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2. Sequence analysis of the msp4 gene of Anaplasma phagocytophilum strains

Author

de la Fuente, J, Massung, R F, Wong, S J, Chu, F K, Lutz, H, Meli, M, von Loewenich, F D, Grzeszczuk, A, Torina, A, Caracappa, S, Mangold, A J, Naranjo, V, Stuen, S, Kocan, K M, de la Fuente, J, Massung, R F, Wong, S J, Chu, F K, Lutz, H, Meli, M, von Loewenich, F D, Grzeszczuk, A, Torina, A, Caracappa, S, Mangold, A J, Naranjo, V, Stuen, S, and Kocan, K M

Abstract

The causative agent of human granulocytic ehrlichiosis was recently reclassified as Anaplasma phagocytophilum, unifying previously described bacteria that cause disease in humans, horses, dogs, and ruminants. For the characterization of genetic heterogeneity in this species, the homologue of Anaplasma marginale major surface protein 4 gene (msp4) was identified, and the coding region was PCR amplified and sequenced from a variety of sources, including 50 samples from the United States, Germany, Poland, Norway, Italy, and Switzerland and 4 samples of A. phagocytophilum-like organisms obtained from white-tailed deer in the United States. Sequence variation between strains of A. phagocytophilum (90 to 100% identity at the nucleotide level and 92 to 100% similarity at the protein level) was higher than in A. marginale. Phylogenetic analyses of msp4 sequences did not provide phylogeographic information but did differentiate strains of A. phagocytophilum obtained from ruminants from those obtained from humans, dogs, and horses. The sequence analysis of the recently discovered A. phagocytophilum msp2 gene corroborated these results. The results reported here suggest that although A. phagocytophilum-like organisms from white-tailed deer may be closely related to A. phagocytophilum, they could be more diverse. These results suggest that A. phagocytophilum strains from ruminants could share some common characteristics, including reservoirs and pathogenicity, which may be different from strains that infect humans.

Published
2005

3. Q Fever, Spotted Fever Group, and Typhus Group Rickettsioses Among Hospitalized Febrile Patients in Northern Tanzania

Author

Prabhu, M., primary, Nicholson, W. L., additional, Roche, A. J., additional, Kersh, G. J., additional, Fitzpatrick, K. A., additional, Oliver, L. D., additional, Massung, R. F., additional, Morrissey, A. B., additional, Bartlett, J. A., additional, Onyango, J. J., additional, Maro, V. P., additional, Kinabo, G. D., additional, Saganda, W., additional, and Crump, J. A., additional

Published
2011
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15. Molecular cloning, sequencing, expression, and characterization of an immunogenic 43-kilodalton lipoprotein of Bartonella bacilliformis that has homology to NlpD/LppB.

Author

Padmalayam, I, Kelly, T, Baumstark, B, and Massung, R

Abstract

A recombinant clone expressing an immunoreactive antigen of Bartonella bacilliformis was isolated by screening a genomic DNA library with serum from a patient with the chronic verruga phase of bartonellosis. The clone, pBIPIM-17, contained a partial open reading frame that expressed an immunoreactive fusion protein. Subsequent rescreening of the library by plaque hybridization resulted in the isolation of recombinant clones that contain the entire open reading frame. The open reading frame (ORF-401) is capable of encoding a protein of 401 amino acids with a predicted molecular mass of 43 kDa. The deduced amino acid sequence of the encoded protein was found to be highly homologous to a recently identified bacterial lipoprotein (LppB/NlpD) which has been associated with virulence. Evidence has been provided to show that the 43-kDa antigen of B. bacilliformis is a lipoprotein and that it is likely to use the same biosynthetic pathway as other bacterial lipoproteins. This is the first report to date that characterizes a lipoprotein of B. bacilliformis. The immunogenicity of the B. bacilliformis LppB homologue was demonstrated by Western blot analysis using sera from patients with clinical bartonellosis. Sera from patients who had a high titer for Bartonella henselae, the causative agent of bacillary angiomatosis and cat scratch disease, also recognized the recombinant 43-kDa antigen, suggesting that a homologue of this antigen is present in B. henselae. Using a cocktail of synthetic peptides corresponding to predicted major antigenic sites, polyclonal antiserum specific for the LppB homologue of B. bacilliformis was generated. This antiserum did not recognize the NlpD homologue of Escherichia coli or the 43-kDa antigen of B. henselae.

Published
2000

16. Sequence analysis of the ank gene of granulocytic ehrlichiae.

Author

Massung, R F, Owens, J H, Ross, D, Reed, K D, Petrovec, M, Bjoersdorff, A, Coughlin, R T, Beltz, G A, and Murphy, C I

Abstract

The ank gene of the agent of human granulocytic ehrlichiosis (HGE) codes for a protein with a predicted molecular size of 131.2 kDa that is recognized by serum from both dogs and humans infected with granulocytic ehrlichiae. As part of an effort to assess the phylogenetic relatedness of granulocytic ehrlichiae from different geographic regions and in different host species, the ank gene was PCR amplified and sequenced from a variety of sources. These included 10 blood specimens from patients with confirmed human granulocytic ehrlichiosis (three from New York, four from Wisconsin, two from Slovenia, and one from Sweden). Also examined was a canine granulocytic ehrlichia sample obtained from Minnesota, Ehrlichia equi from California, Ehrlichia phagocytophila from Sweden, and the granulocytic ehrlichia isolate USG3. The sequences showed a high level of homology (>95.5% identity), with the lowest homology occurring between a New York HGE agent and the Swedish E. phagocytophila. Several 3-bp deletions and a variable number of 51- and 81-bp direct repeats were noted. Although the North American HGE sequences showed the highest conservation (>98.1% identity), phylogenetic analyses indicated that these samples represent two separate clades, one including the three New York HGE samples and the USG3 strain and another with the Wisconsin HGE and Minnesota canine sequences. Two of the New York samples and the USG3 strain showed 100% identity over the entire 3,696-bp product. Likewise, three of the Wisconsin human samples and the Minnesota dog sample were identical (3,693 bp). Whereas phylogenetic analysis showed that the E. equi sequence was most closely related to the Upper Midwest samples, analysis of the repeat structures showed it to be more similar to the European samples. Overall, the genetic analysis based on the ank gene showed that the granulocytic ehrlichiae are closely related, appear to infect multiple species, and can be grouped into at least three different clades, two North American and one European.

Published
2000

17. IS1111 insertion sequences of Coxiella burnetii: characterization and use for repetitive element PCR-based differentiation of Coxiella burnetii isolates

Author

Massung Robert F, Thompson Herbert A, and Denison Amy M

Subjects
Microbiology, QR1-502
Abstract

Abstract Background Coxiella burnetii contains the IS1111 transposase which is present 20 times in the Nine Mile phase I (9Mi/I) genome. A single PCR primer that binds to each IS element, and primers specific to a region ~500-bp upstream of each of the 20 IS1111 elements were designed. The amplified products were characterized and used to develop a repetitive element PCR genotyping method. Results Isolates Nine Mile phase II, Nine Mile RSA 514, Nine Mile Baca, Scottish, Ohio, Australian QD, Henzerling phase I, Henzerling phase II, M44, KAV, PAV, Q238, Q195 and WAV were tested by PCR and compared to 9Mi/I. Sequencing was used to determine the exact differences in isolates which lacked specific IS elements or produced PCR products of differing size. From this data, an algorithm was created utilizing four primer pairs that allows for differentiation of unknown isolates into five genomic groups. Additional isolates (Priscilla Q177, Idaho Q, Qiyi, Poker Cat, Q229 and Q172) and nine veterinary samples were characterized using the algorithm which resulted in their placement into three distinct genomic groups. Conclusion Through this study significant differences, including missing elements and sequence alterations within and near IS element coding regions, were found between the isolates tested. Further, a method for differentiation of C. burnetii isolates into one of five genomic groups was created. This algorithm may ultimately help to determine the relatedness between known and unknown isolates of C. burnetii.

