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3. Cell-Mediated Hypersensitivity in Guinea-Pigs Infected with Toxoplasma gondii

Author

Lunde Mn, Ourth Dd, and Watson Rr

Subjects
medicine.medical_treatment, Phosphate buffered saline, Toxoplasma gondii, General Medicine, Biology, biology.organism_classification, Cell mediated hypersensitivity, Titer, Macrophage migration inhibition, Delayed hypersensitivity, Toxoplasmin, Immunology, medicine, Adjuvant
Abstract

This investigation demonstrated delayed hypersensitivity by macrophage migration inhibition (MMI) and skin-testing (ST) at 4, 8, 12, and 17 weeks and by lymphocyte transformation (LT) at 4, 12, and 17 weeks after infection of guinea-pigs (GP) with Toxoplasma gondii (C-37 strain). MMI and LT were both most pronounced at 4 and 17 weeks post-infection. GP immunized with toxoplasmin in complete Freund's adjuvant (CFA) demonstrated positive blast transformation and ST, but GP immunized with phosphate buffered saline in CFA did not. MMI was demonstrated with both immunizing preparations. Positive dye test and indirect hemagglutination test titers from 4 through 17 weeks were found.

Published
1976

5. Effects of a phytogenic feed additive on growth performance, susceptibility of channel catfish to Edwardsiella ictaluri and levels of mannose binding lectin.

Author

Peterson BC, Peatman E, Ourth DD, and Waldbieser GC

Subjects
Animal Feed analysis, Animals, Disease Susceptibility microbiology, Disease Susceptibility veterinary, Enterobacteriaceae Infections microbiology, Ictaluridae growth & development, Ictaluridae microbiology, Mannose-Binding Lectin administration & dosage, Oils, Volatile administration & dosage, Diet veterinary, Dietary Supplements analysis, Edwardsiella ictaluri physiology, Enterobacteriaceae Infections veterinary, Fish Diseases microbiology, Ictaluridae immunology, Mannose-Binding Lectin immunology
Abstract

A study was conducted to investigate the effect of a phytogenic feed additive (Digestarom® P.E.P. MGE; containing the essential oils carvacrol, thymol, anethol, and limonene) on growth performance and disease susceptibility to Edwardsiella ictaluri. Two hundred and fifty juvenile channel catfish, Ictalurus punctatus (7.2 ± 0.1 g) were allotted into the following treatments: Control (floating diet) and EO (floating diet supplemented with essential oils). The fish were fed their respective diets for 6 weeks. At the end of the study, all fish were exposed to virulent E. ictaluri by bath immersion (1.9 × 10(7) cfu/mL; final concentration). Plasma and tissue samples were taken to quantify protein and mRNA expression levels of mannose binding lectin (MBL). Weight gain and food conversion ratio were similar between treatments. After exposing fish to virulent E. ictaluri and monitoring mortality for 21 days, survival was 43% higher (69.5 vs 48.4%) in fish fed EO compared to fish not treated with EO (P < 0.05). One day after challenge, plasma MBL levels were down-regulated in the non-treated fish compared to non-challenged fish. In the EO fish, MBL levels were similar to non-challenged fish but significantly higher than non-treated fed fish (P < 0.001). By d 7, plasma MBL levels increased in non-treated fed fish to levels observed in the EO and non-challenged fish. On d 14, MBL mRNA levels were upregulated 15-fold in fish fed EO compared to non-treated fed fish and non-challenged fish (P < 0.001). The results demonstrate that essential oils improved survival of channel catfish challenged with E. ictaluri. Mechanisms through which essential oils improve survival may involve MBL., (Published by Elsevier Ltd.)

Published
2015
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6. Spleen index and mannose-binding lectin levels in four channel catfish families exhibiting different susceptibilities to Flavobacterium columnare and Edwardsiella ictaluri.

Author

LaFrentz BR, Shoemaker CA, Booth NJ, Peterson BC, and Ourth DD

Subjects
Animals, Edwardsiella ictaluri, Enterobacteriaceae Infections genetics, Enterobacteriaceae Infections microbiology, Enterobacteriaceae Infections veterinary, Fish Diseases genetics, Fish Diseases metabolism, Flavobacteriaceae Infections genetics, Flavobacteriaceae Infections microbiology, Flavobacteriaceae Infections veterinary, Genetic Predisposition to Disease, Fish Diseases microbiology, Flavobacterium, Ictaluridae genetics, Ictaluridae metabolism, Mannose-Binding Lectins metabolism, Spleen physiology
Abstract

Edwardsiella ictaluri and Flavobacterium columnare are two bacterial pathogens that affect channel catfish Ictalurus punctatus aquaculture. At the Catfish Genetics Research Unit (U.S. Department of Agriculture, Agricultural Research Service), some progress has been made in selectively breeding for resistance to E. ictaluri; however, the susceptibility of these families to F. columnare is not known. Our objectives were to obtain baseline information on the susceptibility of channel catfish families (maintained as part of the selective breeding program) to E. ictaluri and F. columnare and to determine whether the spleen index and plasma levels of mannose-binding lectin (MBL) are predictive indicators of susceptibility to these pathogens. Four channel catfish families were used: family A was randomly chosen from spawns of fish that were not selectively bred for resistance; families B, C, and D were obtained after selection for resistance to E. ictaluri. All four families were immersion challenged with both bacterial pathogens; the spleen index and plasma MBL levels of unchallenged fish from each family were determined. Mean cumulative percent mortality (CPM) after E. ictaluri challenge ranged from 4% to 33% among families. Families A and B were more susceptible to F. columnare (mean CPM of three independent challenges = 95% and 93%) than families C and D (45% and 48%), demonstrating that there is genetic variation in resistance to F. columnare. Spleen index values and MBL levels were not significantly different, indicating that these metrics are not predictive indicators of F. columnare or E. ictaluri susceptibility in the four tested families. Interestingly, the two families that exhibited the highest CPM after F. columnare challenges had the lowest CPM after E. ictaluri challenge. Further research on larger numbers of families is needed to determine whether there is any genetic correlation between resistance to E. ictaluri and resistance to F. columnare.

Published
2012
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7. Antitumor cell activity in vitro by myristoylated-peptide.

Author

Ourth DD

Subjects
Animals, Antineoplastic Agents chemical synthesis, Antineoplastic Agents isolation & purification, Antineoplastic Agents toxicity, Cell Culture Techniques, Cell Line, Tumor, Cell Proliferation drug effects, Cell Survival drug effects, Fibroblasts drug effects, Hemolymph chemistry, Humans, Lipopeptides chemical synthesis, Lipopeptides isolation & purification, Lipopeptides toxicity, Moths, Antineoplastic Agents pharmacology, Lipopeptides pharmacology
Abstract

New anticancer drugs are needed to support cancer treatment. Cancer involves the uncontrolled proliferation of tumor cells, and many anticancer drugs are agents that inhibit tumor cell growth. The antitumor cell N-myristoylated-peptide is a natural product purified from Heliothis virescens insect hemolymph with essentially no cytotoxicity against human foreskin fibroblast cells. A synthesized structure of six amino acids (Myristoyl-Cys-Ala-Val-Ala-Tyr-[3 methyl]His-OMe; M.W. 902.2 Da) was screened at 10 μM for in vitro antitumor activity against 56 human tumor cell lines by the National Cancer Institute (NCI). The NCI found that 34 of the 56 tumor cell lines (representing eight major tumor types) were sensitive (> 50% growth inhibition of tumor cells) to the myristoylated-peptide. The best overall antitumor activities (>60% average growth inhibition) were seen against 17 tumor cell lines for non-small cell lung cancer, leukemia and melanoma and for eight other tumor cell lines. The NCI finds that their in vitro screen is an effective selector of compounds with in vivo antitumor activity., (Copyright © 2011 Elsevier Masson SAS. All rights reserved.)

