cord blood CD34 cells contained a higher percentage of CD38-cells than the other cell preparations. A magnetic bead system was used with anti-CD34 antibody to purify CD34 cells from mobilized peripheral blood apheresis products, cord blood, and bone marrow. Efficient selection with high purities of CD34 cells was achieved with each of the cell preparations. Comparison of colony-forming activity of each of the cell preparations showed cord blood and mobilized peripheral blood to have slightly higher cloning efficiencies than bone marrow with higher numbers of erythroid blast-forming units (BFU-E) also observed in cord blood CD34 cells. Culture of isolated CD34 cells in liquid culture with interleukin-3, stem cell factor, G-CSF, and granulocyte-macrophage GM-CSF showed over a 100-fold expansion in cell numbers after 25 days, with the peak expansion of colony-forming cells occurring between days 11 and 16. Analysis of day-10 cells from these cultures showed them to be predominantly promyelocytes, myelocytes, and metamyelocytes, with cord blood CD34 cultures showing more promyelocytes than peripheral blood or bone marrow and bone marrow showing more metamyelocytes. Comparison of the proliferation of CD34 cells from these different cell preparations showed that cord blood CD34 cells cultured for 10 days averaged an 85-fold increase in cell numbers followed by mobilized peripheral blood CD34 cells, with an average 56-fold increase, and bone marrow CD34 cells, with an average 49-fold increase.

Published

1994

45. Phenotypic analysis and characterization of CD34+ cells from normal human bone marrow, cord blood, peripheral blood, and mobilized peripheral blood from patients undergoing autologous stem cell transplantation.

Author

Bender JG, Unverzagt K, Walker DE, Lee W, Smith S, Williams S, and Van Epps DE

Subjects

Adult, Antigens, CD19, Antigens, CD34, Antigens, Differentiation, B-Lymphocyte analysis, Antigens, Differentiation, Myelomonocytic analysis, Bone Marrow immunology, Bone Marrow Cells, CD13 Antigens, Fetal Blood immunology, Humans, Leukocyte Common Antigens analysis, Neprilysin analysis, Phenotype, Receptors, Transferrin, Sialic Acid Binding Ig-like Lectin 3, Transplantation, Autologous, Antigens, CD analysis, Bone Marrow Transplantation, Hematopoietic Stem Cell Transplantation, Leukocytes, Mononuclear immunology

Abstract

Single- and multicolor flow cytometry were used to define progenitor subsets in normal human bone marrow and peripheral blood, cord blood, and blood following mobilization of CD34+ progenitor cells by cyclophosphamide or cyclophosphamide/etoposide/G-CSF treatment. CD34 cells were quantitated and subsets of CD34+ cells were defined by coexpression of CD33, CD13, CD10, CD19, CD45RA, and CD71. Myeloid and erythroid progenitors were quantitated by sorting single CD34+ cells into individual wells of 96-well plates containing methylcellulose, IL-3, GM-CSF, G-CSF, IL-6, and erythropoietin. Comparative studies of CD34 cells showed that the percentage of CD34+ mononuclear cells was greatest in blood samples from patients following mobilization treatment with cyclophosphamide/etoposide/G-CSF averaging 2%. By comparison, the remaining sample groups ranged from 1.68 to 0.15% CD34 cells in this order, bone marrow > cord blood > cyclophosphamide mobilized blood > peripheral blood. Comparison of CD34 cells per milliliter of bone marrow or blood showed a range of 22.4 x 10(4) to 0.65 x 10(4)/ml in the following order, bone marrow > chemotherapy/etoposide/G-CSF > cord blood > cyclophosphamide-mobilized blood. Comparative analysis of CD34 subsets from different sources showed significant differences, particularly bone marrow and blood samples. A distinct population of CD34+ CD19+ (Leu 12) CD10+ (CALLA) pre-B lymphocyte cells was defined in bone marrow with lower side and forward light scatter characteristics and was variable between donors (29.8 +/- 16.9%, mean +/- 1 SD; range, 3-54%; n = 8). This population was not found to a significant degree in blood and also expressed CD45RA (Leu 18). Coexpression studies of CD45RA and CD71 (transferrin receptor) expression on CD34+ cells defined a CD45RA- CD71+ population containing 89 +/- 6.3% (n = 4) BFU-E and a CD45RA+ CD71+ population that contained all CFU-GM (n = 4). LeuM7 (CD13) stained a larger percentage to a greater intensity than MY7 (CD13). Coexpression of CD45RA (Leu 18) and CD13 (LeuM7) defined a subset of CD13+ CD45RA+ cells enriched for CFU-GM and CFU-M with a cloning efficiency of 31%. Coexpression of CD33 (MY9) and CD13 (MY7) defined a population that was predominantly CFU-GM with a cloning efficiency of 38%. These studies define CD34+ phenotypes containing pure populations of B lymphocyte, granulocyte-macrophage, or erythroid progenitors and demonstrate the utility of multiparameter flow cytometry to define lineage-committed CD34+ cells.