Published
2007
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19. A Mixed Outbreak of Epidemic Typhus Fever and Trench Fever in a Youth Rehabilitation Center: Risk Factors for Illness from a Case-Control Study, Rwanda, 2012.

Author

Umulisa I, Omolo J, Muldoon KA, Condo J, Habiyaremye F, Uwimana JM, Muhimpundu MA, Galgalo T, Rwunganira S, Dahourou AG, Tongren E, Koama JB, McQuiston J, Raghunathan PL, Massung R, Gatei W, Boer K, Nyatanyi T, Mills EJ, and Binagwaho A

Subjects
Adolescent, Adult, Animals, Bartonella quintana pathogenicity, Case-Control Studies, Coinfection, Humans, Incidence, Male, Odds Ratio, Rehabilitation Centers, Rickettsia prowazekii pathogenicity, Risk Factors, Rwanda epidemiology, Survival Analysis, Trench Fever diagnosis, Trench Fever mortality, Trench Fever transmission, Typhus, Epidemic Louse-Borne diagnosis, Typhus, Epidemic Louse-Borne mortality, Typhus, Epidemic Louse-Borne transmission, Bartonella quintana isolation & purification, Disease Outbreaks, Phthiraptera microbiology, Rickettsia prowazekii isolation & purification, Trench Fever epidemiology, Typhus, Epidemic Louse-Borne epidemiology
Abstract

In August 2012, laboratory tests confirmed a mixed outbreak of epidemic typhus fever and trench fever in a male youth rehabilitation center in western Rwanda. Seventy-six suspected cases and 118 controls were enrolled into an unmatched case-control study to identify risk factors for symptomatic illness during the outbreak. A suspected case was fever or history of fever, from April 2012, in a resident of the rehabilitation center. In total, 199 suspected cases from a population of 1,910 male youth (attack rate = 10.4%) with seven deaths (case fatality rate = 3.5%) were reported. After multivariate analysis, history of seeing lice in clothing (adjusted odds ratio [aOR] = 2.6, 95% confidence interval [CI] = 1.1-5.8), delayed (≥ 2 days) washing of clothing (aOR = 4.0, 95% CI = 1.6-9.6), and delayed (≥ 1 month) washing of beddings (aOR = 4.6, 95% CI = 2.0-11) were associated with illness, whereas having stayed in the rehabilitation camp for ≥ 6 months was protective (aOR = 0.20, 95% CI = 0.10-0.40). Stronger surveillance and improvements in hygiene could prevent future outbreaks., (© The American Society of Tropical Medicine and Hygiene.)

Published
2016
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20. Development of a TaqMan Array Card for Acute-Febrile-Illness Outbreak Investigation and Surveillance of Emerging Pathogens, Including Ebola Virus.

Author

Liu J, Ochieng C, Wiersma S, Ströher U, Towner JS, Whitmer S, Nichol ST, Moore CC, Kersh GJ, Kato C, Sexton C, Petersen J, Massung R, Hercik C, Crump JA, Kibiki G, Maro A, Mujaga B, Gratz J, Jacob ST, Banura P, Scheld WM, Juma B, Onyango CO, Montgomery JM, Houpt E, and Fields B

Subjects
Adult, Epidemiological Monitoring, Humans, Molecular Diagnostic Techniques standards, Real-Time Polymerase Chain Reaction standards, Reference Standards, Sensitivity and Specificity, Time Factors, Communicable Diseases diagnosis, Communicable Diseases epidemiology, Disease Outbreaks, Fever of Unknown Origin diagnosis, Fever of Unknown Origin epidemiology, Molecular Diagnostic Techniques methods, Real-Time Polymerase Chain Reaction methods
Abstract

Acute febrile illness (AFI) is associated with substantial morbidity and mortality worldwide, yet an etiologic agent is often not identified. Convalescent-phase serology is impractical, blood culture is slow, and many pathogens are fastidious or impossible to cultivate. We developed a real-time PCR-based TaqMan array card (TAC) that can test six to eight samples within 2.5 h from sample to results and can simultaneously detect 26 AFI-associated organisms, including 15 viruses (chikungunya, Crimean-Congo hemorrhagic fever [CCHF] virus, dengue, Ebola virus, Bundibugyo virus, Sudan virus, hantaviruses [Hantaan and Seoul], hepatitis E, Marburg, Nipah virus, o'nyong-nyong virus, Rift Valley fever virus, West Nile virus, and yellow fever virus), 8 bacteria (Bartonella spp., Brucella spp., Coxiella burnetii, Leptospira spp., Rickettsia spp., Salmonella enterica and Salmonella enterica serovar Typhi, and Yersinia pestis), and 3 protozoa (Leishmania spp., Plasmodium spp., and Trypanosoma brucei). Two extrinsic controls (phocine herpesvirus 1 and bacteriophage MS2) were included to ensure extraction and amplification efficiency. Analytical validation was performed on spiked specimens for linearity, intra-assay precision, interassay precision, limit of detection, and specificity. The performance of the card on clinical specimens was evaluated with 1,050 blood samples by comparison to the individual real-time PCR assays, and the TAC exhibited an overall 88% (278/315; 95% confidence interval [CI], 84% to 92%) sensitivity and a 99% (5,261/5,326, 98% to 99%) specificity. This TaqMan array card can be used in field settings as a rapid screen for outbreak investigation or for the surveillance of pathogens, including Ebola virus., (Copyright © 2015, American Society for Microbiology. All Rights Reserved.)

Published
2016
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21. Community-based control of the brown dog tick in a region with high rates of Rocky Mountain spotted fever, 2012-2013.

Author

Drexler N, Miller M, Gerding J, Todd S, Adams L, Dahlgren FS, Bryant N, Weis E, Herrick K, Francies J, Komatsu K, Piontkowski S, Velascosoltero J, Shelhamer T, Hamilton B, Eribes C, Brock A, Sneezy P, Goseyun C, Bendle H, Hovet R, Williams V, Massung R, and McQuiston JH

Subjects
Animals, Arachnid Vectors pathogenicity, Arizona, Dogs, Humans, Indians, North American, Residence Characteristics, Rhipicephalus sanguineus genetics, Rickettsia rickettsii isolation & purification, Rickettsia rickettsii pathogenicity, Rocky Mountain Spotted Fever transmission, Rocky Mountain Spotted Fever virology, Rhipicephalus sanguineus parasitology, Rocky Mountain Spotted Fever epidemiology, Tick Infestations epidemiology
Abstract

Rocky Mountain spotted fever (RMSF) transmitted by the brown dog tick (Rhipicephalus sanguineus sensu lato) has emerged as a significant public health risk on American Indian reservations in eastern Arizona. During 2003-2012, more than 250 RMSF cases and 19 deaths were documented among Arizona's American Indian population. The high case fatality rate makes community-level interventions aimed at rapid and sustained reduction of ticks urgent. Beginning in 2012, a two year pilot integrated tick prevention campaign called the RMSF Rodeo was launched in a ∼ 600-home tribal community with high rates of RMSF. During year one, long-acting tick collars were placed on all dogs in the community, environmental acaricides were applied to yards monthly, and animal care practices such as spay and neuter and proper tethering procedures were encouraged. Tick levels, indicated by visible inspection of dogs, tick traps and homeowner reports were used to monitor tick presence and evaluate the efficacy of interventions throughout the project. By the end of year one, <1% of dogs in the RMSF Rodeo community had visible tick infestations five months after the project was started, compared to 64% of dogs in Non-Rodeo communities, and environmental tick levels were reduced below detectable levels. The second year of the project focused on use of the long-acting collar alone and achieved sustained tick control with fewer than 3% of dogs in the RMSF Rodeo community with visible tick infestations by the end of the second year. Homeowner reports of tick activity in the domestic and peridomestic setting showed similar decreases in tick activity compared to the non-project communities. Expansion of this successful project to other areas with Rhipicephalus-transmitted RMSF has the potential to reduce brown dog tick infestations and save human lives.