Published
2011
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8. Susceptibility in vitro of Epstein-Barr Virus to myristoylated-peptide.

Author

Ourth DD

Subjects
Antiviral Agents chemistry, Cells, Cultured, DNA, Viral metabolism, Fibroblasts drug effects, Fibroblasts metabolism, Herpesvirus 4, Human metabolism, Humans, Lipopeptides chemistry, Peptides chemistry, Viral Matrix Proteins metabolism, Antiviral Agents pharmacology, Herpesvirus 4, Human drug effects, Lipopeptides pharmacology, Peptides pharmacology
Abstract

The anti-Epstein-Barr Virus (EBV) myristoylated-peptide (M.W. 916.2Da) is a natural product isolated from Heliothis virescens insect larval hemolymph (blood) that essentially has no cytotoxicity against human foreskin fibroblast cells. A (3 methyl only) version (M.W. 902.2 Da) of the structure was synthesized and tested for in vitro anti-EBV activity and cytotoxicity. The N-terminal end is lipophilic and used to get the compound across the cell membrane. The C-terminal end with its ring-shaped structures is likely used to inhibit DNA synthesis. The synthetic compound inhibited DNA synthesis/replication of EBV in Akata cells (B-lymphocyte from Burkitt's lymphoma patient) in in vitro tissue culture. A DNA hybridization assay for anti-EBV activity using the Akata B-cell and two cytotoxicity assays using human foreskin fibroblast cells were done with the synthetic peptide. Effective concentration (EC90) at 20 microM inhibited viral replication by 90%. The EBV, known as Human Herpesvirus-4 (HHV-4) of the Herpesviridae family, has been described as a cancer-promoting double-stranded DNA virus that may also be involved in autoimmune disease. There are no antiviral drugs in clinical use for diseases caused by the EBV., (Copyright 2010 Elsevier Inc. All rights reserved.)

Published
2010
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9. Isolation of lysozyme and an antifungal peptide from sea lamprey (Petromyzon marinus) plasma.

Author

Rose WM and Ourth DD

Subjects
Animals, Antifungal Agents immunology, Antifungal Agents isolation & purification, Antifungal Agents pharmacology, Antimicrobial Cationic Peptides blood, Antimicrobial Cationic Peptides immunology, Antimicrobial Cationic Peptides isolation & purification, Antimicrobial Cationic Peptides pharmacology, Aspergillus flavus drug effects, Chromatography, Gel, Fish Proteins immunology, Fish Proteins isolation & purification, Fish Proteins pharmacology, Gram-Negative Bacteria drug effects, Gram-Positive Bacteria drug effects, Immunity, Innate, Microbial Sensitivity Tests, Molecular Weight, Muramidase immunology, Muramidase isolation & purification, Muramidase pharmacology, Penicillium chrysogenum drug effects, Petromyzon blood, Antifungal Agents blood, Fish Proteins blood, Muramidase blood, Petromyzon immunology
Abstract

The sea lamprey (Petromyzon marinus) belongs to the most primitive class of fish and has only innate immunity. The innate immune factors, lysozyme and an antifungal peptide, were isolated from sea lamprey plasma. Sea lamprey plasma (40.1mg protein/ml) was assayed for lysozyme activity by gel diffusion assay. Using hen egg white lysozyme standards, plasma concentration of lamprey lysozyme was 5microg lysozyme/mg total protein. The presence of lysozyme in such high concentration in lamprey plasma could be important in their innate immunity and resistance to infection. Lysozyme and the antifungal peptide were isolated by low molecular weight gel filtration chromatography from sea lamprey plasma. Gel filtration chromatography yielded two peak tubes containing lysozyme (1microg/211microg total protein) and antifungal peptide (1microg/66microg total protein). Lysozyme and antifungal activity of each fraction were determined by well diffusion assay using Gram-negative bacteria, Gram-positive bacteria and two fungal species. The molecular weight of lamprey lysozyme was 14.3kDa. The sea lamprey lysozyme was effective against Gram-positive bacteria but not against Gram-negative bacteria or fungi. Molecular weight of the antifungal peptide was approximately 3000Da. Antifungal plasma activity was seen against Penicillium notatum and Aspergillus flavus. No plasma antibacterial peptide was found.

Published
2009
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10. Isolation of mannose-binding C-type lectin from sea lamprey (Petromyzon marinus) plasma and binding to Aeromonas salmonicida.

Author

Ourth DD, Rose WM, and Siefkes MJ

Subjects
Amino Acid Sequence, Animals, Blotting, Western, Chromatography, Affinity, Electrophoresis, Polyacrylamide Gel, Mannose metabolism, Mannose-Binding Lectin blood, Molecular Sequence Data, Sequence Analysis, Protein, Aeromonas salmonicida metabolism, Mannose-Binding Lectin genetics, Mannose-Binding Lectin metabolism, Petromyzon genetics
Abstract

The sea lamprey (Petromyzon marinus) is a parasitic cartilaginous fish of the North American Great Lakes and a predator of many bony fish species of commercial importance to the fishing industry. Mannose-binding C-type lectin (MBL) was isolated by mannan-agarose affinity chromatography from sea lamprey plasma. Mannose-binding lectin has not before been identified and quantitated in the plasma of this sea lamprey species. The affinity-purified and 2-ME reduced lamprey MBL showed two bands of 35kDa and 65kDa by SDS-PAGE and Western blotting using guinea pig anti-MBL IgG as the primary antibody. Amino acid composition analysis (mol%) of the purified lamprey MBL found high amounts of histidine, threonine, tyrosine and phenylalanine present when compared with three other vertebrate MBLs. N-terminal amino acid sequencing by Edman degradation for the first 10 residues gave XXXTKGCPDA. Lamprey plasma contained 261mug of MBL/ml of plasma. Plasma protein concentration was 40.1mg/ml. Lamprey MBL was present then in plasma at 6.5mug MBL/mg total protein. The sea lamprey MBL also specifically binds to mannose on the surface of the pathogen Aeromonas salmonicida. The presence of MBL in high concentration in lamprey plasma could be important in their innate immunity and resistance to infection. This study describes the presence of MBL in sea lamprey plasma and evidence for a C-type lectin complement pathway of innate immunity.

Published
2008
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11. Comparative study of mannose-binding C-type lectin isolated from channel catfish (Ictalurus punctatus) and blue catfish (Ictalurus furcatus).

Author

Ourth DD, Narra MB, and Simco BA

Subjects
Animals, Blotting, Western, Chromatography, Affinity veterinary, Edwardsiella ictaluri immunology, Guinea Pigs, Immunoglobulin G biosynthesis, Immunoglobulin G metabolism, Species Specificity, Ictaluridae immunology, Mannose-Binding Lectin blood, Mannose-Binding Lectin chemistry, Mannose-Binding Lectin isolation & purification, Mannose-Binding Lectin metabolism
Abstract

Mannose-binding C-type lectin (MBL) was isolated from channel catfish (Ictalurus punctatus) NWAC 102 and 103 strains, blue catfish (Ictalurus furcatus) D+B and Rio Grande strains, hybrid catfish (channel catfish female NWAC 103 x blue catfish male D+B) sera, and purified by affinity chromatography from channel catfish Norris strain serum. Reduction of purified channel catfish MBL with 2-ME yielded a single band of 62 kDa by SDS-PAGE and Western blot analysis using guinea pig anti-MBL IgG as primary antibody. Channel catfish NWAC 102 strain, channel catfish NWAC 103 strain and hybrid catfish sera had molecular masses of 63 kDa for MBL. Blue catfish (D+B strain) serum MBL had a molecular mass of 66 kDa. Rio Grande blue catfish serum MBL had a molecular mass of 65 kDa. Amino acid composition analysis (mol%) of the affinity-purified channel catfish MBL found a high content of serine present. Functional binding studies of channel catfish and blue catfish MBLs binding to Edwardsiella ictaluri were done using a dot-immunoblot ELISA method. A dot-immunoblot ELISA binding assay was done to compare nine different strains and species of channel catfish and blue catfish for their levels of serum MBL. Blue catfish had higher levels of MBL than did the various strains of channel catfish tested. MBL could be used as a genetic marker for selection of disease resistance in the different strains of catfish used in aquaculture. This study describes the presence of serum MBL in catfish and evidence for a C-type lectin complement pathway of innate immunity.