Published

1994

46. Expansion of neutrophil precursors and progenitors in suspension cultures of CD34+ cells enriched from human bone marrow.

Author

Smith SL, Bender JG, Maples PB, Unverzagt K, Schilling M, Lum L, Williams S, and Van Epps DE

Subjects

Antigens, CD34, Antigens, Differentiation, Myelomonocytic analysis, Bone Marrow immunology, CD11 Antigens, Cell Adhesion, Cell Differentiation, Cell Division, Cells, Cultured, Flow Cytometry, Granulocyte Colony-Stimulating Factor pharmacology, Granulocyte-Macrophage Colony-Stimulating Factor pharmacology, Hematopoietic Cell Growth Factors pharmacology, Hematopoietic Stem Cells immunology, Humans, Immunophenotyping, Interleukin-3 pharmacology, Lewis X Antigen, Neutrophils immunology, Stem Cell Factor, Antigens, CD analysis, Bone Marrow Cells, Hematopoietic Stem Cells cytology, Neutrophils cytology

Abstract

The growth and differentiation of selected bone marrow CD34+ cells stimulated with hematopoietic growth factors in lipid cultures were evaluated to determine whether cell types that may be useful for reducing the neutropenia associated with high-dose chemotherapy (HDC) can be produced and quantitated in vitro. CD34+ cells enriched from bone marrow were cultured for up to 5 weeks in interleukin-3 (IL-3), granulocyte-macrophage colony-stimulating factor (GM-CSF) and granulocyte colony-stimulating factor (G-CSF) with or without stem cell factor (SCF) (also termed c-kit ligand). The mixture of IL-3, GM-CSF and G-CSF resulted in an 18-fold increase in cells after 10 to 12 days of culture and a 94-fold increase after 21 days. A 3-fold increase in colony-forming unit granulocyte-macrophage (CFU-GM) was observed after 10 days of culture. The addition of SCF during the first 10 days of culture further augmented the proliferation of cell numbers to 24-fold and colony-forming cells (CFC) to 8-fold after 10 days while cell numbers increased 130-fold after 21 days. Two-color flow cytometry defined phenotypes expressing CD11b and CD15 that represented maturation stages of neutrophils. Maturation of neutrophils in these cultures could be followed by the initial appearance after 3 to 7 days of a CD15+CD11b- phenotype representing promyelocytes, which gave rise after 2 to 3 weeks to a CD15+CD11b+ phenotype representing more mature neutrophil forms (metamyelocytes to segmented neutrophils). In contrast to normal neutrophil development, only a small fraction (10 to 15%) of the culture-derived neutrophils expressed CD16. These data define the kinetics and differentiation of neutrophils and neutrophil precursors from selected CD34+ cells in liquid cultures.

Published

1993

47. Relationship of C5a receptor modulation to the functional responsiveness of human polymorphonuclear leukocytes to C5a.

Author

Van Epps DE, Simpson SJ, and Johnson R

Subjects

Complement C5a metabolism, Humans, Hydrogen Peroxide metabolism, N-Formylmethionine Leucyl-Phenylalanine analogs & derivatives, N-Formylmethionine Leucyl-Phenylalanine pharmacology, Neutrophils drug effects, Neutrophils physiology, Receptor, Anaphylatoxin C5a, Receptors, Complement drug effects, Receptors, Complement physiology, Receptors, Formyl Peptide, Receptors, Immunologic drug effects, Receptors, Immunologic metabolism, Complement C5a pharmacology, Neutrophils metabolism, Receptors, Complement metabolism