Published
2014
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22. A large Q fever outbreak in an urban school in central Israel.

Author

Amitai Z, Bromberg M, Bernstein M, Raveh D, Keysary A, David D, Pitlik S, Swerdlow D, Massung R, Rzotkiewicz S, Halutz O, and Shohat T

Subjects
Adolescent, Adult, Aged, Aged, 80 and over, Air Conditioning, Antibodies, Bacterial blood, Case-Control Studies, DNA, Bacterial isolation & purification, Environmental Microbiology, Female, Humans, Israel epidemiology, Male, Middle Aged, Polymerase Chain Reaction, Schools, Urban Population, Young Adult, Coxiella burnetii isolation & purification, Disease Outbreaks, Q Fever epidemiology
Abstract

BACKGROUND. On 28 June 2005, numerous cases of febrile illness were reported among 322 students and employees of a boarding high school located in an urban area in central Israel. Subsequent investigation identified a large outbreak of Q fever which started 2 weeks earlier. We describe the investigation of this outbreak and its possible implications. METHODS. We conducted a case-control study to identify risk factors for Q fever disease. Environmental sampling was conducted to identify the source and the mode of transmission of Coxiella burnetii, the infectious agent. RESULTS. Of 303 individuals, 187 (62%) reported being ill between 15 June and 13 July 2005. Serological evidence for C. burnetii infection was evident in 144 (88%) of the 164 tested individuals. Being a student, dining regularly at the school dining room, and boarding at school during a June religious holiday and the preceding weekend were all significant risk factors for contracting Q fever. C. burnetii DNA was detected using polymerase chain reaction on samples from the school dining room's air conditioning system, supporting contribution of the air conditioning system to the aerosol transmission of the infectious agent. CONCLUSIONS. We report a large outbreak of Q fever in an urban school, possibly transmitted through an air conditioning system. A high level of suspicion for C. burnetii infection should be maintained when investigating point source outbreaks of influenza-like disease, especially outside the influenza season.

Published
2010
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23. Distinct ecologically relevant strains of Anaplasma phagocytophilum.

Author

Foley JE, Nieto NC, Massung R, Barbet A, Madigan J, and Brown RN

Subjects
Animals, Arvicolinae microbiology, Ehrlichiosis microbiology, Europe, Horse Diseases microbiology, Horse Diseases parasitology, Horses microbiology, Humans, Mice, Mice, Inbred C3H, North America, Phenotype, Polymerase Chain Reaction, Sciuridae microbiology, Anaplasma phagocytophilum classification, Anaplasma phagocytophilum genetics, Anaplasma phagocytophilum pathogenicity, Anaplasma phagocytophilum physiology, Ecosystem, Ehrlichiosis veterinary
Published
2009
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24. Bartonella spp. and Rickettsia felis in fleas, Democratic Republic of Congo.

Author

Sackal C, Laudisoit A, Kosoy M, Massung R, Eremeeva ME, Karpathy SE, Van Wyk K, Gabitzsch E, and Zeidner NS

Subjects
Animals, Bacterial Proteins genetics, Bartonella classification, Bartonella genetics, DNA, Bacterial analysis, Democratic Republic of the Congo, Humans, Phylogeny, Polymerase Chain Reaction, Rickettsia felis classification, Rickettsia felis genetics, Bartonella isolation & purification, Insect Vectors microbiology, Rickettsia felis isolation & purification, Siphonaptera microbiology
Published
2008
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25. Identification of a p28 gene in Ehrlichia ewingii: evaluation of gene for use as a target for a species-specific PCR diagnostic assay.

Author

Gusa AA, Buller RS, Storch GA, Huycke MM, Machado LJ, Slater LN, Stockham SL, and Massung RF

Subjects
Amino Acid Sequence, Animals, Bacterial Outer Membrane Proteins chemistry, Base Sequence, DNA, Bacterial genetics, Dog Diseases diagnosis, Dog Diseases microbiology, Dogs, Ehrlichia classification, Ehrlichiosis microbiology, Ehrlichiosis veterinary, Humans, Molecular Sequence Data, Sensitivity and Specificity, Sequence Analysis, DNA, Species Specificity, Bacterial Outer Membrane Proteins genetics, Ehrlichia genetics, Ehrlichia isolation & purification, Ehrlichiosis diagnosis, Polymerase Chain Reaction methods
Abstract

PCR was used to amplify a 537-bp region of an Ehrlichia ewingii gene encoding a homologue of the 28-kDa major antigenic protein (P28) of Ehrlichia chaffeensis. The E. ewingii p28 gene homologue was amplified from DNA extracted from whole blood obtained from four humans and one canine with confirmed cases of infection. Sequencing of the PCR products (505 bp) revealed a partial gene with homology to outer membrane protein genes from Ehrlichia and Cowdria spp.: p30 of Ehrlichia canis (< or =71.3%), p28 of E. chaffeensis (< or =68.3%), and map1 of Cowdria ruminantium (67.3%). The peptide sequence of the E. ewingii partial gene product was deduced (168 amino acids) and the antigenicity profile was analyzed, revealing a hydrophilic protein with < or =69.1% identity to P28 of E. chaffeensis, < or =67.3% identity to P30 of E. canis, and < or =63.1% identity to MAP1 of C. ruminantium. Primers were selected from the E. ewingii p28 sequence and used to develop a species-specific PCR diagnostic assay. The p28 PCR assay amplified the expected 215-bp product from DNA that was extracted from EDTA-treated blood from each of the confirmed E. ewingii infections that were available. The assay did not produce PCR products with DNA extracted from E. chaffeensis-, E. canis-, or E. phagocytophila-infected samples, confirming the specificity of the p28 assay for E. ewingii. The sensitivity of the E. ewingii-specific PCR assay was evaluated and determined to detect as few as 38 copies of the p28 gene.

Published
2001
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26. Ehrlichia-infected ticks on migrating birds.

Author

Bjöersdorff A, Bergström S, Massung RF, Haemig PD, and Olsen B

Subjects
Animals, Bird Diseases parasitology, DNA, Ribosomal analysis, Ehrlichia genetics, Ehrlichiosis microbiology, Ehrlichiosis transmission, Genes, rRNA, Humans, Ixodes growth & development, Molecular Sequence Data, RNA, Ribosomal, 16S genetics, Sequence Analysis, DNA, Songbirds parasitology, Tick Infestations parasitology, Ehrlichia isolation & purification, Flight, Animal, Ixodes microbiology, Songbirds physiology, Tick Infestations veterinary
Abstract

During the spring of 1996, an estimated 581,395 Ehrlichia-infected ticks were imported into Sweden by migrating birds. Ehrlichia gene sequences found in ticks collected from these migrating birds were identical to those of granulocytic ehrlichiosis found in domestic animals and humans in Sweden. These findings support the idea that birds may play a role in dispersing Ehrlichia.

Published
2001
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27. Human granulocytic ehrlichiosis--a clinical case in Scandinavia.

Author

Karlsson U, Bjöersdorff A, Massung RF, and Christensson B

Subjects
Adult, Anti-Bacterial Agents therapeutic use, Doxycycline therapeutic use, Ehrlichia genetics, Ehrlichiosis drug therapy, Humans, Male, Scandinavian and Nordic Countries, Ehrlichia isolation & purification, Ehrlichiosis diagnosis
Abstract

A clinical case of human granulocytic ehrlichiosis in Scandinavia is presented. The patient developed high fever, myalgia, headache and dyspnoea. Doxycycline treatment resulted in a dramatic improvement. Laboratory confirmation included a fourfold change in anti-Ehrlichia equi IFA titre and a positive PCR confirmed by gene sequence analysis.