Published
2007
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12. Isolation of mannose-binding C-type lectin from Heliothis virescens pupae.

Author

Ourth DD, Narra MB, and Chung KT

Subjects
Amino Acid Sequence, Animals, Mannose-Binding Lectins analysis, Molecular Sequence Data, Molecular Weight, Pupa metabolism, Hemolymph metabolism, Mannose-Binding Lectin analysis, Mannose-Binding Lectin chemistry, Mannose-Binding Lectins chemistry, Moths metabolism, Sequence Analysis, Protein
Abstract

A mannose-binding C-type lectin (MBL) was isolated by affinity chromatography from Heliothis virescens immune pupal hemolymph. The immune pupal hemolymph was obtained after bacterial injection of live Enterobacter cloacae bacteria. MBL in mammals acts as an opsonin for phagocytosis and activates the lectin complement pathway of the innate immune response, which leads to killing of gram-negative bacteria and enveloped viruses. The affinity-purified and reduced pupal MBL showed a single band of 36 kDa by SDS-PAGE (12% gel). A dot-immunoblot ELISA (using guinea pig anti-MBL IgG as primary antibody) demonstrated specificity of the antibody for the affinity-purified pupal MBL. The immune pupal hemolymph contained 21 microg of MBL per ml of hemolymph. The amino acid composition of the purified pupal MBL was determined with high amounts of arginine and histidine detected. The presence of MBL in insect pupae has not before been reported and could be important in pupal innate immunity to bacterial infection.

Published
2005
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13. Ureaplasma urealyticum binds mannose-binding lectin.

Author

Benstein BD, Ourth DD, Crouse DT, and Shanklin DR

Subjects
Animals, Autopsy, Guinea Pigs, Humans, Infant, Lung immunology, Lung metabolism, Lung Diseases immunology, Lung Diseases microbiology, Mannose-Binding Lectin genetics, Mannose-Binding Lectin immunology, Mice, Protein Binding, Rabbits, Ureaplasma Infections immunology, Ureaplasma Infections metabolism, Ureaplasma Infections microbiology, Lung microbiology, Lung Diseases metabolism, Mannose-Binding Lectin metabolism, Ureaplasma urealyticum metabolism
Abstract

Mannose-binding C-type lectin (MBL) is an important component of innate immunity in mammals. Mannose-binding lectin (MBL), an acute phase protein, acts as an opsonin for phagocytosis and also activates the mannan-binding lectin complement pathway. It may play a particularly significant role during infancy before adequate specific protection can be provided by the adaptive immune system. Ureaplasma urealyticum has been linked to several diseases including pneumonia and chronic lung disease (CLD) in premature infants. We therefore investigated the ability of U. urealyticum to bind MBL. A guinea pig IgG anti-rabbit-MBL antiserum was produced. An immunoblot (dot-blot) assay done on nitrocellulose membrane determined that the anti-MBL antibody had specificity against both rabbit and human MBL. Pure cultures of U. urealyticum, serotype 3, were used to make slide preparations. The slides containing the organisms were then incubated with nonimmune rabbit serum containing MBL. Ureaplasma was shown to bind rabbit MBL with an immunocytochemical assay using the guinea pig IgG anti-rabbit MBL antiserum. Horseradish peroxidase (HRP)-labeled anti-guinea pig IgG was used to localize the reaction. The anti-MBL antiserum was also used in an immunocytochemical assay to localize U. urealyticum in histological sections of lungs from mice specifically infected with this organism. The same method also indicated binding of MBL by ureaplasma in human lung tissue obtained at autopsy from culture positive infants. Our results demonstrate that ureaplasma has the capacity to bind MBL. The absence of MBL may play a role in the predisposition of diseases related to this organism.

Published
2004
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14. Antiviral activity against human immunodeficiency virus-1 in vitro by myristoylated-peptide from Heliothis virescens.

Author

Ourth DD

Subjects
Animals, Cells, Cultured, Insect Proteins chemistry, Insect Proteins isolation & purification, Antiviral Agents pharmacology, HIV-1 drug effects, HIV-1 growth & development, Insect Proteins metabolism, Insect Proteins pharmacology, Moths metabolism
Abstract

An insect antiviral compound was purified from Heliothis virescens larval hemolymph by gel-filtration high pressure liquid chromatography (HPLC) and C-18 reverse-phase HPLC and its structure was determined by mass spectrometry. The antiviral compound is an N-myristoylated-peptide containing six amino acids with calculated molecular weight of 916 Da. The N-terminus contains the fatty acid myristoyl, and the C-terminus contains histidine with two methyl groups giving the histidine a permanent positive charge. The remainder of the compound is essentially non-polar. The structure of the compound corresponds with the 'myristate plus basic' motif expressed by certain viral proteins in their binding to the cytoplasmic side of the plasma membrane to initiate viral assembly and budding from a host cell. The insect antiviral compound may inhibit viral assembly and/or budding of viruses from host cells that could include the human immunodeficiency virus-1 (HIV-1) and herpes simplex virus-1 that use this motif for exit from a host cell. Using the formazan assay, the myristoylated-peptide was effective against HIV-1, with a nine times increase in the viability and protection in vitro of treated CEM-SS cells when compared with infected but untreated control cells.

Published
2004
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15. Purification of antimicrobial factor from granules of channel catfish peripheral blood leucocytes.

Author

Ourth DD and Chung KT

Subjects
Aeromonas hydrophila drug effects, Animals, Anti-Bacterial Agents chemistry, Anti-Bacterial Agents isolation & purification, Anti-Bacterial Agents pharmacology, Antiviral Agents chemistry, Antiviral Agents isolation & purification, Antiviral Agents pharmacology, Blood Proteins chemistry, Blood Proteins pharmacology, Diffusion, Edwardsiella ictaluri drug effects, Electrophoresis, Polyacrylamide Gel, Escherichia coli drug effects, Herpesvirus 1, Human drug effects, Microbial Sensitivity Tests methods, Molecular Weight, Anti-Bacterial Agents blood, Blood Proteins isolation & purification, Catfishes blood, Cytoplasmic Granules chemistry, Leukocytes chemistry
Abstract

The channel catfish (Ictalurus punctatus) is extensively used in aquaculture in the Southeast US and is susceptible to many bacterial infections acquired from its pond environment. Research is needed to better understand the defensive response and innate immunity of channel catfish against fish pathogens like Edwardsiella ictaluri and Aeromonas hydrophila. The main objectives were purification and characterization of an innate antimicrobial factor isolated from catfish leucocytes that has both bactericidal and antiviral activities. Oxygen-independent mechanisms of innate immunity for killing microorganisms have not been identified in leucocytes of channel catfish. Leucocytes were separated from catfish blood, and granule extracts were obtained by homogenization, centrifugation, and extraction with 10% acetic acid. The granule extracts were further purified by gel filtration chromatography. Bactericidal assays against the two fish pathogens and SDS-PAGE analysis were done on the isolated antimicrobial factor. Determination of antiviral activity of the factor was done by in vitro tissue culture using herpes simplex virus-type 1. Mass spectrometry analyses were done for molecular weight (655 Da), purity, and structural characterization of the innate non-peptide antimicrobial factor.