Abstract

The relationship of C5a receptor expression on human polymorphonuclear leukocytes (PMN) to the functional response of these cells to C5a was studied using flow cytometry. C5a receptor expression was determined with a fluorescein conjugate of C5a and oxidative burst activity was monitored by conversion of dichlorofluorescein to dichlorofluorescein (DCF) as a measure of H2O2 production. These studies showed that after incubation of PMN with increasing concentrations of C5a, and allowing for internalization of bound ligand, more than 40% of the cell surface C5a receptors were internalized before the DCF response to optimal concentrations of C5a was decreased below the levels for untreated control cells. Although C5a responsiveness was lost after preincubation with 10(-8) M C5a, cells remained responsive to formyl peptide. In other studies, cells were preincubated with unlabeled C5a under conditions that provided for internalization of nearly all C5a receptors. PMN were then cultured for up to 90 min and monitored for C5a receptor reexpression and return of cell function. In these studies, the DCF response of PMN to C5a returned to 100% much earlier than the cells regained full expression of C5a receptors. The DCF response to formyl peptide remained intact throughout the period of C5a receptor reexpression. These studies showed that once > 40% of the original population of C5a receptors are reexpressed on the PMN, that these cells regain 100% of their functional responsiveness to C5a in the DCF assay. Evaluation of the affinity and number of C5a receptors using 125I-labeled C5a after receptor reexpression showed that maximal receptor reexpression was approximately 73% of that obtained with control cells and the Kd of reexpressed receptors was 0.60 vs 0.94 nM for control cells. These studies demonstrate that only a portion of the total C5a receptors expressed on PMN are essential to stimulate a 100% functional response in PMN and that the reexpressed receptors are capable of transducing a signal that activates the oxidative burst in these cells.

Published

1993

48. Chemical modification of interleukin-1 beta: biochemical characterization of a carbodiimide-catalyzed intramolecular cross-linked protein.

Author

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

Subjects

Amino Acid Sequence, Animals, Cell Division, Chromatography, Gel, Chromatography, Ion Exchange, Circular Dichroism, Interleukin-1 pharmacology, Isoelectric Point, Metalloendopeptidases metabolism, Mice, Molecular Sequence Data, Peptide Fragments chemistry, Peptide Fragments metabolism, Peptide Mapping, Recombinant Proteins chemistry, Spectrometry, Fluorescence, Spectrometry, Mass, Fast Atom Bombardment, T-Lymphocytes cytology, Cross-Linking Reagents chemistry, Ethyldimethylaminopropyl Carbodiimide chemistry, Interleukin-1 chemistry

Abstract

We have modified recombinant human Interleukin-1 beta using 1-ethyl-3(3-dimethylaminopropyl)-carbodiimide at pH 6.5, resulting in the formation of an internally cross-linked protein. The major product (30% yield) of the reaction (17 kD; pI = 6.2) was purified and fully characterized by peptide mapping using Endoproteinase Lys C. When digests were conducted under nondenaturing conditions, we found that the modified protein is different from the native protein. The native protein yielded 14 peptides after digestion, whereas only two large peptides and a tetrapeptide, Asn-Tyr-Pro-Lys, were released from the cross-linked protein (i.e., cleavage occurs only at residues Lys88 and Lys92). Using gel filtration, the two peptides were found to co-elute as a single species (15 kD), which represent a noncovalent complex of the amino terminal and C-terminal portions of the molecule. Further analysis of the modified protein by peptide mapping under denaturing conditions and by FAB MS analysis showed that Glu111 and Lys138 were internally cross-linked. The cross-linked protein had bioactivity (T-cell proliferation), fluorescence, and circular dichroism spectra similar to native IL-1 beta. In contrast, while having similar secondary structure, the digested cross-linked protein had less than 1% of T-cell proliferative activity of the undigested protein. These data show that the structural integrity surrounding and perhaps including the Asn-Tyr-Pro-Lys region may be crucial for the biological activity of rIL-1 beta and may be important for the binding of IL-1 to its receptor.

Published

1992

49. Functional characterization of mouse granulocytes and macrophages produced in vitro from bone marrow progenitors stimulated with interleukin 3 (IL-3) or granulocyte-macrophage colony-stimulating factor (GM-CSF).