Published
2001
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28. Detection and differentiation of old world orthopoxviruses: restriction fragment length polymorphism of the crmB gene region.

Author

Loparev VN, Massung RF, Esposito JJ, and Meyer H

Subjects
Humans, Orthopoxvirus genetics, Polymerase Chain Reaction methods, Poxviridae Infections virology, Orthopoxvirus classification, Orthopoxvirus isolation & purification, Polymorphism, Restriction Fragment Length, Poxviridae Infections diagnosis, Receptors, Tumor Necrosis Factor genetics, Viral Proteins genetics
Abstract

A restriction fragment length polymorphism (RFLP) assay was developed to identify and differentiate Old World, African-Eurasian orthopoxviruses (OPV): variola, vaccinia, cowpox, monkeypox, camelpox, ectromelia, and taterapox viruses. The test uses amplicons produced from virus genome DNA by PCR with a consensus primer pair designed from sequences determined for the cytokine response modifier B (crmB) gene of 43 different OPV strains of known taxonomic origin. The primer pair amplified a single specific product from each of the 115 OPV samples tested. Size-specific amplicons identified and differentiated ectromelia and vaccinia virus strains, which contain a truncated crmB gene, and enabled their differentiation from other OPV species. Restriction digests of amplified products allowed the identification and differentiation of variola, monkeypox, camelpox, vaccinia, and cowpox virus species and strains.

Published
2001
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29. Coinfection with Borrelia burgdorferi and the agent of human granulocytic ehrlichiosis suppresses IL-2 and IFN gamma production and promotes an IL-4 response in C3H/HeJ mice.

Author

Zeidner NS, Dolan MC, Massung R, Piesman J, and Fish D

Subjects
Animals, Borrelia burgdorferi Group genetics, Cytokines immunology, Cytokines metabolism, Ehrlichia genetics, Ehrlichiosis complications, Ehrlichiosis transmission, Flow Cytometry, Humans, Interferon-gamma biosynthesis, Interleukin-2 biosynthesis, Interleukin-4 biosynthesis, Ixodes microbiology, Lyme Disease complications, Lyme Disease transmission, Mice, Mice, Inbred C3H, Polymerase Chain Reaction, Spleen cytology, Spleen immunology, Spleen microbiology, Borrelia burgdorferi Group immunology, Cytokines biosynthesis, Ehrlichia immunology, Ehrlichiosis immunology, Lyme Disease immunology, Th2 Cells immunology
Abstract

Previously we demonstrated that Borrelia burgdorferi transmission by Ixodes scapularis suppressed IL-2 and IFN gamma production and promoted IL-4 production in mice. The present studies were conducted to determine whether coinfection with the human granulocytic ehrlichiosis (HE) agent would promote a Th2 cytokine response in mice. Transmission to the spleen of the agent of human granulocytic ehrlichiosis (aoHGE) and B. burgdorferi occurred 4 and 7 days, respectively, after tick infestation. Coinfection synergized to suppress splenic IL-2 production 7-14 days after tick infestion. Transmission of B. burgdorferi or aoHGE alone significantly decreased splenic IFN gamma 4-7 days after tick infestation, while coinfection suppressed IFN gamma production 7-14 days after tick infestation. Splenic IL-4 production was significantly increased 4 days after coinfection, and by day 10, aoHGE plus B. burgdorferi induced greater splenic IL-4 (57.2 pg/ml, 348% of control values) than either organism transmitted alone (aoHGE, 22.7 pg/ml, B. burgdorferi, 25.1 pg/ml). Coinfection enhanced expansion of splenic T cells, CD4+ lymphocytes and B cells while decreasing CD8+ T cells. These data demonstrate that aoHGE and B. burgdorferi, when cotransmitted, suppress a systemic IL-2 and IFN gamma response, while strongly promoting systemic IL-4 production in the susceptible host. The antigen(s) responsible for this polarization are unknown and will be the subject of future studies.

Published
2000
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30. Transmission of the agent of human granulocytic ehrlichiosis by Ixodes spinipalpis ticks: evidence of an enzootic cycle of dual infection with Borrelia burgdorferi in Northern Colorado.

Author

Zeidner NS, Burkot TR, Massung R, Nicholson WL, Dolan MC, Rutherford JS, Biggerstaff BJ, and Maupin GO

Subjects
Animals, Colorado epidemiology, Ehrlichiosis epidemiology, Granulocytes, Humans, Incidence, Lyme Disease epidemiology, Disease Reservoirs, Ehrlichiosis transmission, Ixodes, Lyme Disease transmission, Rodentia
Abstract

Previous work described an enzootic cycle of Borrelia burgdorferi sensu lato (hereafter referred to as B. burgdorferi) maintained by the rodent Neotoma mexicana and the tick Ixodes spinipalpis in northern Colorado. We investigated the incidence of coinfection among rodents with the agent of human granulocytic ehrlichiosis (aoHGE). aoHGE was detected in 23.5% of 119 rodent spleens examined. Biopsy results indicated that 78 (65.5%) of the 119 rodents were positive for B. burgdorferi, whereas 22 (78.5%) of the 28 animals that harbored aoHGE were also infected with B. burgdorferi. In 14 of 25 I. spinipalpis tick pools, aoHGE was detected by amplifying both the 16s rRNA and p44 gene of aoHGE. The ability of I. spinipalpis to transmit aoHGE was examined in C3H/HeJ mice. aoHGE was detected in their blood 5 days after I. spinipalpis infestation. This study confirms that both B. burgdorferi and aoHGE can be transmitted by I. spinipalpis ticks and that there is a high incidence of coinfection in rodents, predominantly Peromyscus maniculatus and N. mexicana, that inhabit the foothills of northern Colorado.

Published
2000
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31. The gene encoding the 17-kDa antigen of Bartonella henselae is located within a cluster of genes homologous to the virB virulence operon.

Author

Padmalayam I, Karem K, Baumstark B, and Massung R

Subjects
Animals, Bartonella henselae immunology, Cloning, Molecular, Gene Library, In Situ Hybridization, Mice, Molecular Sequence Data, Multigene Family, Open Reading Frames, Operon, Sequence Analysis, Sequence Homology, Nucleic Acid, Virulence genetics, Antigens, Bacterial genetics, Bacterial Proteins genetics, Bartonella henselae genetics, Bartonella henselae pathogenicity, Virulence Factors
Abstract

A Bartonella henselae genomic A library was screened with antiserum generated in mice against live B. henselae. One of the immunoreactive clones expressed a 17-kDa antigen that was characterized previously as an immunodominant protein of B. henselae. Sequence analysis of the recombinant clone, pBHIM-2, revealed that the open reading frame (ORF) encoding the 17-kDa antigen was situated between homologs of virB4 and virB6, two genes that belong to the virB operon. The virB operon has been associated with the transfer of oncogenic T-DNA in Agrobacterium tumefaciens and with secretion of the pertussis toxin in Bordetella pertussis. Downstream of the virB6 gene within pBHIM-2 was a partial open reading frame that was homologous to the virB8 gene. Rescreening of the library by plaque hybridization using probes specific to the 5' and 3' ends of the pBHIM-2 insert resulted in the isolation of recombinant clones containing additional virB genes. Assembly of the sequences obtained from the recombinant clones revealed that eight of the open reading frames encode homologs of the VirB proteins. The homology and colinearity with the virB genes suggest that the gene encoding the 17-kDa antigen is expressed within the virB locus of B. henselae.

Published
2000
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32. PCR detection of granulocytic ehrlichiae in Ixodes ricinus ticks and wild small mammals in western Switzerland.