Published
2004
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16. Ureaplasma in lung. 2. Association with bronchopulmonary dysplasia in premature newborns.

Author

Benstein BD, Crouse DT, Shanklin DR, and Ourth DD

Subjects
Birth Weight, Bronchopulmonary Dysplasia pathology, Female, Gestational Age, Humans, In Situ Hybridization, Incidence, Infant, Infant, Newborn, Lung microbiology, Lung pathology, Risk Factors, Ureaplasma Infections pathology, Bronchopulmonary Dysplasia microbiology, Infant, Premature, Ureaplasma Infections microbiology, Ureaplasma urealyticum isolation & purification
Abstract

Infants with Ureaplasma urealyticum in the lower respiratory tract are at risk for chronic lung disease (CLD) or bronchopulmonary dysplasia (BPD) but causality has been difficult to prove. The goal of this study was to identify ureaplasma in human neonatal lung tissue using the in situ hybridization (ISH) procedure described in Part 1 (Exp. Mol. Pathol., in press) of this report. By correlating their presence with the histopathologic findings, it may be possible to provide further evidence of the pathogenicity of ureaplasmas and their association with BPD. Lung autopsy tissue from seven infants with positive cultures and seven infants with negative cultures for ureaplasma were included in the study. All culture-positive infants were positive for ureaplasma on ISH and all had histopathologic evidence of BPD. Two of the seven infants with negative cultures were positive for ureaplasma with ISH. Of interest, these two infants were also found to have BPD at autopsy. The other five infants with negative cultures were also negative for ureaplasma on ISH and had no evidence of BPD. This study correlates the presence of U. urealyticum by ISH with the finding of BPD on histopathologic evaluation and provides evidence that it has a role in the development of CLD.

Published
2003
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17. Ureaplasma in lung. 1. Localization by in situ hybridization in a mouse model.

Author

Benstein BD, Crouse DT, Shanklin DR, and Ourth DD

Subjects
Administration, Intranasal, Animals, Animals, Newborn, Bronchopulmonary Dysplasia pathology, DNA, Viral analysis, Humans, Immunoenzyme Techniques, In Situ Hybridization, Infant, Newborn, Lung microbiology, Lung ultrastructure, Mice, Polymerase Chain Reaction, Ureaplasma Infections pathology, Ureaplasma urealyticum genetics, Ureaplasma urealyticum ultrastructure, Bronchopulmonary Dysplasia microbiology, Disease Models, Animal, Ureaplasma Infections microbiology, Ureaplasma urealyticum isolation & purification
Abstract

Ureaplasma urealyticum is a common inhabitant of mucosal surfaces but is also associated with a higher incidence of pneumonia and bronchopulmonary dysplasia in preterm infants. Culture and polymerase chain reaction demonstrate high isolation rates of ureaplasma in clinical specimens documenting their presence but do not associate the organism directly with the diseased tissue. In this study, lung tissue samples from newborn mice inoculated intranasally with U. urealyticum were used to develop an in situ hybridization (ISH) test for the organism. In situ hybridization allows the localization of gene expression for visualization within the context of tissue morphology. New techniques which use biotinyl-tyramide based signal amplification have been able to greatly enhance the sensitivity of ISH. Using the Dako GenPoint Catalyzed Signal Amplification system to detect a biotinylated DNA probe specific for an internal nucleotide sequence within the urease gene of U. urealyticum, the organism was detected within the infected murine lung tissues. Electron microscopy was used to verify the presence of the organisms in the positive ISH areas. The ISH procedure developed in this study can be used to analyze the presence of ureaplasma in human neonatal lung tissue with the corresponding histopathology.

Published
2003
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18. Purification and characterization of apolipophorin III from immune hemolymph of Heliothis virescens pupae.

Author

Chung KT and Ourth DD

Subjects
Amino Acid Sequence, Animals, Apolipoproteins metabolism, Apolipoproteins pharmacology, Chromatography, Gel, Chromatography, High Pressure Liquid, Erythrocytes metabolism, Hemagglutination Tests, Lectins metabolism, Lepidoptera immunology, Molecular Sequence Data, Molecular Weight, Pupa immunology, Rabbits, Sequence Alignment, Sequence Analysis, Protein, Spectrum Analysis, Apolipoproteins chemistry, Apolipoproteins isolation & purification, Hemolymph chemistry, Hemolymph immunology, Lepidoptera chemistry, Lepidoptera growth & development, Pupa chemistry
Abstract

Apolipophorin III (ApoLp-III) from Heliothis virescens pupae was purified by heat-treatment followed by Sephadex G-50 filtration and reverse phase-HPLC. The molecular mass of the purified ApoLp-III was determined as 17965.9+/-5 Da by mass spectrometry. The N-terminal sequence confirmed the protein as ApoLp-III with homology of 56-83% to other insect ApoLp-III molecules. The amino acid spatial arrangement of the predicted alpha-helix 1 of Heliothis ApoLp-III was nearly identical to that of the amphipatic alpha-helix 1 of Manduca sexta ApoLp-III. The absorption spectrum from 240-340 nm of the Heliothis ApoLp-III was the same as the UV spectra of ApoLp-III from Manduca sexta and Galleria mellonella, showing absorption maxima at 280, 268, 264 and 259 nm. These results indicated that the primary structure of ApoLp-III is conserved in lepidopterans. The Heliothis ApoLp-III was not a glycoprotein and showed hemagglutination activity against rabbit red blood cells. This hemagglutination activity was abolished by Tween 80, but not by six different carbohydrates. Hydrophobic interaction of ApoLp-III with red blood cells agreed with structural studies since ApoLp-III binds lipid through hydrophobic interaction after conformational change. Bacterial injection apparently increased the amount of ApoLp-III in immune hemolymph when compared with normal hemolymph, and may indicate that ApoLp-III plays a role in insect immunity.

Published
2002
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19. Larval and pupal induction and N-terminal amino acid sequence of lysozyme from Heliothis virescens.

Author

Chung KT and Ourth DD

Abstract

Fifth instar larvae and prepupae of Heliothis virescens (tobacco budworm) were injected with live Enterobacter cloacae and bled at different times after vaccination. Immune pupal hemolymph showed a 54 times increase in lysozyme activity when compared with normal larval hemolymph, and an 11 times increase of lysozyme activity when compared with immune larval hemolymph. Lysozyme activity of the normal pupal hemolymph increased as greatly as did lysozyme activity of the immune larval hemolymph after metamorphosis. The pupal immune response with regard to lysozyme was much greater than the larval immune response in H. virescens. Lysozyme was purified by heat treatment at 100 degrees C and a chromatography series that included reverse-phase HPLC. The molecular mass of H. virescens lysozyme was approximately 16 kDa by SDS-PAGE which is greater than other insect lysozymes and chicken lysozyme. Amino acid sequence of the N-terminus showed that H. virescens lysozyme is 82% homologous with lysozyme of Manduca sexta and Galleria mellonella. CNBr cleavage of H. virescens lysozyme produced 11 and 6 kDa peptide fragments indicating that one methionine was present, which was also supported by amino acid analysis. However, methionine was located at the carboxyl terminal side rather than the N-terminal side as judged by the N-terminal sequences of each peptide fragment. The residue 22 in most lepidopteran lysozymes is methionine, whereas H. virescens lysozyme had a leucine at residue 22. There was an amino acid deletion near the carboxyl terminal side of H. virescens lysozyme as also found in Trichoplusia ni.

Published
2000
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20. Binding sites for human interferon-gamma in protocerebrum and hemolymph of tobacco hornworm (Manduca sexta) larvae differ in sensitivity to polycationic peptides.

