Your search keyword '"Clinkenbeard KD"' showing total 63 results

1. [21] Cytosolic acetoacetyl-CoA thiolase from chicken liver

Author

Lane, Clinkenbeard Kd, and Sugiyama T

Subjects

chemistry.chemical_classification, ATP synthase, biology, Thiolase, Stereochemistry, Cleavage (embryo), Divalent, Cytosol, Enzyme, chemistry, Biochemistry, biology.protein, Specific activity, Magnesium ion

Abstract

Publisher Summary This chapter discusses the determination of cytosolic acetoacetyl-CoA thiolase from chicken liver. Cytosolic acetoacetyl-CoA thiolase catalyzes the reversible thiolytic cleavage of acetoacetyl-CoA by CoA to yield two molecules of acetyl-CoA. It has been demonstrated that the 3-hydroxy-3-methylglutaryl-CoA necessary for hepatic cholesterogenesis is synthesized in the cytoplasmic cell compartment from acetyl-CoA by the actions of two cytosolic enzymes: aetoacetyl-CoA thiolase and 3-hydroxy-3-methylglutaryl-CoA synthase. Thiolase activity is most conveniently determined in the direction of thiolytic cleavage by following the CoA-dependent disappearance of acetoacetyl-CoA using a modification of the assay developed by Stern. Thiolase-catalyzed formation of acetoacetyl-CoA from acetyl-CoA can be measured spectrophotometrically at 303 nm in the presence of divalent magnesium ion at pH 8.8. The latter mentioned factors promote enolization of acetoacetyl-CoA thereby enhancing its extinction coefficient and shifting the otherwise unfavorable equilibrium more toward condensation. One unit of thiolase catalyzes the CoA-dependent cleavage of 1 μmole of acetoacetyl-CoA per minute. Specific activity is expressed in units per milligram of protein.

Published

1975

2. Intracellular localization of the 3-hydroxy-3-methylglutaryl coenzme A cycle enzymes in liver. Separate cytoplasmic and mitochondrial 3-hydroxy-3-methylglutaryl coenzyme A generating systems for cholesterogenesis and ketogenesis.

Author

Clinkenbeard, KD, primary, Reed, WD, additional, Mooney, RA, additional, and Lane, MD, additional

Published

1975

3. Lyophilization of Bdellovibrio bacteriovorus 109J for Long-Term Storage.

Author

Boileau MJ, Mani R, and Clinkenbeard KD

Subjects

Bdellovibrio bacteriovorus growth & development, Bdellovibrio bacteriovorus physiology, Freeze Drying methods, Preservation, Biological methods

Abstract

Bdellovibrio bacteriovorus 109J is a Gram-negative predatory bacterium with obligate host dependency on other Gram-negative bacteria. This bacteriolytic predator collides with, enters, and establishes growth within the prey (host) periplasm, eventually lysing the prey cell wall to release fresh, motile B. bacteriovorus progeny. Laboratory maintenance of B. bacteriovorus has been previously described by other investigators. The protocols included in this unit deal with the technique required to lyophilize or freeze dry host-dependent B. bacteriovorus. This is an alternative means to frozen glycerol stocks for the long-term storage of B. bacteriovorus. It includes the cultivation process and methods to lyophilize B. bacteriovorus as well as recommended storage conditions. In addition, this unit provides insight on the formulation's shelf-life including the time to active culture after reviving lyophilized stocks of B. bacteriovorus following short-, medium-, and long-term storage. © 2017 by John Wiley & Sons, Inc., (Copyright © 2017 John Wiley & Sons, Inc.)

Published

2017

4. Efficacy of Bdellovibrio bacteriovorus 109J for the treatment of dairy calves with experimentally induced infectious bovine keratoconjunctivitis.

Author

Boileau MJ, Mani R, Breshears MA, Gilmour M, Taylor JD, and Clinkenbeard KD

Subjects

Animals, Cattle, Cattle Diseases microbiology, Conjunctivitis, Bacterial microbiology, Conjunctivitis, Bacterial therapy, Cornea, Keratoconjunctivitis therapy, Keratoconjunctivitis, Infectious microbiology, Male, Moraxella bovis, Moraxellaceae Infections microbiology, Moraxellaceae Infections therapy, Vaccination veterinary, Bdellovibrio bacteriovorus, Cattle Diseases therapy, Conjunctivitis, Bacterial veterinary, Keratoconjunctivitis veterinary, Moraxellaceae Infections veterinary

Abstract

OBJECTIVE To determine the efficacy of Bdellovibrio bacteriovorus 109J for the treatment of calves with experimentally induced infectious bovine keratoconjunctivitis (IBK). ANIMALS 12 healthy dairy calves. PROCEDURES For each calf, a grid keratotomy was performed on both eyes immediately before inoculation with Moraxella bovis hemolytic strain Epp63-300 (n = 11 calves) or nonhemolytic strain 12040577 (1 calf). For each calf inoculated with M bovis Epp63-300, the eyes were randomly assigned to receive an artificial tear solution with (treatment group) or without (control group) lyophilized B bacteriovorus 109J. Six doses of the assigned treatment (0.2 mL/eye, topically, q 48 h) were administered to each eye. On nontreatment days, eyes were assessed and corneal swab specimens and tear samples were collected for bacterial culture. Calves were euthanized 12 days after M bovis inoculation. The eyes were harvested for gross and histologic evaluation and bacterial culture. RESULTS The calf inoculated with M bovis 12040577 did not develop corneal ulcers. Of the 22 eyes inoculated with M bovis Epp63-300, 18 developed corneal ulcers consistent with IBK within 48 hours after inoculation; 4 of those eyes developed secondary corneal ulcers that were not consistent with IBK. Corneal ulcer size and severity and the time required for ulcer healing did not differ between the treatment and control groups. CONCLUSIONS AND CLINICAL RELEVANCE Results suggested that B bacteriovorus 109J was not effective for the treatment of IBK; however, the experimental model used produced lesions that did not completely mimic naturally occurring IBK.

Published

2016

5. Ecology of Tularemia in Central US Endemic Region.

Author

Mani RJ, Morton RJ, and Clinkenbeard KD

Abstract

Tularemia is a zoonotic disease that occurs in the Northern Hemisphere caused by the gammabacterium Francisella tularensis . The most severe form of human tularemia occurs in the central USA and involves a rabbit enzootic cycle, ixodid tick vectors, and F. tularensis subspecies tularensis genotype A1. Enzootic tularemia is thought to have a spring-summer seasonality corresponding to the questing activity of its primary tick vectors. Domestic cats, another common incidental host, acquire the infection by preying on infected rabbits. The seasonality of tularemia in cats, which demonstrate a bimodal seasonal incidence curve with peaks in the spring and late summer-fall, may serve as a surrogate for the seasonality of the disease in its enzootic host. Human tularemia shows a unimodal late spring, early summer peak, which correlates to the seasonal questing activity of tick vectors of human tularemia. This difference in seasonality suggests that different tick species or tick life stages are involved in maintenance of the enzootic rabbit-tick cycle.

Published

2016

6. Role of Tellurite Resistance Operon in Filamentous Growth of Yersinia pestis in Macrophages.

Author

Ponnusamy D and Clinkenbeard KD

Subjects

Animals, Bacterial Proteins genetics, Cells, Cultured, Genetic Complementation Test, Immunity, Innate genetics, Mice, Plague drug therapy, Plague genetics, Virulence genetics, Yersinia pestis drug effects, Drug Resistance, Bacterial genetics, Gene Expression Regulation, Bacterial, Macrophages microbiology, Operon genetics, Plague microbiology, Tellurium pharmacology, Yersinia pestis pathogenicity

Abstract

Background: Yersinia pestis initiates infection by parasitism of host macrophages. In response to macrophage infections, intracellular Y. pestis can assume a filamentous cellular morphology which may mediate resistance to host cell innate immune responses. We previously observed the expression of Y. pestis tellurite resistance proteins TerD and TerE from the terZABCDE operon during macrophage infections. Others have observed a filamentous response associated with expression of tellurite resistance operon in Escherichia coli exposed to tellurite. Therefore, in this study we examine the potential role of Y. pestis tellurite resistance operon in filamentous cellular morphology during macrophage infections., Principal Findings: In vitro treatment of Y. pestis culture with sodium tellurite (Na2TeO3) caused the bacterial cells to assume a filamentous phenotype similar to the filamentous phenotype observed during macrophage infections. A deletion mutant for genes terZAB abolished the filamentous morphologic response to tellurite exposure or intracellular parasitism, but without affecting tellurite resistance. However, a terZABCDE deletion mutant abolished both filamentous morphologic response and tellurite resistance. Complementation of the terZABCDE deletion mutant with terCDE, but not terZAB, partially restored tellurite resistance. When the terZABCDE deletion mutant was complemented with terZAB or terCDE, Y. pestis exhibited filamentous morphology during macrophage infections as well as while these complemented genes were being expressed under an in vitro condition. Further in E. coli, expression of Y. pestis terZAB, but not terCDE, conferred a filamentous phenotype., Conclusions: These findings support the role of Y. pestis terZAB mediation of the filamentous response phenotype; whereas, terCDE confers tellurite resistance. Although the beneficial role of filamentous morphological responses by Y. pestis during macrophage infections is yet to be fully defined, it may be a bacterial adaptive strategy to macrophage associated stresses.

Published

2015

7. Amblyomma americanum as a Bridging Vector for Human Infection with Francisella tularensis.

Author

Mani RJ, Metcalf JA, and Clinkenbeard KD

Subjects

Animals, Female, Humans, Larva genetics, Male, Mice, Mice, Inbred BALB C, Molting genetics, Nymph genetics, Ovary metabolism, Ovary microbiology, Rabbits, Salivary Glands microbiology, Stem Cells, Francisella tularensis, Ixodidae microbiology, Tularemia microbiology, Tularemia transmission

Abstract

The γ-proteobacterium Francisella tularensis causes seasonal tick-transmitted tularemia outbreaks in natural rabbit hosts and incidental infections in humans in the south-central United States. Although Dermacentor variabilis is considered a primary vector for F. tularensis, Amblyomma americanum is the most abundant tick species in this endemic region. A systematic study of F. tularensis colonization of A. americanum was undertaken to better understand its potential to serve as an overwintering reservoir for F. tularensis and as a bridging vector for human infections. Colony-reared A. americanum were artificially fed F. tularensis subspecies holarctica strain LVS via glass capillaries and colonization levels determined. Capillary-fed larva and nymph were initially infected with 10(4) CFU/tick which declined prior to molting for both stages, but rebounded post-molting in nymphs and persisted in 53% at 10(3) to 10(8) CFU/nymph at 168 days post-capillary feeding (longest sampling time in the study). In contrast, only 18% of adults molted from colonized nymphs maintained LVS colonization at 10(1) to 10(5) CFU/adult at 168 days post-capillary feeding (longest sampling time). For adults, LVS initially colonized the gut and disseminated to salivary glands by 24 h and had an ID50 of <5CFU in mice. Francisella tularensis infected the ovaries of gravid females, but transmission to eggs was infrequent and transovarial transmission to hatched larvae was not observed. The prolonged persistence of F. tularensis in A. americanum nymphs supports A. americanum as an overwintering reservoir for F. tularensis from which seasonal epizootics may originate; however, although the rapid dissemination of F. tularensis from gut to salivary glands in adults A. americanum is compatible with intermittent feeding adult males acting as bridging vectors for incidental F. tularensis infections of humans, acquisition of F. tularensis by adults may be unlikely based on adult feeding preference for larger mammals which are not involved in maintenance of sylvatic tularemia.