Author

Liz JS, Anderes L, Sumner JW, Massung RF, Gern L, Rutti B, and Brossard M

Subjects
Animals, Animals, Wild, Arvicolinae parasitology, Borrelia burgdorferi Group isolation & purification, Cattle, DNA, Bacterial analysis, Ehrlichia classification, Ehrlichia genetics, Ehrlichiosis diagnosis, Female, Geography, Humans, Larva, Male, Molecular Sequence Data, Muridae parasitology, Polymerase Chain Reaction, Shrews parasitology, Switzerland, Ehrlichia isolation & purification, Ehrlichiosis veterinary, Ixodes microbiology, Mammals parasitology
Abstract

The presence of granulocytic ehrlichiae was demonstrated by PCR in Ixodes ricinus ticks and wild small mammals in Switzerland in two areas of endemicity for bovine ehrlichiosis. Six ticks (three females and three nymphs) (1.4%) of 417 I. ricinus ticks collected by flagging vegetation contained ehrlichial DNA. A total of 201 small mammals from five species, wood mouse (Apodemus sylvaticus), yellow-necked mouse (Apodemus flavicollis), earth vole (Pitymys subterraneus), bank vole (Clethrionomys glareolus), and common shrew (Sorex araneus), were trapped. The analysis of I. ricinus ticks [corrected] collected on 116 small mammals showed that nine C. glareolus voles and two A. sylvaticus mice hosted infected tick larvae. In these rodents, granulocytic ehrlichia infection was also detected in blood, spleen, liver, and ear samples. Further examinations of 190 small mammals without ticks or with noninfected ticks showed the presence of ehrlichial DNA in spleen and other tissues from six additional C. glareolus, three A. flavicollis, and one S. araneus mammals. This study suggests that A. sylvaticus, A. flavicollis, S. araneus, and particularly C. glareolus are likely to be natural reservoirs for granulocytic ehrlichiae. Partial 16S rRNA gene sequences of granulocytic ehrlichiae from ticks and rodents showed a high degree of homology (99 to 100%) with granulocytic ehrlichiae isolated from humans. In contrast, groESL heat shock operon sequence analysis showed a strong divergence (approximately 5%) between the sequences in samples derived from rodents and those derived from samples from questing ticks or from other published ehrlichia sequences. Dual infections with granulocytic ehrlichia and Borrelia burgdorferi were found in ticks and small mammals.

Published
2000
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33. Alastrim smallpox variola minor virus genome DNA sequences.

Author

Shchelkunov SN, Totmenin AV, Loparev VN, Safronov PF, Gutorov VV, Chizhikov VE, Knight JC, Parsons JM, Massung RF, and Esposito JJ

Subjects
3-Hydroxysteroid Dehydrogenases genetics, Amino Acid Sequence, Ankyrin Repeat, Base Sequence, Cell Line, Cowpox virus genetics, DNA-Binding Proteins genetics, Humans, Infant, Newborn, Molecular Sequence Data, Open Reading Frames, Orthopoxvirus genetics, Sequence Homology, Amino Acid, Transcription Factors genetics, Vaccinia virus genetics, Viral Proteins genetics, DNA, Viral genetics, Genome, Viral, Variola virus genetics
Abstract

Alastrim variola minor virus, which causes mild smallpox, was first recognized in Florida and South America in the late 19th century. Genome linear double-stranded DNA sequences (186,986 bp) of the alastrim virus Garcia-1966, a laboratory reference strain from an outbreak associated with 0.8% case fatalities in Brazil in 1966, were determined except for a 530-bp fragment of hairpin-loop sequences at each terminus. The DNA sequences (EMBL Accession No. Y16780) showed 206 potential open reading frames for proteins containing >/=60 amino acids. The amino acid sequences of the putative proteins were compared with those reported for vaccinia virus strain Copenhagen and the Asian variola major strains India-1967 and Bangladesh-1975. About one-third of the alastrim viral proteins were 100% identical to correlates in the variola major strains and the remainder were >/=95% identical. Compared with variola major virus DNA, alastrim virus DNA has additional segments of 898 and 627 bp, respectively, within the left and right terminal regions. The former segment aligns well with sequences in other orthopoxviruses, particularly cowpox and vaccinia viruses, and the latter is apparently alastrim-specific., (Copyright 2000 Academic Press.)

Published
2000
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34. Infection with agents of human granulocytic ehrlichiosis, lyme disease, and babesiosis in wild white-footed mice (Peromyscus leucopus) in Connecticut.

Author

Stafford KC 3rd, Massung RF, Magnarelli LA, Ijdo JW, and Anderson JF

Subjects
Animals, Antibodies, Bacterial blood, DNA, Bacterial blood, Ehrlichiosis microbiology, HL-60 Cells, Humans, Lyme Disease microbiology, Mice, Mice, Inbred C3H, Polymerase Chain Reaction, Babesiosis parasitology, Ehrlichiosis veterinary, Lyme Disease veterinary, Peromyscus microbiology, Peromyscus parasitology
Abstract

White-footed mice, Peromyscus leucopus, were captured in southern Connecticut during 1997 and 1998 to determine the prevalence of infections caused by granulocytic Ehrlichia sp., Borrelia burgdorferi, and Babesia microti. Of the 50 mice captured and recaptured, 25 of 47 (53.2%) and 23 of 48 (47.9%) contained antibodies to the BDS or NCH-1 Ehrlichia strains, respectively, as determined by indirect fluorescent antibody (IFA) staining methods. The majority (83.3%) of 48 mice also contained antibodies to B. burgdorferi, as determined by enzyme-linked immunosorbent assay. Moreover, 20 of 26 (76.9%) contained antibodies to B. microti by IFA staining methods. In nested PCR tests using the 16S rRNA gene, the DNA of the human granulocytic ehrlichiosis (HGE) agent was detected in 17 of 47 mice (36.2%), but only 4 (23.5%) of these 17 mice were PCR positive at each capture. Antibody-positive reactions to granulocytic Ehrlichia sp. organisms were detected in 17 of 23 (73. 9%) of the PCR-positive mice. The sequences from PCR products from nine positive blood samples were identical to the HGE agent. Ehrlichia spp. were cultured from three of five mice captured in April 1998, including one that was PCR positive in April 1997. In addition, 2 of 14 larval Ixodes scapularis pools, which were attached to two PCR-positive mice, contained DNA of the HGE agent. A high percentage of white-footed mice are infected or have been infected naturally by the HGE agent with low-level persistent infection or frequent reinfection in some individual mice. However, the changes noted in the presence of DNA and antibodies in repeated blood and serum samples from individual mice over several months of field collection suggests that infection with granulocytic Ehrlichia is transient in most wild P. leucopus.

Published
1999
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35. Outcome of diagnostic tests using samples from patients with culture-proven human monocytic ehrlichiosis: implications for surveillance.

Author

Childs JE, Sumner JW, Nicholson WL, Massung RF, Standaert SM, and Paddock CD

Subjects
Fluorescent Antibody Technique, Indirect, Humans, Immunoglobulin G blood, Immunoglobulin M blood, Polymerase Chain Reaction, Antibodies, Bacterial blood, Ehrlichia chaffeensis immunology, Ehrlichiosis diagnosis
Abstract

We describe the concordance among results from various laboratory tests using samples derived from nine culture-proven cases of human monocytic ehrlichiosis (HME) caused by Ehrlichia chaffeensis. A class-specific indirect immunofluorescence assay for immunoglobulin M (IgM) and IgG, using E. chaffeensis antigen, identified 44 and 33% of the isolation-confirmed HME patients on the basis of samples obtained at initial clinical presentation, respectively; detection of morulae in blood smears was similarly insensitive (22% positive). PCR amplifications of ehrlichial DNA targeting the 16S rRNA gene, the variable-length PCR target gene, and the groESL operon were positive for whole blood specimens obtained from all patients at initial presentation. As most case definitions of HME require a serologic response with compatible illness for a categorization of even probable disease, PCR would have been required to confirm the diagnosis of HME in all nine of these patients without the submission of a convalescent-phase serum sample. These data suggest that many, if not most, cases of HME in patients who present early in the course of the disease may be missed and underscore the limitations of serologically based surveillance systems.