Author

Parker MS and Ourth DD

Subjects
Amino Acids metabolism, Amino Acids pharmacology, Animals, Binding, Competitive, Brain Chemistry, Humans, Interferon-gamma antagonists & inhibitors, Kinetics, Larva chemistry, Larva metabolism, Manduca metabolism, Protein Binding, Rabbits, Radioligand Assay, Receptors, Neuropeptide Y metabolism, Tissue Extracts, Hemolymph chemistry, Interferon-gamma metabolism, Manduca chemistry
Abstract

We have recently characterized specific binding sites for human interferon-gamma on particulates prepared from the protocerebrum and hemolymph of tobacco hornworm larvae, Manduca sexta ¿(Parker, M.S., Ourth, D.D., 1999. Comp. Biochem. Physiol. B 122, 155-163). The sensitivity to sulfated polysaccharides indicated an involvement of oligobasic epitopes of hIFN-gamma in the binding. In the present study, we found that polycationic peptides inhibited the binding of [125I]hIFN-gamma to particulates from either the hemolymph or the protocerebrum of Manduca sexta larvae. With amino acid homopolymers, the rank order of potency was poly-L-lysine > poly-L-arginine >> poly-L-ornithine, while the acidic side chain polymer poly-L-aspartate was not inhibitory. However, the potency of all polycationic peptides was at least three-fold greater at the hemolymph particulates. Also, acidic polysaccharides such as heparin were much more efficacious in the inhibition of hIFN-gamma binding to hemolymph relative to protocerebral particulates. The peptide polycations inhibited the binding of [125I](Leu31,Pro34)human peptide YY, a ligand selective for the Y1 subtype of the neuropeptide Y receptor, to rabbit kidney or to parietal cortex particulates with the expected rank order of poly-L-arginine > poly-L-lysine >> poly-L-ornithine, and with little cross-tissue difference in affinity. The selectivity observed with M. sexta particulates indicates a preferential involvement of oligobasic lysine-rich C-terminal sequences of IFN-gamma, while large insect tissue-related affinity differences point to involvement of diverse oligoacidic sequences in binding to protocerebrum and hemolymph sites. This study provides evidence for the presence of molecules in lepidopteran larvae that are similar in structure to vertebrate co-receptors of IFN-gamma, and adds to the characterization of these binding sites.

Published
2000
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21. Viresin. A novel antibacterial protein from immune hemolymph of Heliothis virescens pupae.

Author

Chung KT and Ourth DD

Subjects
Amino Acid Sequence, Animals, Anti-Bacterial Agents chemistry, Anti-Bacterial Agents pharmacology, Gram-Negative Bacteria drug effects, Hemolymph chemistry, Hemolymph immunology, Insect Proteins genetics, Insect Proteins pharmacology, Larva chemistry, Larva immunology, Lepidoptera genetics, Lepidoptera immunology, Molecular Sequence Data, Molecular Weight, Pupa chemistry, Pupa immunology, Sequence Homology, Amino Acid, Anti-Bacterial Agents isolation & purification, Insect Proteins isolation & purification, Lepidoptera chemistry
Abstract

Immune hemolymph was collected from fifth instar larvae and 1-day-old pupae of Heliothis virescens after injection of prepupae with live Enterobacter cloacae. Induction of antibacterial activity against Escherichia coli K12 D31 was 7.5 times greater in pupal than in larval immune hemolymph. Lysozyme activity of immune pupal hemolymph against Micrococcus lysodeikticus was 11 times greater when compared with lysozyme activity of immune larval hemolymph. Early pupal immune response with regard to antibacterial activity was much greater than larval immune response in H. virescens. Normal pupal hemolymph showed an increase in antibacterial activity and lysozyme that was induced during metamorphosis. Antibacterial protein was isolated together with lysozyme by gel filtration chromatography and then separated from lysozyme by sequential electrophoresis with a native acid gel and SDS gel. Molecular mass of antibacterial protein was estimated to be 12 kDa. The N-terminal amino acid sequence of 12-kDa protein was different from those of antibacterial molecules found in other insects and has not been identified before. A sample containing 12-kDa protein was negative for immunoblotting with anti-synthetic cecropin B antibody. We have named the novel 12-kDa antibacterial protein viresin. Viresin showed antibacterial activity against several Gram-negative bacteria including E. cloacae but not against Gram-positive bacteria.

Published
2000
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22. Specific binding of human interferon-gamma to particulates from hemolymph and protocerebrum of tobacco hornworm (Manduca sexta) larvae.

Author

Parker MS and Ourth DD

Subjects
Amino Acid Sequence, Animals, Binding Sites, Blood Platelets metabolism, Female, Growth Hormone metabolism, Hemolymph drug effects, Heparin pharmacology, Humans, Interferon-gamma antagonists & inhibitors, Iodine Radioisotopes, Larva metabolism, Molecular Sequence Data, Plants, Toxic, Pregnancy, Prolactin metabolism, Rats, Recombinant Proteins metabolism, Nicotiana parasitology, Brain metabolism, Hemolymph metabolism, Interferon-gamma metabolism, Manduca physiology
Abstract

Specific binding sites for human interferon-gamma (hIFN-gamma) were found on particulates prepared from the hemolymph and protocerebrum of fifth-instar larvae of the tobacco hornworm, Manduca sexta. A portion of these sites could be solubilized in an active form by the zwitterionic detergent 3-[(3-cholamidopropyl)dimethylammonio]-1-propane sulfonate (CHAPS). A well-defined specific binding was also associated with hemolymph particulate residue after solubilization by CHAPS. About one-half of [125I]hIFN-gamma binding could be displaced by heparin. The bound hIFN-gamma could be covalently cross-linked to the binding sites using disuccinylamide suberate, and the molecular weight range of these complexes was 200-800 kDa as determined by density gradient sedimentation and gel-exclusion chromatography. Only a small fraction of the hemolymph IFN-gamma binding could be competed by another mammalian cytokine, rat prolactin (rPRL), while there was no sensitivity to rat growth hormone. The small specific rPRL binding found in Manduca hemolymph showed an affinity similar to the prolactin sites found in the liver of pregnant rats. The detergent-insoluble Manduca hIFN-gamma binding was bimodal and similar in affinity distribution to the binding found with human platelet membranes (Kdiss range 0.1-2 nM). The detergent-solubilized IFN-gamma sites were homogenous, with a Kdiss of about 1.5 nM. The IFN-gamma binding sites in Manduca tissues may therefore include molecular species similar to the known invertebrate cytokine receptors and proteoglycan co-receptors.

Published
1999
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23. Purification and characterization of lysozyme from hemolymph of Heliothis virescens larvae.

Author

Lockey TD and Ourth DD

Subjects
Animals, Anti-Bacterial Agents isolation & purification, Anti-Bacterial Agents pharmacology, Chromatography, Gel, Chromatography, Ion Exchange, Electrophoresis, Polyacrylamide Gel, Enzyme Stability, Escherichia coli drug effects, Gram-Positive Bacteria drug effects, Hot Temperature, Larva, Microbial Sensitivity Tests, Molecular Weight, Muramidase pharmacology, Thermodynamics, Hemolymph enzymology, Lepidoptera enzymology, Muramidase isolation & purification, Muramidase metabolism
Abstract

Lysozyme is an important antibacterial protein in the insect defense system. Lysozyme was isolated from hemolymph of Heliothis virescens larvae using gel filtration and ion-exchange chromatography. Heliothis lysozyme had a molecular mass of 16,000 daltons by SDS-PAGE. Using acid gel electrophoresis, Heliothis lysozyme migrated faster than egg white lysozyme. The pI of Heliothis lysozyme was estimated as greater than 9.5. Heliothis lysozyme had specific bactericidal activity against three Gram-positive bacteria but no activity against Escherichia coli. The bactericidal activity was stable at 100 degrees C at pH 3.0 after 60 min incubation, but was labile at 100 degrees C at pH 6.8 after 60 min incubation. Heliothis lysozyme was an inducible protein that increased 9 times when comparing unvaccinated with vaccinated larvae. Lysozyme from H. virescens was more similar in molecular mass, heat sensitivity and pH sensitivity to lysozyme isolated from Galleria mellonella and Bombyx mori than to lysozyme isolated from Hyalophora cecropia.