Published

2015

8. High-throughput screening of a diversity collection using biodefense category A and B priority pathogens.

Author

Barrow EW, Clinkenbeard PA, Duncan-Decocq RA, Perteet RF, Hill KD, Bourne PC, Valderas MW, Bourne CR, Clarkson NL, Clinkenbeard KD, and Barrow WW

Subjects

Bacillus anthracis drug effects, Brucella abortus drug effects, Drug Discovery, Escherichia coli drug effects, Francisella tularensis drug effects, Humans, National Institute of Allergy and Infectious Diseases (U.S.), Staphylococcus aureus drug effects, United States, Yersinia pestis drug effects, Anti-Bacterial Agents pharmacology, Bacteria drug effects, Bioterrorism, High-Throughput Screening Assays methods, Microbial Sensitivity Tests

Abstract

One of the objectives of the National Institutes of Allergy and Infectious Diseases (NIAID) Biodefense Program is to identify or develop broad-spectrum antimicrobials for use against bioterrorism pathogens and emerging infectious agents. As a part of that program, our institution has screened the 10 000-compound MyriaScreen Diversity Collection of high-purity druglike compounds against three NIAID category A and one category B priority pathogens in an effort to identify potential compound classes for further drug development. The effective use of a Clinical and Laboratory Standards Institute-based high-throughput screening (HTS) 96-well-based format allowed for the identification of 49 compounds that had in vitro activity against all four pathogens with minimum inhibitory concentration values of ≤16 µg/mL. Adaptation of the HTS process was necessary to conduct the work in higher-level containment, in this case, biosafety level 3. Examination of chemical scaffolds shared by some of the 49 compounds and assessment of available chemical databases indicates that several may represent broad-spectrum antimicrobials whose activity is based on novel mechanisms of action.

Published

2012

9. Yersinia pestis intracellular parasitism of macrophages from hosts exhibiting high and low severity of plague.

Author

Ponnusamy D and Clinkenbeard KD

Subjects

Animals, Cell Line, Dogs, Female, Macrophages microbiology, Macrophages parasitology, Mice, Intracellular Space microbiology, Intracellular Space parasitology, Macrophages cytology, Plague immunology, Yersinia pestis physiology

Abstract

Background: Yersinia pestis causes severe disease in natural rodent hosts, but mild to inapparent disease in certain rodent predators such as dogs. Y. pestis initiates infection in susceptible hosts by parasitizing and multiplying intracellularly in local macrophages prior to systemic dissemination. Thus, we hypothesize that Y. pestis disease severity may depend on the degree to which intracellular Y. pestis overcomes the initial host macrophage imposed stress., Methodology/principal Findings: To test this hypothesis, the progression of in vitro infection by Y. pestis KIM62053.1+ of mouse splenic and RAW264.7 tissue culture macrophages and dog peripheral blood-derived and DH82 tissue culture macrophages was studied using microscopy and various parameters of infection. The study showed that during the early stage of infection, intracellular Y. pestis assumed filamentous cellular morphology with multiple copies of the genome per bacterium in both mouse and dog macrophages. Later, in mouse macrophages, the infection elicited spacious vacuolar extension of Yersinia containing vacuoles (YCV), and the filamentous Y. pestis reverted to coccobacillary morphology with genomic equivalents approximately equaling colony forming units. In contrast, Y. pestis infected dog macrophages did not show noticeable extension of YCV, and intracellular Y. pestis retained the filamentous cellular morphology for the entire experiment in DH82 cells or were killed by blood-derived macrophages. In addition, during the later stage of infection, Y. pestis infected mouse macrophages exhibited cell lysis whereas dog macrophages did not., Conclusion/significance: Overall, these results support our hypothesis that Y. pestis in mouse macrophages can overcome the initial intracellular stress necessary for subsequent systemic infection. However, in dogs, failure of Y. pestis to overcome macrophage imposed stress may result in mild or in apparent disease in dogs.

Published

2012

10. Biology of Francisella tularensis subspecies holarctica live vaccine strain in the tick vector Dermacentor variabilis.

Author

Mani RJ, Reichard MV, Morton RJ, Kocan KM, and Clinkenbeard KD

Subjects

Animals, Arthropod Vectors growth & development, Dermacentor growth & development, Female, Larva microbiology, Male, Mice, Mice, Inbred BALB C, Nymph microbiology, Oocytes microbiology, Salivary Glands microbiology, Arthropod Vectors microbiology, Dermacentor microbiology, Francisella tularensis physiology, Tularemia transmission

Abstract

Background: The γ-proteobacterium Francisella tularensis is the etiologic agent of seasonal tick-transmitted tularemia epizootics in rodents and rabbits and of incidental infections in humans. The biology of F. tularensis in its tick vectors has not been fully described, particularly with respect to its quanta and duration of colonization, tissue dissemination, and transovarial transmission. A systematic study of the colonization of Dermacentor variabilis by the F. tularensis subsp. holarctica live vaccine strain (LVS) was undertaken to better understand whether D. variabilis may serve as an inter-epizootic reservoir for F. tularensis., Methodology/principal Findings: Colony-reared larva, nymph, and adult D. variabilis were artificially fed LVS via glass capillary tubes fitted over the tick mouthparts, and the level of colonization determined by microbial culture. Larvae and nymphs were initially colonized with 8.8 ± 0.8 × 10(1) and 1.1 ± 0.03 × 10(3) CFU/tick, respectively. Post-molting, a significant increase in colonization of both molted nymphs and adults occurred, and LVS persisted in 42% of molted adult ticks at 126 days post-capillary tube feeding. In adult ticks, LVS initially colonized the gut, disseminated to hemolymph and salivary glands by 21 days, and persisted up to 165 days. LVS was detected in the salivary secretions of adult ticks after four days post intra-hemocoelic inoculation, and LVS recovered from salivary gland was infectious to mice with an infectious dose 50% of 3 CFU. LVS in gravid female ticks colonized via the intra-hemocoelic route disseminated to the ovaries and then to the oocytes, but the pathogen was not recovered from the subsequently-hatched larvae., Conclusions/significance: This study demonstrates that D. variabilis can be efficiently colonized with F. tularensis using artificial methods. The persistence of F. tularensis in D. variabilis suggests that this tick species may be involved in the maintenance of enzootic foci of tularemia in the central United States.

Published

2012

11. Assessment of Bdellovibrio bacteriovorus 109J killing of Moraxella bovis in an in vitro model of infectious bovine keratoconjunctivitis.

Author

Boileau MJ, Clinkenbeard KD, and Iandolo JJ

Subjects

Animals, Bacterial Adhesion, Cattle, Coculture Techniques, Dogs, Keratoconjunctivitis microbiology, Kidney cytology, Bdellovibrio physiology, Cattle Diseases microbiology, Keratoconjunctivitis veterinary, Moraxella bovis physiology

Abstract

The objective of this study was to determine the potential of Bdellovibrio bacteriovorus 109J as an alternative non-chemotherapeutic treatment of infectious bovine keratoconjunctivitis (IBK). To accomplish this, various parameters of B. bacteriovorus predation of Moraxella bovis were determined in vitro. Initial passage of B. bacteriovorus using M. bovis as prey required 10 d for active cultures to develop compared with 2 d for culture on normal Escherichia coli prey; however by the 5th passage, time to active predatory morphology was reduced to 2 d. This high passage B. bacteriovorus culture [1 × 10(10) plaque forming units (PFU)/mL] killed 76% of M. bovis [1 × 10(7) colony forming units (CFU)/mL] present in suspension broth in a 4 h assay. The minimal level of M. bovis supporting B. bacteriovorus predation was 1 × 10(4) CFU/mL. To assess the ability of B. bacteriovorus to kill M. bovis on an epithelial surface mimicking IBK, an in vitro assay with Madin-Darby bovine kidney (MDBK) cells inoculated with 4 × 10(7) CFU/mL M. bovis was used. Treatment with a B. bacteriovorus suspension (1.6 × 10(11) PFU/mL) decreased adherence of M. bovis to MDBK cells by 6-fold at 12 h of treatment, as well as decreased the number of unattached M. bovis cells by 1.4-fold. This study demonstrates that B. bacteriovorus has potential as an effective biological control of M. bovis at levels likely present in IBK-infected corneal epithelia and ocular secretions.

Published

2011

12. Bi-cell surface plasmon resonance detection of aptamer mediated thrombin capture in serum.

Author

Mani RJ, Dye RG, Snider TA, Wang S, and Clinkenbeard KD

Subjects

Humans, Limit of Detection, Serum chemistry, Thrombin metabolism, Aptamers, Nucleotide metabolism, Surface Plasmon Resonance methods, Thrombin analysis

Abstract

The serine protease coagulation factor thrombin functions primarily in hemostasis, but is also involved in atherosclerosis, thromboembolic disease, cancer and inflammatory disease. Direct measurement of coagulation proteins including thrombin in plasma samples poses a significant challenge because of lack of specific probes and low thrombin concentrations. In addition, high plasma protein concentrations in samples can result in high backgrounds. These challenges were overcome using a bi-cell surface plasmon resonance (SPR) spectrometer with an immobilized thrombin aptamer to measure thrombin in samples passed through a low volume flow cell. For thrombin in Tris-EDTA buffer, the limit of detection (LOD) was 25 nM. Coefficient of variation (CV) for detection of 50 nM was 12.2% and 12.4% for intra and inter-day measurements respectively. This detection was specific for both thrombin aptamer and for thrombin. Using serum samples spiked with thrombin, the LOD was 50 nM with a linear range of detection from 50 nM to 200 nM. However use of serum samples was associated with consistent, low-level background drift. The contributions of nonspecific protein absorption onto the sensor surface and sample flow speed were assessed, and strategies to reduce this background drift were explored. We conclude that the bi-cell SPR platform with an aptamer capture probe can be employed as a highly sensitive real-time, label-free biosensor for the detection of coagulation factors in plasma samples., (Copyright © 2011 Elsevier B.V. All rights reserved.)

