Bartonella henselae in porpoise blood.We report detection of Bartonella henselae DNA DNA: see nucleic acid. DNA or deoxyribonucleic acid One of two types of nucleic acid (the other is RNA); a complex organic compound found in all living cells and many viruses. It is the chemical substance of genes. in blood samples from 2 harbor porpoises (Phocoena phocoena). By using real-time polymerase chain reaction In Molecular Biology, real-time polymerase chain reaction, also called quantitative real time polymerase chain reaction (QRT-PCR) or kinetic polymerase chain reaction , we directly amplified Bartonella species DNA from blood of a harbor porpoise stranded along the northern North Carolina coast and from a pre-enrichment blood culture from a second harbor porpoise. The second porpoise was captured out of habitat (in a low-salinity canal along the northern North Carolina coast) and relocated back into the ocean. Subsequently, DNA was amplified by conventional polymerase chain reaction polymerase chain reaction (pŏl`ĭmərās') (PCR), laboratory process in which a particular DNA segment from a mixture of DNA chains is rapidly replicated, producing a large, readily analyzed sample of a piece of DNA; the process is for DNA sequencing. The 16S-23S intergenic transcribed spacer region obtained from each porpoise was 99.8% similar to that of B. henselae strain San Antonio 2 (SA2), whereas both heme-binding phage-associated pap31 gene sequences were 100% homologous to that of B. henselae SA2. Currently, the geographic distribution, mode of transmission, reservoir potential, and pathogenicity of bloodborne Bartonella species in porpoises have not been determined. ********** Bartonellosis is a newly emerging worldwide zoonotic disease (1,2) that can be caused by a spectrum of Bartonella species. These members of the alpha subdivision of the class Proteobacteria are gram-negative aerobic bacilli and comprise at least 20 species and subspecies. Infection with Bartonella species causes lymphadenopathy lymphadenopathy /lym·phad·e·nop·a·thy/ (-op´ah-the) disease of the lymph nodes. angioimmunoblastic lymphadenopathy , angioimmunoblastic lymphadenopathy with dysproteinemia (3), disorders of the central nervous system (including encephalopathy, hemiplegia hemiplegia /hemi·ple·gia/ (-ple´jah) paralysis of one side of the body.hemiple´gic alternate hemiplegia paralysis of one side of the face and the opposite side of the body. , epilepsy, and subcortical subcortical /sub·cor·ti·cal/ (-kor´ti-k'l) beneath a cortex, such as the cerebral cortex. frontoparietal lesions) (4-7), bacillary angiomatosis and bacillary bacillary /bac·il·la·ry/ (bas´i-lar?e) pertaining to bacilli or to rodlike structures. bac·il·lar·y or ba·cil·lar adj. 1. Shaped like a rod. 2. peliosis (8), fever, adenitis adenitis /ad·e·ni·tis/ (ad?e-ni´tis) inflammation of a gland. Bartholin adenitis inflammation of the greater vestibular gland (Bartholin's gland) resulting from acute infection of the gland. , endocarditis endocarditis (ĕn'dōkärdī`tĭs), bacterial or fungal infection of the endocardium (inner lining of the heart) that can be either acute or subacute. (9-12), hepatosplenic involvement, cutaneous vasculitis, and osteomyelitis in domestic animals and humans (13-15). Bartonella species have been isolated from numerous domestic and wild terrestrial animals, including cats, dogs, deer, cattle, lions, rabbits, and rodents (16-20). Because Bartonella spp. frequently induce persistent intravascular infections, particularly in reservoir hosts, attributing disease causation to Bartonella infection in animals or in human patients has been difficult, and satisfying Koch postulates for disease causation remains challenging (21). Because conventional microbiologic techniques lack sensitivity, bartonellosis is usually diagnosed by using polymerase chain reaction amplification of organism-specific DNA sequences or serologic testing (1,22-25). Recently, a more sensitive isolation approach was developed by using Bartonella alpha Proteobacteria growth medium (BAPGM) followed by real-time polymerase chain reaction (PCR PCR polymerase chain reaction. PCR abbr. polymerase chain reaction Polymerase chain reaction (PCR) ). This method has greatly facilitated the molecular detection or isolation of Bartonella species from the blood of sick and healthy animals (24). The relative sensitivity of diagnostic methods used to detect Bartonella species infection greatly influences the ability to establish disease causation. The use of these optimized microbiologic techniques facilitated the recognition of bloodborne Bartonella spp. infections in porpoises, as reported in this