Published
1996
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24. Formation of pores in Escherichia coli cell membranes by a cecropin isolated from hemolymph of Heliothis virescens larvae.

Author

Lockey TD and Ourth DD

Subjects
Animals, Anti-Bacterial Agents pharmacology, Cell Membrane drug effects, Cell Membrane ultrastructure, Escherichia coli drug effects, Escherichia coli ultrastructure, Insect Hormones immunology, Insect Hormones pharmacology, Larva chemistry, Anti-Bacterial Agents isolation & purification, Chromatography, Affinity methods, Hemolymph chemistry, Insect Hormones isolation & purification, Insect Proteins, Lepidoptera chemistry
Abstract

The insect humoral defense system produces antibacterial peptides called cecropins. Cecropins were initially isolated from Hyalophora cecropia pupae and have since been isolated and identified in various insects. In this study, we have isolated and identified a cecropin from Heliothis virescens larvae. Rabbit IgG were raised against synthetic cecropin B. Affinity chromatography with the rabbit anti-(cecropin B) IgG was used to isolate a cecropin from hemolymph of H. virescens larvae. Acid gel electrophoresis followed by a bacterial-overlay analysis showed that Heliothis cecropin is a basic peptide of low molecular mass with bactericidal activity against Escherichia coli K12 D31. Heliothis cecropin is therefore analogous to synthetic cecropin B. One unresolved issue concerning cecropins and other antibiotic peptides is the mode of action by which they kill bacteria. By means of electron microscopy and immunocytochemistry with gold-labeled rabbit anti-cecropin IgG, binding of purified and synthetic cecropin to the cell membranes of E. coli K12 D31 cells was observed. Small lesions in the cell membrane were seen that had a diameter of 9.6 nm and internal pore of 4.2 nm. The Heliothis cecropin was found to be a pore-forming molecule that causes lesions in the cell membrane of E. coli K12 D31. The lesions lead to leakage of cytoplasmic contents and death of bacteria.

Published
1996
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25. Induction of cecropin-like and attacin-like antibacterial but not antiviral activity in Heliothis virescens larvae.

Author

Ourth DD, Lockey TD, and Renis HE

Subjects
Animals, Anti-Bacterial Agents, Cell Membrane drug effects, Cell Membrane ultrastructure, Enterobacter cloacae drug effects, Escherichia coli drug effects, Escherichia coli ultrastructure, Hemolymph physiology, Insect Hormones isolation & purification, Insect Hormones toxicity, Larva, Lepidoptera metabolism, Microbial Sensitivity Tests, Microscopy, Electron, Scanning, Molecular Weight, Pseudomonas aeruginosa drug effects, Anti-Infective Agents isolation & purification, Anti-Infective Agents toxicity, Antiviral Agents, Insect Hormones biosynthesis, Insect Proteins, Lepidoptera physiology
Abstract

Inducible cecropin-like and attacin-like proteins were isolated from immune hemolymph obtained from vaccinated Heliothis virescens larvae. The attacin-like protein had a molecular weight of approximately 25,000 daltons and was not dialyzable. The cecropin-like peptide had an estimated molecular weight of 6,000-7,000 daltons and was dialyzable, heat-stable and sensitive to trypsin digestion. The cecropin-like peptide showed bactericidal activity against Escherichia coli and Enterobacter cloacae, and the attacin-like protein showed bactericidal activity against E. coli. The immune hemolymph was bactericidal against E. coli, E. cloacae and Pseudomonas aeruginosa. Ultrastructural cell envelope damage to E. coli, produced by the immune hemolymph, was observed by scanning electron microscopy. No antiviral activity by the inducible cecropin-like and attacin-like proteins was detected against herpes simplex virus-1 and the vesicular stomatitis virus.

Published
1994
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26. Opsonic effect of the alternative complement pathway on channel catfish peripheral blood phagocytes.

Author

Jenkins JA and Ourth DD

Subjects
Animals, Bacteria immunology, Complement Activation immunology, Microspheres, Monocytes immunology, Neutrophils immunology, Phagocytosis immunology, Receptors, Complement immunology, Complement Pathway, Alternative immunology, Ictaluridae immunology, Opsonin Proteins immunology, Phagocytes immunology
Abstract

This study determined the effect of the alternative complement pathway (ACP) on neutrophil and monocyte phagocytes from peripheral blood of channel catfish, Ictalurus punctatus. Fluorescent-labeled latex microspheres, Edwardsiella ictaluri and Escherichia coli were used to quantify phagocytic attachment and ingestion. Activation of the ACP enhanced the attachment of bacteria and microspheres to neutrophils and monocytes. Activation of the ACP by serum opsonization of Escherichia coli increased its ingestion by neutrophils in comparison with Edwardsiella ictaluri and microspheres. Inactivation of the ACP and C3b diminished attachment by neutrophils and monocytes, and ingestion by neutrophils of microspheres and bacteria. Ingestion by monocytes was not affected by activation of the ACP. In the present study, we found that the ACP functions in opsonophagocytosis in catfish and that ingestion by neutrophils was especially enhanced.

Published
1993
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27. Antiviral melanization reaction of Heliothis virescens hemolymph against DNA and RNA viruses in vitro.

Author

Ourth DD and Renis HE

Subjects
Animals, Basidiomycota enzymology, Enterovirus B, Human growth & development, Hemolymph immunology, Immunization, Larva, Monophenol Monooxygenase metabolism, Parainfluenza Virus 3, Human growth & development, Simplexvirus growth & development, Sindbis Virus growth & development, Vero Cells, Vesicular stomatitis Indiana virus growth & development, Antiviral Agents pharmacology, DNA Viruses growth & development, Hemolymph physiology, Moths, RNA Viruses growth & development
Abstract

1. Antiviral activity of Heliothis virescens larval hemolymph was determined using a cytotoxicity/virus inhibition test (TClD50) done in Vero cell tissue cultures. Excellent antiviral activity was found especially against herpes simplex viruses-1 and -2 and also against vesicular stomatitis, parainfluenza-3, coxsackie B3 and sindbis viruses. 2. Prolonged incubation of herpes simplex virus-1 and vesicular stomatitis virus with hemolymph was virucidal and greatly reduced infectivity of the two viruses in tissue culture. 3. Antiviral activity was produced by both normal and immune (vaccinated larvae) cell-free hemolymphs. 4. Antiviral activity against herpes simplex virus-1 could be generated in vitro with hemolymph phenoloxidase or mushroom tyrosinase using four different substrates including tyrosine. 5. Activation of the insect melanization reaction by phenoloxidase was necessary for antiviral activity to occur.

Published
1993
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28. Membrane damage to Escherichia coli and bactericidal kinetics by the alternative complement pathway of channel catfish.

Author

Jenkins JA and Ourth DD

Subjects
Animals, Cell Membrane Permeability immunology, Escherichia coli immunology, Escherichia coli ultrastructure, In Vitro Techniques, Kinetics, Blood Bactericidal Activity immunology, Complement Pathway, Alternative, Ictaluridae immunology
Abstract

1. Increased permeability of cytoplasmic membranes in Escherichia coli was a consequence of alternative complement pathway (ACP) activity of serum of channel catfish, Ictalurus punctatus. Evidence was provided by beta-galactosidase activity extracellularly when E. coli was incubated with catfish serum. 2. Lesions were detected on outer membranes of E. coli following exposure to catfish serum. 3. Catfish ACP induced a temporal sequence of pre-killing and killing phases. 4. Loss of cell viability, killing rate and cytoplasmic enzyme release increased with increasing serum concentrations. 5. By incubating E. coli with sera treated to remove complement, both release of cytoplasmic enzyme and bactericidal activity were eliminated. 6. Lethal activity associated with channel catfish ACP against Gram-negative bacteria was functionally comparable to that seen in mammalian and reptilian systems.