Published

2011

13. In vitro efficacy of antibiotics commonly used to treat human plague against intracellular Yersinia pestis.

Author

Wendte JM, Ponnusamy D, Reiber D, Blair JL, and Clinkenbeard KD

Subjects

Amoxicillin pharmacology, Animals, Cell Line, Chloramphenicol pharmacology, Ciprofloxacin pharmacology, Doxycycline pharmacology, Gentamicins pharmacology, Humans, Macrophages microbiology, Mice, Microbial Sensitivity Tests, Plague prevention & control, Streptomycin pharmacology, Anti-Bacterial Agents pharmacology, High-Throughput Screening Assays methods, Plague drug therapy, Yersinia pestis drug effects, Yersinia pestis pathogenicity

Abstract

Yersinia pestis initiates infection as a facultative intracellular parasite in host macrophages; however, little is known about the efficacy of antibiotics commonly used to treat human plague against intracellular Y. pestis. Intracellular minimal bactericidal concentrations (MBCs) were determined using a high-throughput broth microdilution assay in which human THP-1 macrophage-like cells were infected with Y. pestis strain KIM6-2053.1+ and exposed to 2-fold serial dilutions of antibiotics for 24 h in 96-well plates. The numbers of CFU, upon which minimal bactericidal concentrations were based, were determined by counting "microcolonies" in wells of 96-well plates following lysis of tissue culture cells to release surviving Y. pestis, replica dilution, and plating in soft tryptic soy broth agar. For THP-1 cells, streptomycin and ciprofloxacin had comparable efficacies for intra- and extracellular Y. pestis, but the MBCs for chloramphenicol, gentamicin, doxycycline, and amoxicillin were two-, three-, four-, and five 2-fold serial dilutions greater, respectively, for intracellular than for extracellular Y. pestis. During the initial stage of plague, intracellular Y. pestis may be less susceptible to antibiotic killing by particular antibiotics recommended for treatment of plague, such as gentamicin or doxycycline, whereas others, such as streptomycin and ciprofloxacin, may have similar efficacies against extracellular or intracellular Y. pestis. This may be of particular importance in the selection of antibiotics for prophylactic treatment in the case of a bioterrorism event.

Published

2011

14. Intracellular Yersinia pestis expresses general stress response and tellurite resistance proteins in mouse macrophages.

Author

Ponnusamy D, Hartson SD, and Clinkenbeard KD

Subjects

Animals, Bacterial Proteins genetics, Cell Line, Electrophoresis, Gel, Two-Dimensional, Mice, Phagosomes microbiology, Yersinia pestis genetics, Bacterial Proteins metabolism, Macrophages microbiology, Proteomics, Yersinia pestis physiology

Abstract

Yersinia pestis inoculated subcutaneously via fleabite or experimental injection in natural rodent hosts multiply initially in macrophage phagolysosomes. Survival and multiplication of Y. pestis in this acidic low [Ca(2+)] and [Mg(2+)] environment likely necessitates compensatory mechanisms involving expression of specific proteins compared to those expressed during extracellular growth. A proteomics approach was used to identify these proteins using mouse macrophage RAW264.7 cells infected with Y. pestis strain KIM6-2053.1+ for 8h. Intracellular Y. pestis protein samples were prepared by detergent lysis of infected RAW264.7 cells, isolation of intracellular Y. pestis by differential centrifugation, and sonication of isolated Y. pestis. Protein samples were similarly prepared from Y. pestis grown extracellularly in tissue culture media. Two intracellular and extracellular Y. pestis protein samples were analyzed by two-dimensional polyacrylamide gel electrophoresis and compared in silico identifying 12 protein spots present in both intracellular samples but absent in extracellularly grown Y. pestis. Mass spectrometry analysis of these identified nine proteins at a high level of confidence in the Y. pestis genome: superoxide dismutase-A (sodA), inorganic pyrophosphatase, autonomous glycyl radical cofactor GrcA, molecular chaperone DnaK, serine endoprotease GsrA, global DNA-binding transcriptional dual regulator H-NS, urease subunit gamma UreA, and tellurite resistance proteins TerD and TerE. These results support the involvement of various general stress response regulators of Y. pestis during the intracellular parasitism of host macrophages as well as identification of UreA, TerD and TerE with as yet unknown roles in the process of intracellular survival of Y. pestis., (Copyright © 2011 Elsevier B.V. All rights reserved.)

Published

2011

15. E. coli O157:H7 catabolism of intestinal mucin-derived carbohydrates and colonization.

Author

Snider TA, Fabich AJ, Conway T, and Clinkenbeard KD

Subjects

Animals, Biopsy veterinary, Cattle, Cattle Diseases metabolism, Colony Count, Microbial veterinary, Escherichia coli Infections metabolism, Escherichia coli Infections microbiology, Escherichia coli O157 growth & development, Feces microbiology, Female, Histocytochemistry veterinary, Intestinal Diseases metabolism, Intestinal Diseases microbiology, Intestinal Mucosa metabolism, Intestinal Mucosa microbiology, Male, Acetylgalactosamine metabolism, Cattle Diseases microbiology, Escherichia coli Infections veterinary, Escherichia coli O157 metabolism, Fucose metabolism, Intestinal Diseases veterinary

Abstract

E. coli O157:H7 colonizes the bovine intestine, can contaminate food through fecal shedding, and causes human diarrheal and systemic illnesses. Catabolism of particular carbohydrates by E. coli has been found to be important for intestinal colonization of mice. In this study, we assessed whether catabolism of two mucin-derived carbohydrates are important for E. coli O157:H7 colonization of adult cattle. This was accomplished by competitively co-colonizing streptomycin-treated adult cattle with a wild-type strain of E. coli O157:H7 and isogenic mutants in catabolic pathways for mucin-derived carbohydrates N-acetylgalactosamine or l-fucose. Both mutants colonized poorly compared to the wild-type during the initiation stage of colonization (days 0-6). During the maintenance stage of colonization (days 7-15), the mutant unable to use N-acetylgalactosamine did not show a colonization defect, whereas the strain unable to use fucose had a significant colonization defect. These results support the concept that growth and colonization of E. coli O157:H7 in the bovine rectum has a nutritional basis, with a nutrient preference for l-fucose over N-acetylgalactosamine.

Published

2009

16. Mannheimia haemolytica serotype A1 exhibits differential pathogenicity in two related species, Ovis canadensis and Ovis aries.

Author

Dassanayake RP, Shanthalingam S, Herndon CN, Lawrence PK, Frances Cassirer E, Potter KA, Foreyt WJ, Clinkenbeard KD, and Srikumaran S

Subjects

Animals, Pasteurellosis, Pneumonic pathology, Sheep Diseases pathology, Species Specificity, Mannheimia haemolytica classification, Mannheimia haemolytica pathogenicity, Pasteurellosis, Pneumonic microbiology, Sheep Diseases microbiology, Sheep, Bighorn, Sheep, Domestic

Abstract

Mannheimia haemolytica causes pneumonia in both bighorn sheep (BHS, Ovis canadensis) and domestic sheep (DS, Ovis aries). Under experimental conditions, co-pasturing of BHS and DS results in fatal pneumonia in BHS. It is conceivable that certain serotypes of M. haemolytica carried by DS are non-pathogenic to them, but lethal for BHS. M. haemolytica serotypes A1 and A2 are carried by DS in the nasopharynx. However, it is the serotype A2 that predominantly causes pneumonia in DS. The objectives of this study were to determine whether serotype A1 exhibits differential pathogenicity to BHS and DS, and to determine whether leukotoxin (Lkt) secreted by this organism is its primary virulence factor. Three groups each of BHS and DS were intra-tracheally administered either 1 x 10(9)cfu of serotype A1 wild-type (lktA-Wt group), Lkt-deletion mutant of serotype A1-(lktA-Mt group), or saline (control group), respectively. In the lktA-Wt groups, all four BHS died within 48h while none of the DS died during the 2-week study period. In the lktA-Mt groups, none of the BHS or DS died. In the control groups, one DS died due to an unrelated cause. Necropsy and histopathological findings revealed that death of BHS in the lktA-Wt group was due to bilateral, fibrinohemorrhagic pneumonia. Although the A1-Mt-inoculated BHS were clinically normal, on necropsy, lungs of two BHS showed varying degrees of mild chronic pneumonia. These results indicate that M. haemolytica serotype A1 is non-pathogenic to DS, but highly lethal to BHS, and that Lkt is the primary virulence factor of M. haemolytica.

Published

2009

17. Disseminated histoplasmosis in an African pygmy hedgehog.

Author

Snider TA, Joyner PH, and Clinkenbeard KD

Subjects

Animals, Anti-Bacterial Agents therapeutic use, Antifungal Agents therapeutic use, Diagnosis, Differential, Fatal Outcome, Female, Histoplasma pathogenicity, Histoplasmosis diagnosis, Histoplasmosis drug therapy, Histoplasmosis pathology, Air Microbiology, Hedgehogs, Histoplasma isolation & purification, Histoplasmosis veterinary

Abstract

Case Description: A 2-year-old captive-bred sexually intact female African pygmy hedgehog (Atelerix albiventris) was evaluated because of vague signs of illness including inappetence, weakness, lethargy, and weight loss over a 20-day period., Clinical Findings: Abnormalities detected via initial clinicopathologic analyses included anemia, thrombocytopenia, leukopenia, hypoproteinemia, and hypoglycemia. Results of a fecal flotation test were negative. Three weeks after the initial evaluation, splenomegaly was detected via palpation and ultrasonography., Treatment and Outcome: The hedgehog was treated with broad-spectrum antibacterial agents, resulting in an initially favorable response. Fenbendazole was also administered against possible occult parasitic infestation. After 3 weeks of illness, the hedgehog's condition had worsened and supportive care and administration of additional antibacterial agents were instituted. The hedgehog died, and pathologic examinations revealed severe splenomegaly; granulomatous infiltrates were evident in multiple organs, and Histoplasma capsulatum yeasts were detected intralesionally., Clinical Relevance: Histoplasmosis can develop in a wide range of mammalian species. African pygmy hedgehogs are becoming increasingly popular as exotic pets, and vague signs of illness and splenomegaly are often attributed to hemolymphatic malignancies, which are somewhat common in this species. Practitioners should be aware that similar clinical signs may be associated with histoplasmosis in these animals. Although the hedgehog of this report was confined indoors, it originated from an area where histoplasmosis was endemic; this indicates that the disease should be included as a differential diagnosis for hedgehogs that develop vague signs of illness and are known to originate from such geographic regions.