Published
1999
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36. Ehrlichial meningitis with cerebrospinal fluid morulae.

Author

Berry DS, Miller RS, Hooke JA, Massung RF, Bennett J, and Ottolini MG

Subjects
Child, Ehrlichiosis diagnosis, Humans, Male, Meningitis, Bacterial diagnosis, Ehrlichia isolation & purification, Ehrlichiosis cerebrospinal fluid, Meningitis, Bacterial cerebrospinal fluid
Published
1999
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37. Serological evidence of Ehrlichia infection in Swedish Lyme borreliosis patients.

Author

Bjöersdorff A, Brouqui P, Eliasson I, Massung RF, Wittesjö B, and Berglund J

Subjects
Acute Disease, Adolescent, Adult, Aged, Aged, 80 and over, Animals, Cattle, Child, Child, Preschool, Ehrlichia classification, Ehrlichia genetics, Ehrlichiosis epidemiology, Ehrlichiosis microbiology, Female, Fluorescent Antibody Technique, Indirect, Humans, Immunoglobulin G blood, Lyme Disease epidemiology, Male, Middle Aged, Polymerase Chain Reaction, Prospective Studies, Sweden epidemiology, Tick-Borne Diseases epidemiology, Tick-Borne Diseases microbiology, Antibodies, Bacterial blood, Ehrlichia immunology, Ehrlichiosis immunology, Lyme Disease immunology, Tick-Borne Diseases immunology
Abstract

We studied sera from patients who had participated in a prospective study of borreliosis in Sweden and had acquired tick bites in areas of the country with a high prevalence of granulocytic ehrlichial infections in animals. The sera were examined for IgG anti Ehrlichia antibodies by an indirect immunofluorescence assay using a locally isolated bovine Ehrlichia antigen. Confirmation of the serological results was done at the Unité des Rickettsies, Marseille, France. Three out of 37 of the investigated patients and 1 out of 100 investigated healthy blood donors had significant antibody titres to granulocytotropic Ehrlichiae. No patient or blood donor had specific antibody titres to Ehrlichia chaffeensis. These data suggest that Scandinavian Ehrlichia species can infect and evoke immunological response in tick-exposed humans.

Published
1999
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38. Nested PCR assay for detection of granulocytic ehrlichiae.

Author

Massung RF, Slater K, Owens JH, Nicholson WL, Mather TN, Solberg VB, and Olson JG

Subjects
Animals, DNA, Bacterial analysis, DNA, Bacterial chemistry, DNA, Ribosomal chemistry, Humans, RNA, Ribosomal, 16S genetics, Sensitivity and Specificity, Ticks microbiology, Ehrlichia isolation & purification, Granulocytes microbiology, Polymerase Chain Reaction
Abstract

A sensitive and specific nested PCR assay was developed for the detection of granulocytic ehrlichiae. The assay amplifies the 16S rRNA gene and was used to examine acute-phase EDTA-blood and serum samples obtained from seven humans with clinical presentations compatible with human granulocytic ehrlichiosis. Five of the seven suspected cases were positive by the PCR assay using DNA extracted from whole blood as the template, compared with a serologic assay that identified only one positive sample. The PCR assay using DNA extracted from the corresponding serum samples as the template identified three positive samples. The sensitivity of the assay on human samples was examined, and the limit of detection was shown to be fewer than 2 copies of the 16S rRNA gene. The application of the assay to nonhuman samples demonstrated products amplified from template DNA extracted from Ixodes scapularis ticks collected in Rhode Island and from EDTA-blood specimens obtained from white-tailed deer in Maryland. All PCR products were sequenced and identified as specific to granulocytic ehrlichiae. A putative variant granulocytic ehrlichia 16S rRNA gene sequence was detected among products amplified from both the ticks and the deer blood specimens.

Published
1998
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39. Terminal region sequence variations in variola virus DNA.

Author

Massung RF, Loparev VN, Knight JC, Totmenin AV, Chizhikov VE, Parsons JM, Safronov PF, Gutorov VV, Shchelkunov SN, and Esposito JJ

Subjects
Africa, Asia, Base Sequence, Brazil, Humans, Molecular Sequence Data, Open Reading Frames, Repetitive Sequences, Nucleic Acid, Sequence Homology, Nucleic Acid, Variola virus isolation & purification, Viral Proteins genetics, DNA, Viral, Genetic Variation, Variola virus genetics
Abstract

Genome DNA terminal region sequences were determined for a Brazilian alastrim variola minor virus strain Garcia-1966 that was associated with an 0.8% case-fatality rate and African smallpox strains Congo-1970 and Somalia-1977 associated with variola major (9.6%) and minor (0.4%) mortality rates, respectively. A base sequence identity of > or = 98.8% was determined after aligning 30 kb of the left- or right-end region sequences with cognate sequences previously determined for Asian variola major strains India-1967 (31% death rate) and Bangladesh-1975 (18.5% death rate). The deduced amino acid sequences of putative proteins of > or = 65 amino acids also showed relatively high identity, although the Asian and African viruses were clearly more related to each other than to alastrim virus. Alastrim virus contained only 10 of 70 proteins that were 100% identical to homologs in Asian strains, and 7 alastrim-specific proteins were noted.

Published
1996
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40. Topography of variola smallpox virus inverted terminal repeats.

Author

Massung RF, Knight JC, and Esposito JJ

Subjects
Africa epidemiology, Asia epidemiology, Base Sequence, DNA, Viral chemistry, DNA, Viral genetics, DNA, Viral isolation & purification, Disease Outbreaks, Europe epidemiology, Genome, Viral, Humans, Molecular Sequence Data, Smallpox epidemiology, South America epidemiology, Variola virus isolation & purification, Repetitive Sequences, Nucleic Acid, Smallpox virology, Variola virus genetics
Abstract

We examined the nucleotide sequences of the inverted terminal repeat (ITR) regions adjacent to the covalently closed hairpin end sequences of three variola major and four minor strains from smallpox outbreaks in Europe, Asia, Africa, and South America. The ITR regions ranged in size from 581 to 1051 base pairs (bp) and contained no apparent open reading frames. Two nonrepetitive sequence elements, NR1 and NR2, were conserved and resembled nonrepetitive elements in the ITRs of other orthopoxviruses. Depending on strain, the terminally positioned NR1 and the more internal NR2 flanked a direct repeat region containing from none to four copies of a 69-bp sequence and one copy of a 54-bp related sequence partial repeat. A distinctive pattern of ITR topography of NR1 and NR2 flanking a single copy of the 69-bp unit characterized each of three examined alastrim variola minor strains. A nonalastrim African minor strain from the last natural case of smallpox in Somalia in 1977 showed the largest ITR region of the examined viruses because of a second direct repeat cluster following NR2.

Published
1995
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41. Analysis of the complete genome of smallpox variola major virus strain Bangladesh-1975.