Published
1990
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31. Comparison of the microagglutination test with bactericidal response to Legionella pneumophila (Legionnaires disease bacterium).

Author

Smalley DL and Ourth DD

Subjects
Agglutination Tests, Bacteria growth & development, Legionnaires' Disease immunology, Antibodies, Bacterial immunology, Blood Bactericidal Activity, Legionnaires' Disease microbiology
Abstract

This investigation found that individuals with microagglutination antibody titers of 1:32 or greater to Legionella pneumophila produced bactericidal activity against the bacterium. Those individuals with microagglutination antibody titers of 1:16 or less demonstrated no bactericidal activity.

Published
1980
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32. Legionnaires' disease bacterium: a non-endospore-former.

Author

Smalley DL, Ourth DD, and Hollis CG

Subjects
Bacteria analysis, Humans, Microscopy, Electron, Scanning, Picolinic Acids analysis, Bacteria ultrastructure, Legionnaires' Disease microbiology
Abstract

This investigation was done to determine whether dipicolinic acid was present in the Legionnaires' disease bacterium. A colorimetric assay for dipicolinic acid was done and the results for the bacterium were compared with those obtained for Escherichia coli and Bacillus subtilis. Dipicolinic acid was not detected in the Legionnaires' disease bacterium. This demonstrated that the bacterium was unable to produce typical bacterial endospores under the experimental conditions examined.

Published
1980
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33. Cell-mediated hypersensitivity in guinea-pigs infected with toxoplasms gondii.

Author

Ourth DD, Lunde MN, and Watson RR

Subjects
Animals, Cell Migration Inhibition, Guinea Pigs, Hemagglutination Tests, Lymphocyte Activation, Macrophages, Methylene Blue, Skin Tests, Toxoplasma immunology, Hypersensitivity, Delayed immunology, Immunity, Cellular, Toxoplasmosis immunology
Abstract

This investigation demonstrated delayed hypersensitivity by macrophage migration inhibition (MMI) and skin-testing (ST) at 4, 8, 12, and 17 weeks and by lymphocyte transformation (LT) at 4, 12, and 17 weeks after infection of guinea-pigs (GP) with Toxoplasma gondii (C-37 strain). MMI and LT were both most pronounced at 4 and 17 weeks post-infection. GP immunized with toxoplasmin in complete Freund's adjuvant (CFA) demonstrated positive blast transformation and ST, but GP immunized with phosphate buffered saline in CFA did not. MMI was demonstrated with both immunizing preparations. Positive dye test and indirect hemagglutination test titers from 4 through 17 weeks were found.

Published
1976

34. Alternate pathway of complement and bactericidal response of the channel catfish to Salmonella paratyphi.

Author

Ourth DD and Wilson EA

Subjects
Ammonium Hydroxide, Animals, Edetic Acid pharmacology, Hot Temperature, Hydroxides pharmacology, Immunity, Innate, Molecular Weight, Oximes pharmacology, Phenols pharmacology, Blood Bactericidal Activity, Complement Activation, Complement Pathway, Alternative drug effects, Fishes immunology, Salmonella paratyphi A immunology
Abstract

Fresh channel catfish (Ictalurus punctatus) serum from unimmunized catfish exhibited 100% bactericidal activity against Salmonella paratyphi. Components responsible for bactericidal activity could be absorbed from the fresh catfish serum with S. paratyphi. The bactericidal system of the fresh catfish serum showed a need for magnesium rather than for calcium after EDTA treatment. The addition of salicylaldoxime or ammonium hydroxide to catfish serum indicated the alternate rather than the classical pathway of complement activation to be important in bactericidal activity against S. paratyphi. Bactericidal activity of catfish serum was labile when incubated at 47 degrees C for 30 min., stable for at least 4 mo. at -80 degrees C and could be absorbed with S. paratyphi at 25 degrees C. Very minimal bactericidal activity was present in the descending portion of the first 13.7S peak with most activity being found in the descending portion of the second 7.1S peak and throughout the entire 3.4S peak after Sephadex G-200 catfish serum fractionation.

Published
1982
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36. Immunological nonidentity of Pseudomonas paucimobilis with Pseudomonas aeruginosa and Pseudomonas cepacia.

Author

Smalley DL and Ourth DD

Subjects
Agglutination Tests, Animals, Immunization, Immunodiffusion, Immunoglobulin G biosynthesis, Immunoglobulin M biosynthesis, Rabbits, Species Specificity, Antibodies, Bacterial biosynthesis, Blood Bactericidal Activity, Pseudomonas immunology, Pseudomonas aeruginosa immunology
Abstract

This investigation determined the serum agglutination activity and serum bactericidal response after rabbit immunization with Pseudomonas paucimobilis. Agglutination activity of antisera showed a twofold increase in titer from before immunization to 4 weeks post-immunization and peaked at 8 weeks post-immunization with a titer of 1:512. 2-Mercaptoethanol reduction of immunoglobulin M decreased agglutination titers. No major antigens were found to be common from crude antigen preparations of P. paucimobilis, Pseudomonas aeruginosa and Pseudomonas cepacia when tested with antisera to P. paucimobilis. Serum bactericidal activity was found in post-immunization antisera at 8 and 12 weeks against P. paucimobilis, with no activity present before immunization or at 4 weeks post-immunization. Antisera against P. paucimobilis showed no bactericidal activity against P. aeruginosa or P. cepacia.

Published
1980
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38. Bactericidal serum response of the channel catfish against Gram-negative bacteria.

Author

Ourth DD and Wilson EA

Subjects
Aeromonas, Animals, Bacterial Infections etiology, Bacterial Infections immunology, Bacterial Infections microbiology, Complement Pathway, Alternative, Fish Diseases etiology, Fish Diseases immunology, Fish Diseases microbiology, Furunculosis etiology, Furunculosis immunology, Pseudomonas, Pseudomonas fluorescens, Salmonella paratyphi A, Blood Bactericidal Activity, Fishes microbiology
Published
1982
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39. An indirect immunofluorescent test for human antibodies to tetanus toxoid using an insoluble toxoid as antigen.

Author

Ourth DD, Murray ES, MacDonald AB, and Spielman JM

Subjects
Absorption, Animals, Antigens, Humans, Microscopy, Fluorescence, Neutralization Tests, Rabbits, Antibodies analysis, Fluorescent Antibody Technique methods, Tetanus Toxoid
Abstract

An indirect fluorescent antibody (FA) test for detection of human antibodies to tetanus toxoid is described using an ethylchloroformate-prepared polymer of tetanus toxoid as the particulate slide test antigen. Titres of the FA test were compared with those obtained with the toxin neutralization (TN) test in mice. No antisera were FA-positive at less than 0-0025 AU/ml. Positive correlation of the FA test with the TN test was 50% between 0-0025 and 0-01 antitoxin units/ml (AU/ml) and 100% between 0-02 and 160 AU/ml. In general, an increase in FA titres correlated with an increase in TN titres beginning at about 0-08-0-16 AU/ml.

Published
1975

40. Bactericidal antibody response to Pseudomonas aeruginosa by adults with urinary tract infections.

Author

Smalley DL and Ourth DD

Subjects
Adult, Aged, Bacteriolysis, Female, Humans, Male, Middle Aged, Antibodies, Bacterial biosynthesis, Blood Bactericidal Activity, Pseudomonas Infections immunology, Pseudomonas aeruginosa immunology, Urinary Tract Infections immunology
Abstract

In this investigation we found that adults with upper urinary tract infections caused by Pseudomonas aeruginosa produced serum antibodies with bactericidal activity against the bacterium. Seventeen of 20 infected adults showed bactericidal activity with a titer range of 1:10 to 1:10,000.