Published

2008

18. Paradoxical DNA repair and peroxide resistance gene conservation in Bacillus pumilus SAFR-032.

Author

Gioia J, Yerrapragada S, Qin X, Jiang H, Igboeli OC, Muzny D, Dugan-Rocha S, Ding Y, Hawes A, Liu W, Perez L, Kovar C, Dinh H, Lee S, Nazareth L, Blyth P, Holder M, Buhay C, Tirumalai MR, Liu Y, Dasgupta I, Bokhetache L, Fujita M, Karouia F, Eswara Moorthy P, Siefert J, Uzman A, Buzumbo P, Verma A, Zwiya H, McWilliams BD, Olowu A, Clinkenbeard KD, Newcombe D, Golebiewski L, Petrosino JF, Nicholson WL, Fox GE, Venkateswaran K, Highlander SK, and Weinstock GM

Subjects

Bacillus drug effects, Bacillus radiation effects, Gamma Rays, Genes, Bacterial, Genome, Bacterial, Oxidative Stress, Sequence Analysis, DNA, Spores, Bacterial drug effects, Spores, Bacterial genetics, Spores, Bacterial radiation effects, Ultraviolet Rays, Bacillus genetics, DNA Repair, Drug Resistance, Bacterial genetics, Hydrogen Peroxide pharmacology

Abstract

Background: Bacillus spores are notoriously resistant to unfavorable conditions such as UV radiation, gamma-radiation, H2O2, desiccation, chemical disinfection, or starvation. Bacillus pumilus SAFR-032 survives standard decontamination procedures of the Jet Propulsion Lab spacecraft assembly facility, and both spores and vegetative cells of this strain exhibit elevated resistance to UV radiation and H2O2 compared to other Bacillus species., Principal Findings: The genome of B. pumilus SAFR-032 was sequenced and annotated. Lists of genes relevant to DNA repair and the oxidative stress response were generated and compared to B. subtilis and B. licheniformis. Differences in conservation of genes, gene order, and protein sequences are highlighted because they potentially explain the extreme resistance phenotype of B. pumilus. The B. pumilus genome includes genes not found in B. subtilis or B. licheniformis and conserved genes with sequence divergence, but paradoxically lacks several genes that function in UV or H2O2 resistance in other Bacillus species., Significance: This study identifies several candidate genes for further research into UV and H2O2 resistance. These findings will help explain the resistance of B. pumilus and are applicable to understanding sterilization survival strategies of microbes.

Published

2007

19. Evaluation of a model for Escherichia coli O157:H7 colonization in streptomycin-treated adult cattle.

Author

Snider TA, Fabich AJ, Washburn KE, Sims WP, Blair JL, Cohen PS, Conway T, and Clinkenbeard KD

Subjects

Animals, Catheterization veterinary, Cattle, Cattle Diseases drug therapy, Colony Count, Microbial veterinary, Duodenum microbiology, Escherichia coli Infections drug therapy, Feces microbiology, Intestinal Mucosa microbiology, Streptomycin therapeutic use, Cattle Diseases microbiology, Disease Models, Animal, Escherichia coli Infections veterinary, Escherichia coli O157

Abstract

Objective: To develop a repeatable model for studying colonization with streptomycin-resistant Escherichia coli O157:H7 in adult cattle., Animals: 5 adult mixed-breed beef cattle., Procedures: Cattle were surgically cannulated in the duodenum, treated daily with streptomycin (33 mg/kg) via the duodenal cannula prior to and during experimental colonizations, and colonized with 10(10) CFUs of streptomycin-resistant E coli O157:H7 via the duodenal cannula. Colonization of rectal mucus and shedding in feces were monitored. Antimicrobials were administered to eliminate the colonizing strain so that 5 repeated colonization experiments could be performed. A comprehensive analysis of colonization was performed at necropsy., Results: Streptomycin treatment resulted in improved experimental colonization variables, compared with untreated controls, during initiation (days 2 to 6) and early maintenance (days 7 to 12) of colonization. Elimination of the colonizing strain followed by 5 repeated colonizations in the same animals indicated the repeatability of the protocol. Positive results of bacteriologic culture of feces 7 and 12 days after colonization were obtained in 100% and 84% of samples, respectively, across all animals and trials. At necropsy, highest magnitude recovery was in terminal rectal mucus., Conclusions and Clinical Relevance: The model was highly repeatable and novel with respect to streptomycin treatment, use of duodenal cannulas, and repeated colonizations of the same animals. Its use in adult cattle, from which most bovine-derived food originates, is critical to the study of preharvest food safety. The findings have implications for understanding intermittency of shedding in the field and for proposed vaccine-based interventions.

Published

2006

20. Chromosome rearrangement and diversification of Francisella tularensis revealed by the type B (OSU18) genome sequence.

Author

Petrosino JF, Xiang Q, Karpathy SE, Jiang H, Yerrapragada S, Liu Y, Gioia J, Hemphill L, Gonzalez A, Raghavan TM, Uzman A, Fox GE, Highlander S, Reichard M, Morton RJ, Clinkenbeard KD, and Weinstock GM

Subjects

DNA Transposable Elements, DNA, Bacterial chemistry, DNA, Bacterial genetics, Evolution, Molecular, Molecular Sequence Data, Pseudogenes, Recombination, Genetic, Sequence Analysis, DNA, Sequence Homology, Virulence genetics, Chromosomes, Bacterial genetics, Francisella tularensis genetics, Gene Rearrangement, Genome, Bacterial, Polymorphism, Genetic

Abstract

The gamma-proteobacterium Francisella tularensis is one of the most infectious human pathogens, and the highly virulent organism F. tularensis subsp. tularensis (type A) and less virulent organism F. tularensis subsp. holarctica (type B) are most commonly associated with significant disease in humans and animals. Here we report the complete genome sequence and annotation for a low-passage type B strain (OSU18) isolated from a dead beaver found near Red Rock, Okla., in 1978. A comparison of the F. tularensis subsp. holarctica sequence with that of F. tularensis subsp. tularensis strain Schu4 (P. Larsson et al., Nat. Genet. 37:153-159, 2005) highlighted genetic differences that may underlie different pathogenicity phenotypes and the evolutionary relationship between type A and type B strains. Despite extensive DNA sequence identity, the most significant difference between type A and type B isolates is the striking amount of genomic rearrangement that exists between the strains. All but two rearrangements can be attributed to homologous recombination occurring between two prominent insertion elements, ISFtu1 and ISFtu2. Numerous pseudogenes have been found in the genomes and are likely contributors to the difference in virulence between the strains. In contrast, no rearrangements have been observed between the OSU18 genome and the genome of the type B live vaccine strain (LVS), and only 448 polymorphisms have been found within non-transposase-coding sequences whose homologs are intact in OSU18. Nonconservative differences between the two strains likely include the LVS attenuating mutation(s).

Published

2006

21. Effects of Mannheimia haemolytica leukotoxin on apoptosis and oncosis of bovine neutrophils.

Author

Cudd LA, Ownby CL, Clarke CR, Sun Y, and Clinkenbeard KD

Subjects

Animals, Cattle, In Vitro Techniques, Microscopy, Electron, Neutrophils pathology, Neutrophils ultrastructure, Staurosporine pharmacology, Time Factors, Apoptosis drug effects, Bacterial Toxins toxicity, Exotoxins toxicity, Mannheimia haemolytica, Neutrophils drug effects

Abstract

Objective: To investigate the concentration-dependent effects of Mannheimia haemolytica (formerly Pasteurella haemolytica) leukotoxin (LKT) on apoptosis and oncosis in bovine neutrophils and to examine the role of calcium ions (Ca2+) in LKT-induced apoptosis., Sample Population: Neutrophils isolated from blood samples obtained from healthy calves., Procedure: Neutrophil suspensions were exposed to lytic or sublytic dilutions of LKT and then examined by use of transmission electron microscopy (TEM) or gel electrophoresis. Contribution of extracellular Ca2+ to LKT-induced apoptosis was investigated by incubating neutrophils with LKT or control solutions in buffer containing 1 mM CaCl2 or in Ca2+-free buffer containing 1 mM ethylene glycol-bis (b-aminoethyl ether)-N,N-tetraacetic acid (EGTA) prior to diphenyl amine analysis., Results: Examination by TEM revealed that bovine neutrophils exposed to lytic dilutions of LKT had changes consistent with oncosis, whereas neutrophils exposed to sublytic dilutions of LKT and staurosporin, an inducer of apoptosis, had changes consistent with apoptosis. Effects of sublytic dilutions of LKT on apoptosis were confirmed by gel electrophoresis. Replacement of extracellular Ca2+ with EGTA, a Ca2+ chelator, reduced apoptosis attributable to the calcium ionophore A23187, but it did not have significant effects on apoptosis induced by LKT or staurosporin., Conclusions and Clinical Relevance: The ability of LKT to cause apoptosis instead of oncosis is concentration-dependent, suggesting that both processes of cell death contribute to an ineffective host-defense response, depending on the LKT concentration in pneumonic lesions. Furthermore, although Ca2+ promotes A23187-induced apoptosis, it is apparently not an essential second messenger for LKT-induced apoptosis.

Published

2001

22. Ultrastructural characterization of apoptosis in bovine lymphocytes exposed to Pasteurella haemolytica leukotoxin.

Author

Sun Y, Clinkenbeard KD, Ownby CL, Cudd L, Clarke CR, and Highlander SK

Subjects

Animals, Apoptosis physiology, Cattle, DNA Fragmentation drug effects, L-Lactate Dehydrogenase analysis, Lymphocytes drug effects, Microscopy, Electron veterinary, Pasteurellosis, Pneumonic physiopathology, Virulence, Apoptosis drug effects, Exotoxins pharmacology, Immunosuppressive Agents pharmacology, Lymphocytes ultrastructure, Mannheimia haemolytica pathogenicity

Abstract

Objective: To characterize ultrastructural changes of bovine lymphocytes exposed to Pasteurella haemolytica leukotoxin (LKT)., Sample Population: Partially purified LKT from a wild type P. haemolytica A1 strain and inactive pro-LKT from an isogeneic mutant Phaemolytica strain. Isolated bovine lymphocytes were obtained from 2 healthy calves., Procedure: Isolated bovine lymphocytes were incubated with various concentrations of LKT and pro-LKT for 3 hours at 37 C and examined by use of transmission electron microscopy. A cytochemical Klenow DNA fragmentation assay was used to examine lymphocytes for DNA fragmentation., Results: Lymphocytes incubated with LKT at a high concentration (1.0 toxic U/ml) had ultrastructural evidence of cytoplasmic and nuclear membrane rupture and swelling or lysis of mitochondria. Low concentrations of leukotoxin (0.1 toxic U/ml) induced DNA fragmentation in 80% of lymphocytes. Ultrastructurally, these cells had nuclear membrane blebbing, cytoplasmic vaculation, chromatin condensation, nuclear fragmentation, and membrane-bound apoptotic bodies. Incubation of lymphocytes with LKT at extremely low concentrations (0.001 toxic U/ml) or with pro-LKT did not alter their ultrastructure. Inclusion of 0.5 mM ZnCl2 in the medium blocked leukotoxin-induced ultrastructural changes in bovine lymphocytes., Conclusions and Clinical Relevance: Low concentrations of LKT induce apoptosis and high concentrations induce oncotic cell lysis in bovine lymphocytes. The ability of low LKT concentrations to induce apoptosis in host leukocytes may allow bacteria to escape host immune surveillance and colonize the host.