study. We report real-time PCR detection of B. henselae SA2 DNA in porpoise blood samples. Harbor porpoises are cetaceans in the family Phocoenidae that are found alone or in small groups in coastal waters, bays, and estuaries in cold, temperate, and subarctic sub·arc·tic adj. Of or resembling regions just south of the Arctic Circle. subarctic Relating to the geographic area just south of the Arctic Circle. waters of the Northern Hemisphere (26). In the western Atlantic, they range from Baffin Island and Labrador in the north, extending as far south as North Carolina in the winter. Initially, blood samples were screened by using real-time PCR targeting the Bartonella 16S-23S RNA RNA: see nucleic acid. RNA in full ribonucleic acid One of the two main types of nucleic acid (the other being DNA), which functions in cellular protein synthesis in all living cells and replaces DNA as the carrier of genetic intergenic spacer (ITS) region, or the heme-binding phage-associated gene pap31 (27). Preenrichment liquid BAPGM blood cultures were also screened by real-time PCR, after which conventional PCR was used to obtain DNA for sequencing and identifying Bartonella species to the strain level. Materials and Methods Sample Testing Blood samples (anticoagulated with EDTA EDTA: see chelating agents. ) were obtained from a live, stranded yearling female harbor porpoise (Phocoena phocoena) that required humane killing in northern North Carolina in May 2005 (MLC (MultiLevel Cell) A flash memory technology that stores more than one bit per cell. Traditional flash memory defines a 0 or 1 bit based on a single voltage threshold. 001) and from a yearling male harbor porpoise. The male porpoise was captured out of habitat (in a low-salinity canal [3 parts salt per 1,000; by comparison, sea water contains 36 parts per 1,000] along the northern North Carolina coast) and relocated to the ocean in March 2005 (AAH 009). The samples were analyzed as follows. Following DNA extraction, real-time PCR (using DNA probes) and conventional PCR were used to screen for Bartonella DNA in each blood sample (23). A preenrichment culture was established from the original sample by using liquid BAPGM (24). After a 7-day incubation period, a sample was removed from the culture flask for conventional PCR and real-time PCR. In addition, sheep blood (used as blood supplement for preenrichment culture) and a sheep blood preenrichment BAPGM culture were screened for Bartonella DNA as a negative control at the time each porpoise sample was processed. Bartonella DNA was not detected in any control samples. Growth Medium Preenrichment culture of EDTA-anticoagulated blood samples from the 2 porpoises tested in this study was performed as follows. A 1-mL aliquot of blood was added to 10 mL of BAPGM and incubated at 35[degrees]C in a 5% C[O.sub.2], water-saturated atmosphere as previously described (24). DNA Extraction and PCR Screening of Blood and Blood Cultures Screening for Bartonella species DNA was conducted by using conventional PCR and real-time PCR directly with EDTA-anticoagulated blood and from the 7-day postenrichment BAPGM blood culture samples. Gene sequencing was used to establish the species and strain classification. DNA was prepared by using the DNA Mini Kit (Qiagen, Valencia, CA, USA) from 200 [micro]L of the blood sample and from 200 [micro]L of preenrichment blood culture in BAPGM medium. After extraction, DNA concentration and quality were measured by using an absorbance ratio at 260:280 nm. Real-Time PCR Analysis Real-time PCR screening for Bartonella species was performed as described previously (23). Scorpion 321 fluorescent probe 5'-FAM-CCG CGT TTT TCA TCA 1. trichloroacetic acid. 2. tricarboxylic acid cycle (Krebs cycle). TCA Tricyclic antidepressant, see there AAG CCC CCC A very speculative grade assigned to a debt obligation by a rating agency. Such a rating indicates default or considerable doubt that interest will be paid or principal repaid. Also called Caa. ACG ACG American College of Gastroenterology; angiocardiography; apexcardiogram. AcG accelerator globulin (coagulation factor V). AcG accelerator globulin (clotting factor V). CGG-QUE-HEG-AGA TGA TGA TCC CAA Caa See CCC. GCC TTC TGG-3' and oligonucleotide 425as 5'-GGA TRA AYY RGW AAA AAA: see American Automobile Association. (Triple A) A common single-cell battery used in a myriad of electronic devices of all variety. Like its double A (AA) cousin, it provides 1.5 volts of DC power. When used in series, the voltage is multiplied. CCT TYM YCG G-3' were used as sense and antisense primers, respectively, for screening of the Bartonella genus-specific ITS region. Identification