Author

Massung RF, Liu LI, Qi J, Knight JC, Yuran TE, Kerlavage AR, Parsons JM, Venter JC, and Esposito JJ

Subjects
Animals, Bangladesh, Base Sequence, Chick Embryo, Child, Preschool, Conserved Sequence, DNA, Viral, Female, Genetic Variation, Humans, Molecular Sequence Data, Open Reading Frames, Protein Kinases genetics, Receptors, Cytokine genetics, Repetitive Sequences, Nucleic Acid, Restriction Mapping, Species Specificity, Variola virus classification, Variola virus isolation & purification, Variola virus pathogenicity, Viral Envelope Proteins genetics, Viral Proteins genetics, Genome, Viral, Smallpox microbiology, Variola virus genetics
Abstract

We analyzed the 186,102 base pairs (bp) that constitute the entire DNA genome of a highly virulent variola virus isolated from Bangladesh in 1975. The linear, double-stranded molecule has relatively small (725 bp) inverted terminal repeat (ITR) sequences containing three 69-bp direct repeat elements, a 54-bp partial repeat element, and a 105-base telomeric end-loop that can be maximally base-paired to contain 17 mismatches. Proximal to the right-end ITR sequences are another seven 69-bp elements and a 53- and a 27-bp partial element. Sequence analysis showed 187 closely spaced open reading frames specifying putative major proteins containing > or = 65 amino acids. Most of the virus proteins correspond to proteins in current databases, including 150 proteins that have > 90% identity to major gene products encoded by vaccinia virus, the smallpox vaccine. Variola virus has a group of proteins that are truncated compared with vaccinia virus counterparts and a smaller group of proteins that are elongated. The terminal regions encode several novel proteins and variants of other poxvirus proteins that potentially augment variola virus transmissibility and virulence for its only natural host, humans.

Published
1994
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42. Potential virulence determinants in terminal regions of variola smallpox virus genome.

Author

Massung RF, Esposito JJ, Liu LI, Qi J, Utterback TR, Knight JC, Aubin L, Yuran TE, Parsons JM, and Loparev VN

Subjects
Animals, Humans, Molecular Sequence Data, Restriction Mapping, Sequence Homology, Amino Acid, Sequence Homology, Nucleic Acid, Vaccinia virus genetics, Variola virus genetics, Viral Proteins physiology, Virulence, DNA, Viral genetics, Genome, Viral, Variola virus pathogenicity
Abstract

Smallpox eradication culminated the most successful antimicrobial campaign in medical history. To characterize further the linear double-stranded DNA genome of the aetiological agent of smallpox, we have determined the entire nucleotide sequence of the highly virulent variola major virus, strain Bangladesh-1975 (VAR-BSH; 186,102 base pairs, 33.7% G + C; Genbank accession number, L22579). Here we highlight features of the molecule and focus on a few of the 187 putative proteins that probably contribute to pathogenicity and virus host-range properties. One hundred and fifty proteins were markedly similar to those of vaccinia virus (smallpox vaccine), for which a complete sequence has been reported for strain Copenhagen (VAC-CPN; 191,636 base pairs, 33.3% G + C). The remaining 37 proteins reflected variola-specific sequences or open reading frame divergences for variant proteins, which are often truncated or elongated compared with their vaccinia counterparts.

Published
1993
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43. DNA sequence analysis of conserved and unique regions of swinepox virus: identification of genetic elements supporting phenotypic observations including a novel G protein-coupled receptor homologue.

Author

Massung RF, Jayarama V, and Moyer RW

Subjects
Amino Acid Sequence, Base Sequence, Conserved Sequence, Genome, Viral, Molecular Sequence Data, Open Reading Frames, Regulatory Sequences, Nucleic Acid, Restriction Mapping, Sequence Analysis, DNA, Sequence Homology, Amino Acid, Time Factors, Transcription, Genetic, GTP-Binding Proteins genetics, Genes, Viral genetics, Suipoxvirus genetics
Abstract

Swinepox virus (SPV) contains a double-stranded cross-linked linear DNA genome of approximately 175 kilobase pairs with terminal inverted repetitions (TIRs) of 4.3 kb. The nucleotide sequence was determined for fragments from several regions of the genome including a 2.85-kb fragment from the central potentially conserved portion and two fragments within the presumed variable near-terminal regions which tend to be unique to a given poxvirus. The core sequence contains one partial and two complete open reading frames that are highly conserved and colinear with three contiguous ORFs within the HindIII D fragment of vaccinia virus (VV). The two near-terminal fragments, encompassing 14.2 and 3.6 kb, are respectively located 2.1 kb internal to the left and right cross-linked termini of the DNA and span the TIR junctions. The sequences encode 25 open reading frames including numerous proteins predicted to be membrane-bound or secreted in infected cells. Several ORFs unique to SPV were identified that may be involved in cell attachment, immune modulation, and pathogenesis including a novel poxvirus G protein-coupled receptor. In addition, several polypeptides encoded within the near-terminal regions of vaccinia virus DNA that function as host range or virulence factors are lacking within this region of swinepox virus including the VV growth factor, complement-binding protein, and ORFs C7L and K1L, associated with host range. The lack of these functional homologues could explain the characteristic attenuated phenotype and limited host range of SPV.

Published
1993
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44. Nucleotide sequence analysis of a unique near-terminal region of the tumorigenic poxvirus, Shope fibroma virus.

Author

Massung RF, McFadden G, and Moyer RW

Subjects
Amino Acid Sequence, Ankyrins genetics, Base Sequence, Molecular Sequence Data, Open Reading Frames, Repetitive Sequences, Nucleic Acid genetics, Sequence Homology, Amino Acid, Vaccinia virus genetics, DNA, Viral genetics, Fibroma Virus, Rabbit genetics, Genes, Viral genetics
Abstract

Shope fibroma virus (SFV), a tumorigenic poxvirus, has a DNA genome of approximately 160 kb. Previous DNA sequence analysis of SFV has been mainly limited to the terminal inverted repetitions (about 12 kb at each end of the genome) and immediately adjacent regions. We have sequenced a 4 kb fragment located approximately 20 kb from the right-terminal hairpin. Within this region three complete and two partial open reading frames (ORFs) have been identified. Each of the putative polypeptides has sequence similarity to one or more previously identified poxvirus or cellular proteins, with homology to protein kinases, erythrocyte ankyrin and a vaccinia virus virulence-related protein (ORF N1L). The potential significance of these gene products with regard to the phenotype of SFV is discussed.

Published
1992
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45. Isolation and molecular characterization of the swinepox virus thymidine kinase gene.

Author

Feller JA, Massung RF, Turner PC, Gibbs EP, Bockamp EO, Beloso A, Talavera A, Viñuela E, and Moyer RW

Subjects
Amino Acid Sequence, Animals, Base Sequence, Bromodeoxyuridine pharmacology, Chromosome Mapping, Cloning, Molecular, DNA, Viral, Drug Resistance, Microbial genetics, Gene Expression, Genes, Viral, Humans, Molecular Sequence Data, Mutation, Open Reading Frames, Poxviridae enzymology, Sequence Alignment, Thymidine Kinase metabolism, Transcription, Genetic, Vaccinia virus genetics, Poxviridae genetics, Thymidine Kinase genetics
Abstract

Swinepox virus (SPV), the only member of the Suipoxvirus genus, shows little antigenic relatedness or DNA homology to members of the other poxvirus genera. A SPV thymidine kinase (TK) gene was detected and mapped to the left end of the HindIII G fragment using degenerate oligonucleotide probes. Cloning and sequencing of a 1.8-kb HindIII-BamHI fragment containing the SPV TK gene revealed an open reading frame (ORF) of 181 amino acids yielding a predicted polypeptide of Mr 20.6 kDa with significant homology to both poxvirus and vertebrate thymidine kinases. Comparison with other TK protein sequences showed that the SPV thymidine kinase was closely related to the TK genes of avipoxviruses (52.0%) and vertebrates (57.1-59.7%). The TK gene from African swine fever virus (ASF) showed little homology (30.5%) to the SPV TK gene suggesting that these two viruses are not closely related though they share many biochemical features and infect a single, common mammalian host (swine). The SPV TK gene, like that of other poxviruses, is transcribed early, and when cloned into a TK- strain of vaccinia converted the virus to a TK+ phenotype. BUdRR mutants of SPV contained frameshift, deletion, and missense mutations in the TK ORF.