Published

2000

23. Correlation of Pasteurella haemolytica leukotoxin binding with susceptibility to intoxication of lymphoid cells from various species.

Author

Sun Y, Clinkenbeard KD, Cudd LA, Clarke CR, and Clinkenbeard PA

Subjects

Animals, Cattle, Cell Line, Cell Survival, Cytotoxins toxicity, Dogs, Horses, Humans, Lymphocytes cytology, Swine, Cytotoxins metabolism, Exotoxins metabolism, Exotoxins toxicity, Lymphocytes metabolism, Mannheimia haemolytica metabolism

Abstract

Pasteurella haemolytica, the causative agent of shipping fever pneumonia in cattle, produces a leukotoxin (LKT) which lyses ruminant leukocytes with high efficiency but is reputed to not affect leukocytes from nonruminant species. In this study, we tested the supposition that LKT binding correlates positively with susceptibility to intoxication of susceptible isolated bovine lymphocytes and lymphoma tissue culture cells (BL3 cells) and negatively with reputed nonsusceptible equine, porcine, and canine lymphocytes and human lymphoid tissue culture cells (Raji cells). Bovine lymphocytes and BL3 cells were highly susceptible to LKT intoxication, exhibiting both substantial increase in intracellular Ca(2+) concentration and marked leukolysis. Exposure of reputed LKT-nonsusceptible porcine lymphocytes and Raji cells to LKT caused a slightly increased intracellular Ca(2+) concentration but no leukolysis. No LKT effect was detected for equine and canine lymphocytes. LKT bound to lymphoid cells from all species tested. Intact 102-kDa LKT was recovered from exposed isolated lymphoid cell membranes. Pro-LKT acylation was not required for LKT binding to BL3 cells. LKT binding was rapid, with maximal binding occurring by 3 min, and was proportional to the LKT concentration in the range 0.04 to 4.0 microg/ml. For this LKT concentration range, BL3 cells bound more LKT than did porcine lymphocytes or Raji cells, suggesting that LKT binds to BL3 cells with higher affinity than to porcine lymphocytes or Raji cells. Above 4.0 microg/ml, LKT demonstrated saturable binding to BL3 cells. Neutralizing anti-LKT monoclonal antibody (MAb) MM601 diminished LKT binding to BL3 by 36% while decreasing leukolysis by 81%. In contrast, MM601 did not diminish LKT binding to Raji cells. Pretreatment of target cells with 120 microg of protease K per ml diminished LKT binding to BL3 cells by 75%, with only a 25% decrease in leukolysis. However, pretreatment with 150 microg of protease K per ml abolished the remaining 25% of LKT binding and 75% leukolysis. Therefore, P. haemolytica LKT binds rapidly to susceptible and to reputed nonsusceptible lymphoid cells. LKT binding resulting in species-specific leukolysis was characterized by high affinity, inhibition by MAb MM601, and relative resistance to protease K pretreatment of lymphoid cells. Two types of LKT binding to lymphoid cells are proposed. High-affinity binding leads to efficient leukolysis. In some lymphoid cells from reputed LKT-nonsusceptible species, low-affinity LKT binding may cause a low-efficiency increase in the intracellular Ca(2+) concentration without leading to leukolysis.

Published

1999

24. Role of phospholipase D in Pasteurella haemolytica leukotoxin-induced increase in phospholipase A(2) activity in bovine neutrophils.

Author

Wang Z, Clarke CR, and Clinkenbeard KD

Subjects

Animals, Calcium physiology, Cattle, Enzyme Activation, Leukotriene B4 biosynthesis, Bacterial Toxins toxicity, Exotoxins toxicity, Mannheimia haemolytica pathogenicity, Neutrophils enzymology, Phospholipase D physiology, Phospholipases A biosynthesis

Abstract

The effects of Pasteurella haemolytica leukotoxin (LKT) on the activity of phospholipase D (PLD) and the regulatory interaction between PLD and phospholipase A(2) (PLA(2)) were investigated in assays using isolated bovine neutrophils labeled with tritiated phospholipid substrates of the two enzymes. Exposure of [(3)H]lysophosphatidylcholine-labeled neutrophils to LKT caused concentration- and time-dependent production of phosphatidic acid (PA), the product of PLD. LKT-induced generation of PA was dependent on extracellular calcium. Both production of PA and metabolism of [(3)H]-arachidonate ([(3)H]AA)-labeled phospholipids by PLA(2) were inhibited when ethanol was used to promote the alternative PLD-mediated transphosphatidylation reaction, resulting in the production of phosphatidylethanol rather than PA. The role of PA in regulation of PLA(2) activity was then confirmed by means of an add-back experiment, whereby addition of PA in the presence of ethanol restored PLA(2)-mediated release of radioactivity from neutrophil membranes. Considering the involvement of chemotactic phospholipase products in the pathogenesis of pneumonic pasteurellosis, development and use of anti-inflammatory agents that inhibit LKT-induced activation of PLD and PLA(2) may improve therapeutic management of the disease.

Published

1999

25. Bovine CD18 identified as a species specific receptor for Pasteurella haemolytica leukotoxin.

Author

Li J, Clinkenbeard KD, and Ritchey JW

Subjects

Animals, Antibodies, Monoclonal, Bacterial Toxins immunology, Blotting, Western veterinary, Electrophoresis, Polyacrylamide Gel veterinary, HL-60 Cells, Humans, Pasteurella Infections veterinary, Precipitin Tests veterinary, Species Specificity, Tumor Cells, Cultured, CD18 Antigens immunology, Cattle immunology, Exotoxins immunology, Mannheimia haemolytica immunology

Abstract

Ligand blotting of Pasteurella haemolytica leukotoxin (LKT) susceptible BL3 bovine lymphoma cell membranes with LKT detected two putative receptors with Mr of 95 and 100 kDa, whereas no LKT binding to membrane proteins was detected for LKT non-susceptible human leukemic cells. Anti-bovine CD18 and CD11a/CD18 mAb recognized 95 and 100kDa bands from BL3 cell membranes. CD18 isolated from BL3 cell membranes bound LKT. Pre-incubation of BL3 cells with anti-bovine CD18 or CD11a/CD18 mAb caused partial inhibition of LKT-induced leukolysis. Therefore, we propose that bovine CD18 acts as a species-specific leukocyte receptor for P. haemolytica LKT.

Published

1999

26. Lipopolysaccharide complexes with Pasteurella haemolytica leukotoxin.

Author

Li J and Clinkenbeard KD

Subjects

Animals, Bacterial Toxins isolation & purification, Cattle, Exotoxins isolation & purification, HL-60 Cells, Humans, Lipopolysaccharides isolation & purification, Mice, Polymyxin B metabolism, Sepharose, Bacterial Toxins metabolism, Exotoxins metabolism, Lipopolysaccharides metabolism, Mannheimia haemolytica metabolism

Abstract

The presence of lipopolysaccharide (LPS) in gram-negative bacterial repeats-in-toxin (RTX) toxin preparations, as well as the harsh conditions required to remove it, suggests that LPS may complex with RTX toxins. Concentrated culture supernatant (CCS) preparations of the RTX toxin Pasteurella haemolytica leukotoxin (LKT) contained LKT and LPS as the most prominent components, with LKT and LPS constituting approximately 30 and 50% of the density of the silver-stained fraction on sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE), respectively. CCS LKT contained 3.69 +/- 0.46 mg of LPS per mg of protein, which was estimated to indicate an LPS/LKT molar ratio of approximately 60:1. Subjection of the CCS LKT to preparative SDS-PAGE resulted in separation of LPS from LKT as detected by silver-stained analytical SDS-PAGE; however, the LKT fraction (SDS-PAGE LKT) contained significant endotoxin activity as detected by the Limulus amebocyte lysate assay. Subjection of the SDS-PAGE LKT to a second preparative SDS-PAGE run resulted in a reduction of the LPS/LKT molar ratio to 1:20. The target cell specificity of LKT for bovine leukocytic cells was retained by the SDS-PAGE LKT, and isolated LPS at comparable concentrations to that in CCS LKT exhibited no leukolytic activity. Addition of isolated LPS back to SDS-PAGE LKT resulted in reconstitution of an LPS-LKT complex. Immediately following reconstitution of the LPS-LKT complex, there was minimal change in leukolytic activity of the complex, but following 9.5 h at temperatures from -135 to 37 degrees C, the LPS-LKT complex exhibited increased leukolytic activity and thermal stability compared to SDS-PAGE LKT. Therefore, it appears that LPS complexes with LKT, resulting in enhanced and stabilized leukolytic activity.

Published

1999

27. Pasteurella haemolytica leukotoxin induced apoptosis of bovine lymphocytes involves DNA fragmentation.

Author

Sun Y, Clinkenbeard KD, Clarke C, Cudd L, Highlander SK, and Dabo SM

Subjects

Animals, Antibodies, Monoclonal, Apoptosis genetics, Apoptosis immunology, Cattle, Colorimetry veterinary, DNA, Bacterial chemistry, Electrophoresis, Agar Gel veterinary, Horses, L-Lactate Dehydrogenase analysis, Lymphocytes immunology, Mannheimia haemolytica chemistry, Pasteurella Infections immunology, Cattle Diseases immunology, DNA Fragmentation, Exotoxins immunology, Immunosuppressive Agents immunology, Mannheimia haemolytica immunology, Pasteurella Infections veterinary

Abstract

It has been reported that Pasteurella haemolytica leukotoxin (LKT) induces morphologic changes in bovine leukocytes consistent with apoptosis in vitro, but DNA fragmentation was not observed. We investigated whether bovine lymphocytes undergo DNA fragmentation during LKT-induced apoptosis. Bovine peripheral blood lymphocytes were isolated by density gradient centrifugation and exposed to LKT or inactive pro-LKT protein from a lktC- mutant strain. After exposure, DNA fragmentation in lymphocytes was quantified colorimetrically by diphenylamine assay and visualized by agarose gel electrophoresis. At high LKT concentrations, bovine lymphocytes were lysed, but at low concentrations, LKT caused DNA fragmentation characteristic of apoptosis. Maximal DNA fragmentation in bovine lymphocytes was induced by 0.1 TU ml(-1) LKT following 3 h exposure, but only background level of DNA fragmentation was observed with the inactive pro-LKT. Equine lymphocytes that are resistant to LKT intoxication did not show DNA fragmentation following exposure to LKT. Preincubation of LKT with a neutralizing anti-LKT monoclonal antibody inhibited LKT-induced DNA fragmentation. Electrophoresis of DNA from bovine lymphocytes treated with 0.1 TU ml(-1) LKT demonstrated the typical 'ladder' pattern of internucleosomal DNA cleavage, the hallmark of apoptosis associated with activation of endonucleases. LKT-induced DNA fragmentation was inhibited by 0.5 mM ZnCl2, an endonuclease inhibitor. The results indicated that LKT at low concentrations induced apoptotic cell death of bovine lymphocytes, which may play a role in initiation and persistence of P. haemolytica infection.