Author

Bender JG, Unverzagt KL, Maples PB, Mehrotra Y, Mellon J, Van Epps DE, and Stewart CC

Subjects

Animals, Antigens, CD analysis, CD11 Antigens, Cell Differentiation drug effects, Cells, Cultured, Flow Cytometry, Granulocytes cytology, Hematopoiesis drug effects, Hematopoiesis physiology, Hematopoietic Stem Cells drug effects, Hematopoietic Stem Cells metabolism, Hydrogen Peroxide metabolism, Macrophages cytology, Mice, Mice, Inbred C3H, Oxidation-Reduction, Oxygen metabolism, Phagocytosis physiology, Bone Marrow Cells, Granulocyte-Macrophage Colony-Stimulating Factor pharmacology, Granulocytes physiology, Hematopoietic Stem Cells physiology, Interleukin-3 pharmacology, Macrophages physiology

Abstract

Bone marrow from C3H/ouj mice was depleted to < 1% of CD11b+ granulocytes and macrophages using paramagnetic beads coated with sheep anti-rat antibodies. CD11b- cells, enriched three- to fourfold in colony-forming cells, were stimulated in liquid culture with interleukin 3 (IL-3) or granulocyte-macrophage colony-stimulating factor (GM-CSF). Cultures stimulated with IL-3 or GM-CSF increased cell numbers fourfold at 7 days, with the CD11b+ population increasing to 63% +/- 9% (n = 5) with IL-3 or 96% +/- 1% (n = 4) cells with GM-CSF. Functional responsiveness of the granulocytes and macrophages was assessed by flow cytometry in an oxidative burst assay using dichlorofluorescein (DCF) and a quantitative phagocytosis assay using opsonized fluorescent beads. Granulocytes and macrophages, identified by light scatter characteristics and allophycocyanine staining of CD11b, were assayed simultaneously with granulocytes from fresh mouse bone marrow and peripheral blood. GM-CSF-generated CD11b+ cells had higher oxidative responses than similar populations produced in response to IL-3. The oxidative burst of these in vitro generated CD11b+ populations was similar to the equivalent fresh bone marrow population. Oxidative burst responses of peripheral blood phagocytic cells could not be adequately measured in this system. Peripheral blood CD11b+ cells were the most phagocytic, followed by GM-CSF-stimulated CD11b+ cells; IL-3-stimulated and bone marrow CD11b+ cells were the least phagocytic. These data demonstrate that functional granulocytes can be produced in vitro using growth factors and that GM-CSF produces a more responsive cell than IL-3.

Published

1992

50. Interaction of antioxidants with depth-dependent fluorescence quenchers and energy transfer probes in lipid bilayers.

Author

Hinzmann JS, McKenna RL, Pierson TS, Han F, Kezdy FJ, and Epps DE

Subjects

Chromans chemistry, Energy Transfer, Ethylamines chemistry, Fluorescent Dyes, Free Radical Scavengers, Models, Molecular, Molecular Probes, Molecular Structure, Phospholipids chemistry, Piperazines chemistry, Pyridines chemistry, Spectrometry, Fluorescence, Steroids chemistry, X-Ray Diffraction, Antioxidants chemistry, Lipid Bilayers chemistry

Abstract

Three fluorescent, lipophilic, heterocyclic antioxidants were incorporated into lipid bilayers and exposed to depth-dependent nitroxyl fatty acid quenchers. The Stern-Volmer plots curved upward at low quencher concentrations. Quantitative analysis of the results showed that this behavior is consistent with complex formation between quencher and fluorescent antioxidant, where the complex is 2-3 times more fluorescent than the parent fluorophore. At higher quencher concentrations, both free antioxidant and 'bright complex' are quenched dynamically, albeit quenching of the latter is less efficient. The complex probably results from ionic, hydrogen bond and pi-pi interactions. Formation of such a 'bright complex' is also observable in a homogeneous solution of the reactants in cyclohexane. Additional evidence for the complexation of these antioxidants with fatty acids in lipid bilayers is provided by the fact that energy transfer from the antioxidants to anthroyloxy fatty acids occurs at surface concentrations where radiative energy transfer between free molecules should be not be efficient. For directly probing the relative depths of these fluorophores in lipid bilayers we used the aqueous quenchers acrylamide and iodide. They showed that in terms of increasing depth in the bilayer, the order was U-78, 517f < U-78,518e < U-75,412e. Our results, in toto, demonstrate that the Lazaroid antioxidants are incorporated into the lipid bilayer where they occupy strictly defined positions and orientations. Complexation with fatty acyl chains should be mechanistically relevant, since it may enhance antioxidant activity by hindering free radical chain propagation.

Published

1992