Published
1991
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46. The molecular biology of swinepox virus. I. A characterization of the viral DNA.

Author

Massung RF and Moyer RW

Subjects
Animals, Blotting, Southern, Cells, Cultured, Electrophoresis, Polyacrylamide Gel, Genes, Viral genetics, Molecular Weight, Nucleic Acid Hybridization, Poxviridae growth & development, Repetitive Sequences, Nucleic Acid, Restriction Mapping, DNA, Viral genetics, Poxviridae genetics
Abstract

Swinepox virus (SPV), the prototype member of the Suipoxvirus genus, is uncharacterized at the molecular level. We have analyzed the DNA of SPV and demonstrate that the genome is 175 kb in size and like the more commonly studied Orthopoxvirus, Avipoxvirus, and Leporipoxvirus genera, is terminally cross-linked and contains inverted terminal repetitions (ITRs). In addition, the ITRs are unstable, probably due to the presence of a variable number of direct repeats of approximately 70 bp in length. Restriction enzyme cleavage maps for the enzymes HindIII, AvaI, HaeII, KpnI, BglI, SalI, and XhoI are also presented.

Published
1991
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47. The molecular biology of swinepox virus. II. The infectious cycle.

Author

Massung RF and Moyer RW

Subjects
Animals, Antigens, Viral immunology, Blotting, Northern, Blotting, Southern, Cell Line, Cross Reactions, Cytopathogenic Effect, Viral, DNA, Viral biosynthesis, DNA, Viral genetics, DNA, Viral isolation & purification, Electrophoresis, Polyacrylamide Gel, Nucleic Acid Hybridization, Poxviridae classification, RNA, Messenger genetics, RNA, Viral biosynthesis, RNA, Viral isolation & purification, RNA, Viral metabolism, Vaccinia virus genetics, Viral Proteins metabolism, Poxviridae physiology, Poxviridae Infections microbiology
Abstract

Studies based on low-stringency hybridizations of radiolabeled swinepox virus (SPV) DNA to Southern blots containing DNA of representative members of the Orthopoxvirus, Leporipoxvirus, and Avipoxvirus genera and the Entomopoxvirus subfamily have revealed no DNA homology at this level of resolution. Antigenic relatedness between SPV and vaccinia was also analyzed using immunoprecipitations and revealed little if any cross-reactivity. The growth characteristics of SPV in tissue culture were examined by light microscopy and revealed both a delayed and a different cytopathology than that of vaccinia virus. SPV causes foci in pig kidney cells that are not evident until at least 4 days postinfection, whereas vaccinia rapidly generates plaques on these cells. The kinetics of DNA accumulation, protein expression, and RNA transcription of SPV have been examined and indicate that each of these facets of the SPV growth cycle is also considerably delayed when compared to vaccinia virus. Our data indicate that swinepox virus is unique from other poxviruses characterized to date and supports the classification of swinepox virus into a separate genus, Suipoxvirus, within the poxvirus family.

Published
1991
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48. Recruitment to the cytoplasm of a cellular lamin-like protein from the nucleus during a poxvirus infection.

Author

Bloom DC, Massung R, Savage L, Morrison DK, and Moyer RW

Subjects
Amino Acid Sequence, Animals, Antibodies, Monoclonal, Base Sequence, Carcinoma, Cell Line, Cell Nucleus analysis, Cytoplasm analysis, DNA analysis, DNA genetics, Fluorescent Antibody Technique, Humans, Immunoblotting, Lamins, Lung Neoplasms, Molecular Sequence Data, Molecular Weight, Nuclear Proteins genetics, Recombinant Fusion Proteins analysis, Recombinant Fusion Proteins genetics, Repetitive Sequences, Nucleic Acid, Tumor Cells, Cultured, Vaccinia virus physiology, Nuclear Proteins analysis, Poxviridae genetics, Vaccinia virus genetics
Abstract

Monoclonal antibodies (Mabs) directed against core proteins of rabbit poxvirus (RPV) have proven effective in the identification of host cell proteins such as RNA polymerase II (Pol II) that may play a role in the infectious process (D. K. Morrison and R. W. Moyer, 1986, Cell 44, 587-596). In this article we describe a Mab that has allowed the detection and characterization of a lamin-like protein derived from the nucleus of the infected cell, which like Pol II is recruited to the cytoplasm following RPV infection. A portion of the gene encoding this protein has been isolated through the screening of a lambda gt11 expression vector library. Sequence analysis of the gene shows it to be derived from a member of the HindIII 1.9-kb repetitive element, a family of mammalian repetitive sequences that are highly conserved. Immunoblot analysis and sequence analysis of the open reading frame show divergent relatedness to certain nuclear lamins. The protein is not, however, one of the three principal lamins characterized to date, but instead appears to be a perinuclear protein related to the highly conserved nuclear lamins that is recruited to the cytoplasm during the infectious process.

Published
1989
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49. Human H1 histone gene promoter CCAAT box binding protein HiNF-B is a mosaic factor.

Author

van Wijnen AJ, Massung RF, Stein JL, and Stein GS

Subjects
Animals, Base Sequence, Cell Nucleus metabolism, DNA Probes, Genetic Vectors, Humans, Mice, Molecular Sequence Data, CCAAT-Enhancer-Binding Proteins, DNA-Binding Proteins metabolism, Genes, Histones genetics, Mosaicism, Promoter Regions, Genetic
Abstract

Vertebrate histone gene promoters in many cases contain an upstream element, 5'dCCAAT, that has been implicated in modulating the efficiency of transcription of a broad spectrum of genes. We have previously isolated a nuclear factor (HiNF-B) that binds specifically to the CCAAT element of a cell cycle regulated human H1 histone gene. This factor shows similarities with other CCAAT box binding proteins in that it recognizes the same sequence but shows a distinct chromatographic behavior. In the present study, we have employed the gel retardation assay to demonstrate that HiNF-B is a cell cycle independent DNA binding protein that is conserved in both human and mouse cells. Using a series of reconstitution experiments with partially purified HiNF-B fractions, we show that this factor requires association of at least two components for site-specific binding. The composite structure of HiNF-B suggests that binding of at least some CCAAT elements in vertebrates may require cooperative interaction of CCAAT box binding proteins with other factors.

Published
1988
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50. Two target sites for protein binding in the promoter region of a cell cycle regulated human H1 histone gene.

Author

van Wijnen AJ, Wright KL, Massung RF, Gerretsen M, Stein JL, and Stein GS

Subjects
Base Sequence, Cloning, Molecular, DNA-Binding Proteins isolation & purification, Endonucleases, Humans, Macromolecular Substances, Molecular Sequence Data, Protein Binding, Single-Strand Specific DNA and RNA Endonucleases, Transcription Factors isolation & purification, Cell Cycle, DNA-Binding Proteins physiology, Histones genetics, Nuclear Proteins physiology, Promoter Regions, Genetic, Regulatory Sequences, Nucleic Acid, Transcription Factors physiology
Abstract

The 5' region of a cell cycle regulated human H1 histone gene appears to contain at least six promoter DNA elements that are shared with some, but not all human core (H2A, H2B, H3 and H4) histone genes. We show that two of these elements represent separate binding sites for two distinct, partially purified factors. The first promoter domain contains A/T rich repeats and is involved in the binding of HiNF-A, a nuclear factor previously found to bind to A/T rich direct repeats in the promoters of human H4 and H3 histone genes. The second domain, containing the general promoter element 5' dACCAAT, acts as a binding site for a two component mosaic factor we have designated HiNF-B. These data suggest that coordinate transcriptional regulation of human H1 and core histone genes may involve two classes of trans-acting factors: those specific for histone gene promoters and those that act on a broad spectrum of human gene promoters.

Published
1988
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