Published

1999

28. Duration of serum antibody responses following vaccination and revaccination of cattle with non-living commercial Pasteurella haemolytica vaccines.

Author

Confer AW, Fulton RW, Clinkenbeard KD, and Driskel BA

Subjects

Animals, Antigens, Bacterial immunology, Antigens, Surface immunology, Bacterial Toxins immunology, Cytotoxins immunology, Exotoxins immunology, Female, Immunization, Secondary veterinary, Immunosuppressive Agents immunology, Male, Vaccines, Attenuated immunology, Antibodies, Bacterial blood, Bacterial Vaccines immunology, Cattle immunology, Mannheimia haemolytica immunology, Pasteurellosis, Pneumonic prevention & control

Abstract

This study was designed to determine the duration of serum antibody responses to Pasteurella haemolytica whole cells (WC) and leukotoxin (LKT) in weanling beef cattle vaccinated with various non-living P. haemolytica vaccines. Serum antibodies to P. haemolytica antigens were determined periodically through day 140 by enzyme-linked immunosorbent assays. At day 140, cattle were revaccinated, and antibody responses periodically determined through day 196. Three vaccines were used in two experiments (A and B), OneShot, Presponse HP/tK, and Septimune PH-K. In general, all three vaccines between 7 and 14 days induced antibody responses to WC after vaccination. Antibodies to LKT were induced with OneShot and Presponse. Revaccination at days 28 and 140 usually stimulated anamnestic responses. Serum antibodies to the various antigens remained significantly increased for up to 84 days after vaccination or revaccination. The intensity and duration of antibody responses were variable depending on the experiment and vaccines used. Vaccination with OneShot usually stimulated the greatest responses to WC. Vaccination with OneShot or Presponse resulted in equivalent primary anti-LKT responses. In experiment B, spontaneous seroconversion was found in numerous calves on day 112. Revaccination of those cattle at day 140 resulted in markedly variable antibody responses such that several groups had no increase in antibody responses.

Published

1998

29. Serum-free culture of Pasteurella haemolytica optimized for leukotoxin production.

Author

Sun Y and Clinkenbeard KD

Subjects

Animals, Bacteriological Techniques, Cattle, Chlorides, Culture Media, Serum-Free, Ferric Compounds, Lung microbiology, Magnesium Sulfate, Mannheimia haemolytica isolation & purification, Mannheimia haemolytica metabolism, Bacterial Toxins biosynthesis, Exotoxins biosynthesis, Mannheimia haemolytica growth & development

Abstract

Objective: To screen supernatants of Pasteurella haemolytica cultures grown in 4 serum-free culture media for maximal leukotoxin (LKT) production and minimal protein concentration as an optimal source of LKT for purification., Sample Population: One strain of P haemolytica biotype A serotype 1 originally isolated from the pneumonic lung of a calf., Procedure: Pasteurella haemolytica was grown in brain-heart infusion (BHI) broth, yeast-tryptone broth, RPMI-1640 medium, and McCoy's modified 5A medium. Culture biomass and protein concentration, LKT activity, and LKT concentration in culture supernatants were measured. Effects of media pH and supplementation with metal cations and glucose on growth rate of P haemolytica and culture supernatant parameters were evaluated., Results: Pasteurella haemolytica cultivated in BHI broth or RPMI-1640 medium containing 0.1 M phosphate (pH 6.8) produced the highest concentrations of LKT. Supplementation of RPMI-1640 medium with 0.36 mM FeCl3 or 1.0 mM MgSO4 further increased specific activity of LKT in culture supernatant, but addition of 1% glucose did not enhance LKT production. Leukotoxin production in MgSO4-supplemented RPMI-1640 medium was comparable to that in serum protein-supplemented medium., Conclusions: Although BHI broth was superior to RPMI-1640 medium for P haemolytica growth and LKT production, the higher protein concentration and lower LKT specific activity made BHI broth a less desirable medium, compared with RPMI-1640 medium. Growth rate and LKT production with minimal protein content was optimal in pH 6.8 phosphate-buffered MgSO4-supplemented RPMI-1640 medium. This medium can serve as a source of culture supernatant for purification of LKT.

Published

1998

30. High-performance liquid chromatography of Pasteurella haemolytica leukotoxin using anion-exchange perfusion columns.

Author

el Rassi Z, Clinkenbeard PA, and Clinkenbeard KD

Subjects

Electrophoresis, Polyacrylamide Gel, Hydrogen-Ion Concentration, Lipopolysaccharides, Molecular Weight, Chromatography, High Pressure Liquid methods, Chromatography, Ion Exchange, Exotoxins isolation & purification, Mannheimia haemolytica

Abstract

An exotoxin, called leukotoxin (LKT), from Pasteurella haemolytica, which had previously proved difficult to purify, was purified by high-performance liquid chromatography using rigid highly hydrophilic microparticulate anion-exchange columns. These anion-exchange stationary phases were employed to overcome difficulties of the relatively hydrophobic LKT interacting with dextran or styrene-based resins. While a short non-porous DEAE column allowed the partial microscale purification of the leukotoxin at pH 7.0, a high capacity strong anion-exchange column of the perfusion chromatography type permitted the purification of LKT on a much larger scale. The purification of the LKT on the large pore strong anion-exchange perfusion column was best achieved when three consecutive linear gradients at increasing NaCl concentration in 20 mM Tris buffer, pH 8.0, containing 6.0 M urea and 0.25% Tween 20 were used. Under these conditions, a better separation was obtained for the tetrameric and aggregate peaks of LKT from the early eluting contaminant peaks. This separation scheme allowed good recovery of activity and purification of the LKT to near homogeneity.

Published

1998

31. Serum antibody responses of cattle vaccinated with partially purified native Pasteurella haemolytica leukotoxin.

Author

Confer AW, Clinkenbeard KD, Gatewood DM, Driskel BA, and Montelongo M

Subjects

Animals, Cattle, Vaccination, Antibodies, Bacterial blood, Bacterial Vaccines immunology, Exotoxins immunology, Mannheimia haemolytica immunology

Abstract

The objective of these experiments was to study the serum antibody responses of cattle to partially purified, native Pasteurella haemolytica A1 leukotoxin (LKT) formulated with a commercial aluminum hydroxide-DDA-bromide adjuvant. In two experiments, calves received two intramuscular injections 21 days apart and sera were obtained periodically. Serum antibody responses to P. haemolytica outer membrane proteins (OMPs), formalinized P. haemolytica, and LKT were determined. In Experiment A, Holstein calves (140 kg each) were vaccinated with either 10, 1.0 or 0.1 micrograms of LKT, 10(9) c.f.u. of live P. haemolytica, or adjuvanted diluent. In Experiment B, mixed-breed beef calves (200 kg each) were vaccinated with either 100, 50 or 10 micrograms of LKT, 10(9) c.f.u. live P. haemolytica, or adjuvanted diluent. Vaccination of dairy calves with 10 micrograms of partially purified LKT stimulated LKT neutralizing antibody responses similar to those stimulated by vaccination of one calf with live P. haemolytica. In Experiment B, which used larger and different breeds of cattle, two vaccinations 3 weeks apart with 50 micrograms LKT stimulated LKT neutralizing responses equivalent to or greater than those stimulated by vaccination with live P. haemolytica. In both experiments, LKT vaccines stimulated only low antibody responses to formalinized P. haemolytica or to OMPs.

Published

1997

32. Bone marrow mast cell hyperplasia in dogs with aplastic anemia.

Author

Walker D, Cowell RL, and Clinkenbeard KD

Published

1997

33. Hemolytic activity of the Pasteurella haemolytica leukotoxin.

Author

Murphy GL, Whitworth LC, Clinkenbeard KD, and Clinkenbeard PA

Subjects

Animals, DNA, Bacterial genetics, Genes, Bacterial, In Vitro Techniques, Mutagenesis, Rabbits, Sheep, Bacterial Toxins toxicity, Exotoxins toxicity, Hemolysin Proteins, Mannheimia haemolytica pathogenicity

Abstract

A Pasteurella haemolytica mutant incapable of producing leukotoxin was created by allelic replacement. Concentrated culture supernatants from wild-type P. haemolytica, but not from the mutant, contained the 102-kDa leukotoxin protein and lysed bovine lymphoma cells and sheep erythrocytes. Wild-type P. haemolytica demonstrated the typical beta-hemolytic phenotype on sheep and rabbit blood agar, whereas the mutant did not.

Published

1995

34. Chaotropic agents cause disaggregation and enhanced activity of Pasteurella haemolytica leukotoxin.

Author

Clinkenbeard KD, Clinkenbeard PA, and Waurzyniak BJ

Subjects

Animals, Bacterial Toxins chemistry, Bacterial Toxins isolation & purification, Cattle, Guanidine, L-Lactate Dehydrogenase drug effects, L-Lactate Dehydrogenase metabolism, Lymphoma, Thiocyanates pharmacology, Tumor Cells, Cultured, Urea pharmacology, Bacterial Toxins pharmacology, Guanidines pharmacology, Mannheimia haemolytica metabolism

Abstract

Pasteurella haemolytica biotype A, serotype 1 grown to late logarithmic growth phase in cell culture medium (RPMI 1640) produced highly aggregated leukotoxin. The multimer mass of the highly aggregated leukotoxin in 0.1 M sodium phosphate buffer pH 7.0 as determined by gel filtration chromatography on Sephacryl S400HR was approximately 8000 kDa. Resuspension of leukotoxin in phosphate buffer containing various chaotropic agents resulted in partial disaggregation of leukotoxin and enhanced leukotoxic activity. 3M guanidine disaggregated leukotoxin to a multimer mass of approximately 800 kDa and enhanced leukotoxic activity 3 to 20-fold. In 6 M urea or 1 M sodium thiocyanate, leukotoxin multimers were observed ranging in mass from 8000 kDa to 400 kDa, and activity enhancement was less than that for leukotoxin in 3 M guanidine. Several detergents were tested for enhancement of leukotoxic activity, but only 1% Tween 20 enhanced leukotoxic activity (4-fold), whereas 1.25% octylglucoside, 10 mM CHAPS, and 5 mM deoxycholate diminished and 1% Triton X-100 abolished leukotoxic activity.

Published

1995

35. Pasteurella haemolytica lipopolysaccharide-induced cytotoxicity in bovine pulmonary artery endothelial monolayers: inhibition by indomethacin.