Published
1979
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44. Neutralization of bacterial exotoxin (tetanus toxin) by catfish IgM antibody.

Author

Ourth DD

Subjects
Animals, Chromatography, Gel, Hemagglutination Tests, Tetanus Toxoid immunology, Fishes immunology, Immunoglobulin M immunology, Tetanus Toxin immunology
Abstract

A bacterial exotoxin neutralization response by fish EgM antibody has not been demonstrated previously in any fish species. Channel catfish, Ictalurus punctatus, were immunized intraperitoneally with alum-adsorbed tetanus toxoid. Catfish immune serum demonstrated 1.28 antitoxin units (a.u.) of antitoxin neutralization and gave an indirect haemagglutination (IHA) titre of 1:65,536. After 2-mercaptoethanol (2ME) reduction of immune serum, no antitoxin neutralization remained by an IHA serum titre of 1:4096 was present. After Sephadex G-200 gel filtration of the catfish immune serum, the 14S antibody gave 0.32 a.u./ml and an IHA titre of 1:256. The 7S antibody gave no antitoxin neutralization but an IHA titre of 1.512 was found. After 2ME reduction, neither the 14S or 7S globulins demonstrated antitoxin neutralization, but minimal IHA titres of 1:16 and 1:4, respectively, were still found. The catfish immune serum and the 14S and 7S globulins did not precipitate tetanus toxoid by immunodiffusion in 1% agar gel.

Published
1982

45. Calmodulin activity in whole body and fat body tissue extracts of Heliothis virescens larvae.

Author

Lockey TD and Ourth DD

Subjects
Adipose Tissue metabolism, Animals, Calmodulin metabolism, Lepidoptera metabolism
Abstract

Calmodulin is an activator of many enzymatic activities. Total calmodulin activity in tissue extracts of Heliothis virescens larvae (5th instar), assayed by cyclic phosphodiesterase activation, was 0.48 unit/gm for whole body and 22.2 units/gm for fat body. Specific calmodulin activity was 0.1 unit/mg protein for whole body and 3.0 units/mg protein for fat body. The larval fat body is therefore the main site of calmodulin activity in this lepidopterous larva.

Published
1989
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46. Seroepidemiology of Legionella pneumophila. A study of adults from Memphis, Tennessee, U. S. A.

Author

Smalley DL and Ourth DD

Subjects
Age Factors, Aged, Agglutination Tests, Female, Humans, Male, Middle Aged, Tennessee, Antibodies, Bacterial analysis, Legionella immunology
Abstract

Sera of 1,000 adults (aged 50 to 104) from Memphis, Tennessee were tested by the microagglutination procedure for antibodies to Legionella pneumophila (Philadelphia 1 strain). Of the 1,000 sera tested, 53 (5.3%) had titers of 1:16 or greater to L. pneumophila.

Published
1981
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48. Isolation and molecular weight determination of two immunoglobulin heavy chains in the channel catfish, Ictalurus punctatus.

Author

Phillips JO and Ourth DD

Subjects
Animals, Electrophoresis, Polyacrylamide Gel, Hemagglutination Tests, Molecular Weight, Catfishes immunology, Ictaluridae immunology, Immunoglobulin Heavy Chains isolation & purification
Abstract

Channel catfish (Ictalurus punctatus), a teleost fish, were immunized over a 4 month period with 4 intraperitoneal injections of bovine serum albumin (BSA) in Freund's adjuvant. The catfish anti-BSA antibody was purified by affinity chromatography and subjected to sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE). By elution of catfish anti-BSA antibody from BSA-affinity columns with 3.0 M KSCN and subsequent SDS-PAGE, two immunoglobulin heavy chains were demonstrated in the channel catfish. The molecular weights and the relative percentages found of the two immunoglobulin heavy chains were 72,000 (94%) and 56,000 (6%). The molecular weight of the single light chain found was 23,000. Using the 72,000 mol. wt heavy chain and 23,000 mol. wt light chain and including a molecular weight of 15,000 for the J-chain, the molecular weight of the predominant channel catfish tetrameric IgM immunoglobulin molecule was calculated to be 775,000. Using the 56,000 low mol. wt heavy chain, the molecular weight of a second subclass of the channel catfish tetrameric IgM molecule was calculated to be 647,000. After Sephadex G-200 gel filtration, anti-BSA antibody activity was found only in the 14S globulin fraction by indirect hemagglutination testing.

Published
1986
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49. Bacterial sialic acid modulates activation of the alternative complement pathway of channel catfish (Ictalurus punctatus).

Author

Ourth DD and Bachinski LM

Subjects
Animals, Bacteria pathogenicity, Blood Bactericidal Activity, N-Acetylneuraminic Acid, Neuraminidase pharmacology, Sialic Acids analysis, Bacteria analysis, Catfishes immunology, Complement Activation drug effects, Complement Pathway, Alternative drug effects, Ictaluridae immunology, Sialic Acids pharmacology
Abstract

The alternative complement pathway (ACP) provides the non-immune channel catfish (Ictalurus punctatus) with protection against many Gram-negative bacteria. Very little serum bactericidal activity (0-13%) was found against 8 fish pathogens, but a strong bactericidal response (100%) was found against 7 non-pathogens. MgEGTA chelation of catfish serum did not essentially change the bactericidal results. Catfish serum heated at 56 degrees C and serum adsorbed with zymosan had no bactericidal activity. This demonstrated that the ACP was responsible for the bactericidal response. The molecular nature of the microbial surface determines whether or not the ACP will be activated. A relative lack of surface sialic acid has been found to be important for binding complement Factor B of the ACP by susceptible microbial surfaces. This study therefore examined the 15 Gram-negative bacterial fish pathogens and non-pathogens by determining their sialic acid content and their ability to elicit a bactericidal response by the catfish ACP. It was found that there was very little bactericidal activity against the fish pathogens that contained sialic acid but a very strong bactericidal response (100%) against the non-pathogens that lacked sialic acid (p = .0043). A relative lack of sialic acid or no sialic acid therefore correlated with a strong bactericidal response by the catfish ACP. Neuraminidase treatment of the bacterial fish pathogens to remove sialic acid greatly increased the bactericidal response against them by the catfish ACP when compared with untreated bacteria (p = .0431).

Published
1987
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50. Neutralization of tetanus toxin by human and rabbit immunoglobulin classes and subunits.

Author

Ourth DD and MacDonald AB

Subjects
Animals, Antigen-Antibody Reactions, Binding Sites, Antibody, Hemagglutination Tests, Humans, Immunoglobulin Fab Fragments, Immunoglobulin M, Rabbits, Tetanus Toxoid, Immunoglobulin G, Tetanus Antitoxin, Tetanus Toxin
Abstract

This investigation found that the human antibody class of importance in neutralizing tetanus toxin in mice was IgG, and that toxin neutralization was retained by the F(ab')2 and Fab' subunits of the human IgG class. Although human IgM and IgA classes appeared to neutralize tetanus toxin at very low levels, evidence was obtained that this neutralization was probably due to IgG contamination. Human Fabmu isolated from the IgM class did not neutralize tetanus toxin. Human antibodies of the IgG, IgM and IgA classes reacted with tetanus toxoid in the indirect haemagglutination (HA) test with IgG giving the highest HA titre. Rabbit antibodies of the IgG class also neutralized tetanus toxin, with neutralization being retained by the F(ab')2 and Fab' subunits of the rabbit IgG class. Absorption of several rabbit antisera to tetanus toxoid with goat-antirabbit Fc which is specific for absorption of IgG from antiserum, rendered them incapable of neutralizing tetanus toxin.

Published
1977

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