Author

Paulsen DB, Confer AW, Clinkenbeard KD, and Mosier DA

Subjects

Animals, Cattle, Cells, Cultured, Endothelium, Vascular pathology, L-Lactate Dehydrogenase drug effects, L-Lactate Dehydrogenase metabolism, Lipopolysaccharides adverse effects, Microscopy, Electron veterinary, Microscopy, Electron, Scanning veterinary, Pilot Projects, Pulmonary Artery pathology, Time Factors, Endothelium, Vascular drug effects, Indomethacin pharmacology, Lipopolysaccharides antagonists & inhibitors, Mannheimia haemolytica chemistry, Pulmonary Artery drug effects

Abstract

Exposure of bovine pulmonary artery endothelial cells to Pasteurella haemolytica lipopolysaccharide caused severe morphologic changes. Initially, there was dilatation of the rough endoplasmic reticulum and mitochondrial swelling followed by cell retraction, membrane bleb formation, and cell detachment. The affected endothelial cells had severe membrane damage resulting in the leakage of lactate dehydrogenase. Indomethacin in concentrations of 0.5 mM or greater caused marked decreases in the lipopolysaccharide-induced leakage of lactate dehydrogenase. Indomethacin at 5 mM also caused a marked reduction of the lipopolysaccharide-induced morphologic changes resulting in apparent maintenance of the monolayer integrity for 8 hours versus 1 hour in the lipopolysaccharide-treated control. A marked decrease in the cell and nuclear membrane effects resulted, but the rough endoplasmic reticulum dilatation and mitochondrial changes proceeded. These results indicate that indomethacin does not prevent lipopolysaccharide binding but interferes with later events in lipopolysaccharide-induced cytotoxicity in the bovine pulmonary endothelial cell. The concentration of indomethacin required to produce this inhibition suggests that the primary mechanism is not cyclooxygenase inhibition.

Published

1995

36. Pasteurella haemolytica leukotoxin-induced synthesis of eicosanoids by bovine neutrophils in vitro.

Author

Clinkenbeard KD, Clarke CR, Hague CM, Clinkenbeard P, Srikumaran S, and Morton RJ

Subjects

Animals, Cattle, Cells, Cultured, Thromboxane B2 biosynthesis, Cytotoxins pharmacology, Exotoxins pharmacology, Leukotriene B4 biosynthesis, Mannheimia haemolytica, Neutrophils metabolism

Abstract

Exposure of isolated bovine neutrophils to partially purified Pasteurella haemolytica leukotoxin caused increased synthesis of leukotriene B4 (LTB4) but not thromboxane B2 (TXB2) from endogenous arachidonic acid. Synthesis of LTB4 was closely correlated with leukotoxin-induced neutrophil lysis. At low toxin concentrations, LTB4 production lagged behind leukotoxin-induced neutrophil lysis over a 3-h period. The neutralizing monoclonal antileukotoxin antibody MM601 neutralized both leukotoxin-induced neutrophil lysis and LTB4 synthesis. Both leukotoxin-induced neutrophil lysis and LTB4 synthesis were Ca(2+)-dependent. When leukotoxin-induced LTB4 synthesis from exogenous arachidonic acid was examined, significant LTB4 synthesis occurred at 5 min of leukotoxin exposure, which was before leukotoxin-induced lysis developed. Leukotoxin-induced LTB4 synthesis from endogenous arachidonic acid appears to require leukotoxin-induced plasma membrane damage (occurring during neutrophil lysis), whereas LTB4 synthesis from exogenous arachidonic acid is initiated rapidly and occurs in the absence of plasma membrane damage.

Published

1994

37. Enhancement of Pasteurella haemolytica leukotoxic activity by bovine serum albumin.

Author

Waurzyniak BJ, Clinkenbeard KD, Confer AW, and Srikumaran S

Subjects

Animals, Bacterial Toxins isolation & purification, Bacterial Toxins toxicity, Cattle, Cell Line, Cell Survival drug effects, Chromatography, Gel, Culture Media, Electrophoresis, Polyacrylamide Gel, Exotoxins isolation & purification, Exotoxins toxicity, L-Lactate Dehydrogenase, Mannheimia haemolytica metabolism, Molecular Weight, Tumor Cells, Cultured, Bacterial Toxins biosynthesis, Exotoxins biosynthesis, Mannheimia haemolytica growth & development, Serum Albumin, Bovine

Abstract

Growth of Pasteurella haemolytica A1 in RPMI 1640 medium containing 0.5% bovine serum albumin (BSA) for 2.5 hours enhanced culture supernatant leukotoxic activity (30,700 +/- 12,900 toxic units/ml, compared with leukotoxic activity of culture supernatants produced in RPMI 1640 medium alone (120 +/- 40 toxic units/ml). Gel filtration chromatography of the leukotoxic activity from RPMI 1640 medium supernatants in buffer containing 50 mM NaCl indicated a single leukotoxic activity peak (peak I) eluting near the gel resin molecular mass exclusion limit (estimated molecular mass of approx 8,000 kd). In contrast, culture supernatants produced in RPMI 1640 plus bovine serum albumin medium (RPMI + BSA) had peak I and 2 additional leukotoxic activity peaks (peaks II and III) with estimated molecular mass of approximately 80 and < 30 kd, respectively. All leukotoxic activity peaks were composed of approximately 100-kd molecular mass leukotoxin protomer, as determined by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and immunoblotting with a monoclonal antibody against leukotoxin. Subjecting culture supernatant leukotoxic activity produced in RPMI + BSA to gel filtration chromatography in buffer containing 500 mM NaCl or 6M urea resulted in detection of only a single leukotoxic activity peak with estimated approximate molecular mass of 250 and 800 kd, respectively. These findings suggest that P haemolytica exists as a high molecular mass aggregate with low leukotoxic activity which, in the presence of BSA, partially disaggregates to multiple toxin forms with enhanced leukotoxic activity. Some of these leukotoxin forms interact with dextran-based gel resins at low ionic strength.

Published

1994

38. Carcinoma in the urinary bladder of a cat: cytologic findings and a review of the literature.

Author

Walker DB, Cowell RL, Clinkenbeard KD, and Turgai J

Abstract

Percutaneous fine needle aspiration biopsy (FNAB) was used to diagnose a urinary bladder carcinoma in an aged cat. The cytologic appearance of specimens collected initially was similar to that reported for canine transitional cell carcinoma. However, impression smears of the tumor made at necropsy 7 weeks later consisted predominantly of atypical squamous epithelial cells compatible with squamous cell carcinoma. Histologically, the malignancy was noted to have intermixed areas of abnormal squamous and transitional cell proliferation. The neoplasia was interpreted as a transitional cell carcinoma with extensive transformation to squamous cell carcinoma. This report examines the use and limitations of FNAB in the diagnosis of feline urinary bladder carcinoma and the incidence and behavior of these tumors in the cat.

Published

1993

39. Dual systemic mycosis caused by Bipolaris spicifera and Torulopsis glabrata in a dog.

Author

Waurzyniak BJ, Hoover JP, Clinkenbeard KD, and Welsh RD

Subjects

Animals, Candidiasis complications, Candidiasis pathology, Dog Diseases pathology, Dogs, Male, Mycoses complications, Mycoses pathology, Candidiasis veterinary, Dog Diseases microbiology, Mitosporic Fungi, Mycoses veterinary

Published

1992

40. Lysis of bovine platelets by Pasteurella haemolytica leukotoxin.

Author

Clinkenbeard KD and Upton ML

Subjects

Animals, Blood Platelets enzymology, Cattle, Cells, Cultured, L-Lactate Dehydrogenase metabolism, Species Specificity, Bacterial Toxins pharmacology, Blood Platelets drug effects, Exotoxins pharmacology, Hemolysis drug effects, Pasteurella

Abstract

Pasteurella haemolytica A1 culture supernatants caused rapid cytolysis (less than 5 minutes) of isolated bovine platelets as measured by leakage of the cytoplasmic enzyme lactate dehydrogenase (LD). The platelet lytic factor had several features similar to P haemolytica leukotoxin. Like P haemolytica leukotoxin, the platelet lytic factor was produced by P haemolytica during logarithmic growth phase, was heat-labile, and was active against target cells (platelets) from ruminant species (cattle and sheep), but not from non-ruminant species (horses, pigs, and human beings). Additionally, the platelet lytic factor was neutralized with antileukotoxin rabbit serum. The amount of LD leaked by a fixed concentration of bovine platelets was proportional to the amount of toxin added at low toxic doses and became maximal at 88 +/- 11% of the total platelet LD activity for high doses of toxin. When a fixed dose of toxin was used and the platelet concentration was varied, LD leakage was initially proportional to the platelet concentration, but plateaued at higher platelet concentrations. The platelet lytic factor required Ca2+ and was inhibited by addition of the Ca2+ chelator ethylene glycol-bis(beta-aminoethyl ether)N,N,N',N'-tetraacetic acid. Toxin-mediated platelet damage may be important in thrombi formation and fibrin exudation typically associated with P haemolytica pleuropneumonia of cattle.

Published

1991

41. Mechanism of action of Moraxella bovis hemolysin.

Author

Clinkenbeard KD and Thiessen AE

Subjects

Animals, Calcium pharmacology, Cattle, Egtazic Acid pharmacology, Erythrocytes metabolism, Hypertonic Solutions, Potassium metabolism, Erythrocytes microbiology, Hemolysin Proteins toxicity, Moraxella pathogenicity

Abstract

Bovine erythrocytes (RBCs) exposed to Moraxella bovis culture supernatants exhibited rapid leakage of intracellular K+ (95% in 10 min), slower cell swelling (1.20-fold increase in mean corpuscular volume in 20 min), and subsequent lysis (76% leakage of hemoglobin in 25 min). Incubation media made hypertonic by the addition of 75 mM carbohydrates with molecular diameters of 0.72 to 1.32 nm prevented hemolysin-induced RBC swelling, but incubation media made hypertonic by the addition of carbohydrates with molecular diameters of less than 0.72 nm did not protect against hemolysin-induced RBC swelling. Raffinose (75 mM; molecular diameter, 1.14 nm) did not block hemolysin-induced K+ leakage but did block hemolysis. These findings support the hypothesis that hemolysin-induced lysis occurs by colloid-osmotic swelling and are compatible with M. bovis hemolysin acting as a pore-forming cytolysin. Assuming that M. bovis hemolysin acts as a transmembrane molecular sieve, then the functional size of the hemolysin transmembrane pores in bovine RBCs is approximately 0.9 nm, the molecular size of sucrose. Hemolytic activity was inhibited by the Ca2+ chelator ethylene glycol-bis (beta-aminoethyl ether)-N,N,N',N'-tetraacetic acid (EGTA), but hemolysin-induced K+ leakage was not affected by EGTA.

Published

1991

42. Pasteurella haemolytica lipopolysaccharide-induced arachidonic acid release from and neutrophil adherence to bovine pulmonary artery endothelial cells.

Author

Paulsen DB, Confer AW, Clinkenbeard KD, and Mosier DA

Subjects

Animals, Arachidonic Acid, Cattle, Cell Adhesion drug effects, Cell Adhesion physiology, Endothelium, Vascular cytology, Endothelium, Vascular physiology, Neutrophils drug effects, Pulmonary Artery cytology, Pulmonary Artery physiology, Arachidonic Acids metabolism, Endothelium, Vascular drug effects, Lipopolysaccharides toxicity, Neutrophils metabolism, Pasteurella, Pulmonary Artery drug effects

Abstract

Bovine pulmonary artery endothelial cells (BPAEC) were labeled with 3H-arachidonic acid. Exposure of the labeled BPAEC to Pasteurella haemolytica lipopolysaccharide (LPS) resulted in a time- and dose-dependent release of radioactivity. The release was inhibited by 5 mM indomethacin, but inhibition was not caused by less than or equal to 500 microM indomethacin or hydrocortisone, which suggests that the release was caused primarily by a mechanism other than cyclooxygenase or phospholipase A2 metabolism of arachidonic acid. Pasteurella haemolytica LPS also caused increased adherence of bovine neutrophils to BPAEC through independent effects on both cell types. The increased adherence was inhibited by treatment of either cell type with cycloheximide or actinomycin D prior to LPS exposure, indicating that de novo protein synthesis was required in both cell types to promote the LPS-induced adherence. Lipopolysaccharide may be an important factor in neutrophil-mediated effects in pneumonic pasteurellosis by causing increased neutrophil adherence and, thus, the vascular sequestration of neutrophils. Together, these experiments provide additional evidence for the involvement of LPS in pneumonic pasteurellosis. Moreover, they provide evidence of LPS-induced endothelial activation, which could have broad ramifications in the inflammatory and immune responses of pneumonic pasteurellosis.

Published

1990

43. Molecular aspects of virulence of Pasteurella haemolytica.

Author

Confer AW, Panciera RJ, Clinkenbeard KD, and Mosier DA

Subjects

Animals, Bacterial Toxins genetics, Exotoxins genetics, Fimbriae, Bacterial physiology, Lipopolysaccharides genetics, Pasteurella pathogenicity, Pasteurella Infections microbiology, Pneumonia microbiology, Polysaccharides, Bacterial genetics, Virulence, Pasteurella genetics, Pasteurella Infections veterinary, Pneumonia veterinary

Abstract

Pasteurella haemolytica is represented by two biotypes (A and T), 15 serotypes, and numerous untypable strains. Specific biotypes and serotypes are associated with fibrinous pleuropneumonia (pneumonic pasteurellosis) in cattle, sheep, and goats, septicemic pasteurellosis in lambs, and mastitis in ewes. Four virulence factors have been associated with P. haemolytica: fimbriae, a polysaccharide capsule, endotoxin [lipopolysaccharide (LPS)], and leukotoxin (LKT). The interactions of these virulence factors with components of the pulmonary alveolus are discussed as a model for the pathogenesis of pasteurellosis. Fimbriae on P. haemolytica may enhance colonization of the upper respiratory tract. The capsule of P. haemolytica varies in composition among serotypes. It inhibits complement-mediated serum killing as well as phagocytosis and intracellular killing of P. haemolytica. The capsule enhances neutrophil directed migration and adhesion of P. haemolytica to alveolar epithelium. Pasteurella haemolytica LPS can alter bovine leukocyte functions, by dose-dependent inhibition or augmentation; it is directly toxic to bovine endothelium; it modifies cardiopulmonary hemodynamics; and it elevates circulatory prostanoids, serotonin, cAMP, and cGMP. Leukotoxin is produced by all known serotypes and many untypable strains. Leukotoxin is a poreforming cytolysin that affects ruminant leukocytes and platelets by altering function at low levels but causing lysis at high levels.

Published

1990

44. Effects of Pasteurella haemolytica leukotoxin on neutrophils from white-tailed deer and several exotic ruminant species.

Author

Confer AW, Simons KR, Barrie MT, and Clinkenbeard KD

Subjects

Animals, Bacterial Toxins pharmacology, Cattle blood, Cytotoxins pharmacology, Antelopes blood, Artiodactyla blood, Deer blood, Exotoxins pharmacology, Neutrophils physiology, Pasteurella

Abstract

Pasteurella haemolytica leukotoxin is a pore-forming cytolysin which acts as a virulence factor in pasteurellosis of domestic ruminants. Leukocytes from cattle, sheep and goats are susceptible to leukotoxin-induced lysis; however, leukocytes from non-ruminant species so far tested are resistant to leukotoxin-induced lysis. Neutrophils obtained from three white-tailed deer, four Saiga antelope, an Addra gazelle, a Grant's gazelle and a Sable antelope were tested for susceptibility to the lytic effects of P. haemolytica leukotoxin using lactate dehydrogenase release. Results were compared to those obtained using neutrophils from a steer and cultured bovine lymphoma cells. Neutrophils obtained from all these ruminants, except the Addra gazelle, were susceptible to P. haemolytica leukotoxin. Individual variation among the Saiga and the deer did not appear to be due to the percentages of neutrophils or the percentage of contaminating erythrocytes in the cell preparations.

Published

1990

45. Identification of Histoplasma organisms in circulating eosinophils of a dog.

Author

Clinkenbeard KD, Cowell RL, and Tyler RD

Subjects

Animals, Dogs, Female, Histoplasmosis microbiology, Monocytes microbiology, Neutrophils microbiology, Dog Diseases microbiology, Eosinophils microbiology, Histoplasma isolation & purification, Histoplasmosis veterinary

Abstract

Disseminated histoplasmosis was diagnosed in a 10-year-old dog that had chronic diarrhea, weight loss, fever, and anemia. The diagnosis was based on detection of Histoplasma organisms in circulating neutrophils, monocytes, and eosinophils. The dog had severe histoplasmal fungemia, which may have been caused by treatment with prednisolone.

Published

1988

46. Cytosolic 3-hydroxy-3-methylglutaryl-CoA synthase from chicken liver.

Author

Clinkenbeard KD, Sugiyama T, and Lane MD

Subjects

Acetoacetates, Animals, Chickens, Chromatography, DEAE-Cellulose, Chromatography, Gel, Chromatography, Ion Exchange, Cytosol enzymology, Glutarates, Hydrogen-Ion Concentration, Kinetics, Methods, Molecular Weight, Oxo-Acid-Lyases metabolism, Liver enzymology, Oxo-Acid-Lyases isolation & purification

Published

1975

47. Hematologic values in horses and interpretation of hematologic data.

Author

Tyler RD, Cowell RL, Clinkenbeard KD, and MacAllister CG

Subjects

Animals, Hematologic Diseases diagnosis, Hematologic Diseases pathology, Horse Diseases pathology, Horses, Reference Values, Hematologic Diseases veterinary, Hematologic Tests veterinary, Horse Diseases diagnosis

Abstract

Normal reference ranges and pertinent background information on equine hematology are presented and briefly discussed. Diagnostic interpretation of hematologic data is discussed and three diagnostic algorithms and two diagnostic tables are provided to facilitate the use of the presented information for diagnosis. Two cases are presented and the information presented in the article is used to interpret the case data.

Published

1987

48. Disseminated histoplasmosis in cats: 12 cases (1981-1986).

Author

Clinkenbeard KD, Cowell RL, and Tyler RD

Subjects

Animals, Bone Marrow microbiology, Cats, Female, Histoplasma isolation & purification, Histoplasmosis diagnosis, Male, Retrospective Studies, Cat Diseases diagnosis, Histoplasmosis veterinary

Abstract

Anemia, weight loss, lethargy, fever, anorexia, and interstitial lung disease were the predominant clinical findings in 12 cats with disseminated histoplasmosis. Some cats were examined because of dysfunction or lesions of bone, eyes, or skin. In most cases, the clinical signs were observed by the owner for 4 weeks or less before seeking veterinary care. Young cats were most commonly affected, with 7 of the 12 cats less than or equal to 1 year old. Identification of Histoplasma organisms in bone marrow aspirates was used to confirm the diagnosis of histoplasmosis in 11 of the 12 cats. Histoplasma infection of multiple organs was found at necropsy. In this study, disseminated histoplasmosis had a higher prevalence in cats than in dogs at the same veterinary medical teaching hospital. Feline disseminated histoplasmosis was not associated with FeLV infection. Treatment was attempted in 7 of the 12 cats.

Published

1987

49. Collection and evaluation of equine peritoneal and pleural effusions.

Author

Cowell RL, Tyler RD, Clinkenbeard KD, and MacAllister CG

Subjects

Animals, Ascites classification, Ascites pathology, Horses, Pleural Effusion classification, Pleural Effusion pathology, Ascites veterinary, Horse Diseases pathology, Pleural Effusion veterinary, Specimen Handling veterinary

Abstract

This article discusses collection, slide preparation, culture technique, fluid analysis and evaluation, and cytologic evaluation of peritoneal and pleural effusions. The morphologic characteristics of various effusions are described, and the physical characteristics (volume, color, turbidity) of effusions are discussed. An algorithm for classifying effusions as transudates, modified transudates, or exudates is included, and each category is discussed.

Published

1987

50. Pasteurella haemolytica antigens associated with resistance to pneumonic pasteurellosis.

Author

Mosier DA, Simons KR, Confer AW, Panciera RJ, and Clinkenbeard KD

Subjects

Animals, Antigens, Surface immunology, Blotting, Western, Cattle, Endotoxins immunology, Molecular Weight, Polysaccharides, Bacterial immunology, Antibodies, Bacterial immunology, Antigens, Bacterial immunology, Pasteurella immunology, Pasteurella Infections immunology

Abstract

Antigens associated with whole Pasteurella haemolytica biotype A serotype 1, a capsular carbohydrate-protein extract of the organism, and P. haemolytica leukotoxin were separated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis. Antigens of the electrophoresed preparations were detected by Western blotting (immunoblotting) with sera from cattle which were either nonvaccinated or vaccinated with live or killed P. haemolytica vaccines and had variable degrees of resistance to experimental pneumonic pasteurellosis. Distinct, easily recognizable antigens of these preparations were identified, and the antibody responses to these antigens were quantified by densitometry. To determine their importance to disease resistance, we then compared antibody responses with experimental lesion scores. Antibody reactivity to surface antigens which were significantly correlated with resistance and present in two or more of the preparations were detected at 86, 66, 51, 49, 34, 31, and 16 kilodaltons (kDa). Of these, antibody responses to antigens at 86, 49, and 31 kDa appeared most important based on their concentration and significance levels. Antibody reactivity to leukotoxin antigens which were significantly correlated with resistance and common with important surface antigens were detected at 86, 66, and 49 kDa. Antibody responses to unique leukotoxin antigens which were significantly correlated with resistance were present at 92 and 58 kDa.

Published

1989