of Bartonella species was conducted by using real-time multiplex PCR with species-specific fluorescent probes (Taqman, Appled Biosystems, Foster City, CA, USA) in conjunction with oligonucleotides 321s 5'-AGA TGA TGA TCC CAA GCC TTC TGG CG-3' and 421 as 5'-GGA TRA AYY RGW AAA CCT TYM YCG G-3' as forward and reverse primers (Integrated DNA Technologies, Coralville, IA, USA), respectively. The species-specific fluorescent probe sequences (Taqman) used were 5'-FAM-CCA CCG TGG GCT TTG AAA AAC GCT-3' DBHQ1 for B. henselae, 5'-TexRed-GGG ACT TTA AGG AAG ACA ACA - Application Control Architecture CTT TTG TG-BHQ2-3' for B. quintana, 5'-ROX-TGC ACA AGC CTC TGA GAG GGA TGA ANG ANG In currencies, this is the abbreviation for the NL Antillian Guilder. Notes: The currency market, also known as the Foreign Exchange market, is the largest financial market in the world, with a daily average volume of over US $1 trillion. A-BHQ2-3' for B. clarridgeiae, and Cy3 5'-CTT TCY TGT AAG AGT AGT antiglobulin test. GTA TTT TTT ATC TAA TAA - Track Average Amplitude GA-BHQ2-3' for B. vinsonii subspecies berkhoffii. Real-time reactions were performed by using a SmartCycler II System (Cepheid, Sunnyvale, CA, USA) in 25-[micro]L reaction volumes as described previously (23). Negative controls were prepared by using DNA extracted from sheep blood samples (the same used as blood supplement in BAPG liquid medium). PCR positive controls contained DNA from sheep blood samples spiked with B. clarridgeiae (ATCC ATCC American Type Culture Collection, see there 700095; American Type Culture Collection American Type Culture Collection (ATCC) is a private, not-for-profit biological resource center whose mission focuses on the acquisition, authentication, production, preservation, development and distribution of standard reference microorganisms, cell lines and other materials for , Manassas, VA, USA), Bartonella henselae Houston-1 (ATCC 49882), B. quintana Fuller (ATCC VR-358), or B. vinsonii subsp. berkhoffii (ATCC 51672) DNA to a final concentration of 10 fg/[micro]L. Real-time PCR conditions were a single hot-start cycle at 95[degrees]C for 30 s, followed by 55 cycles of denaturing at 94[degrees]C for 10 s, annealing at 58[degrees]C for 6 s (for Bartonella) or at 60[degrees]C for 6 sec (for the 4 Bartonella species), and final extension at 72[degrees]C for 10 s. Positive amplicons were detected by reading fluorescence at the appropriate wavelength. Conventional PCR Analysis ITS Region PCR screening of the Bartonella 16S-23S ITS region was performed on samples that were positive by real-time PCR, as described (24), when amplicon size allows preliminary species identification. Oligonucleotides 321s 5'-AGA TGA TGA TCC CAA GCC TTC TGG-3' and 983as 5'-TGT TCT YAC YAC yeast artificial chromosome. AAC AAT Alpha-1-antitrypsin (AAT) A blood component that breaks down infection-fighting enzymes such as elastase. Mentioned in: Chronic Obstructive Lung Disease GAT GAT G-3' were used as forward and reverse primers, respectively. The ITS region was amplified in a 25-[micro]L reaction volume that contained 8.5 [micro]L of molecular grade water (Epicentre, Madison, WI, USA) 0.5 [micro]L 10 mmol/L dNTP mixture, 2.5 [micro]L of 10x PCR buffer, 2.5 [micro]L of 25 mmol/L Mg[Cl.sub.2], and 0.7 units of Amplitaq Gold DNA polymerase (Applied Biosystems). The reaction mixture was completed by adding 0.25 [micro]L of 30 [micro]mol/L of each forward and reverse primer (Integrated DNA Technologies) and 10 [micro]L of DNA from each sample tested. PCR negative controls contained 10 [micro]L of DNA extracted from BAPGM (when testing BAPGM cultures) or 10 [micro]L of DNA extracted from sheep blood (when testing blood samples). Conventional PCR conditions were a single hot-start cycle at 95[degrees]C for 5 min, followed by 45 cycles of denaturing at 94[degrees]C for 45 s, annealing at 54[degrees]C for 45 s, and extension at 72[degrees]C for 45 s. Amplification was completed by an additional cycle at 72[degrees]C for 5 min. Products were analyzed by electrophoresis on 2% agarose gels and detected by staining with ethidium bromide and viewing under UV light. Amplicon products were sequenced to identify species strains. pap31 Gene Amplification PCR species screening was performed by using primers designed to amplify a consensus sequence of the phage-associated gene pap31 found in several species of the Bartonella genus (27). Oligonucleotides Pap31 1(s) 5'-GAC TTC TGT TAT CGC TTT GAT TT-3' and Pap31 688 (as) 5'-CAC CAC See Consumer Advisory Council. CAG CAG 1 Chronic atrophic gastritis 2 Coronary angiography, see there CAA MAT AAG GCA T-3' were used as forward and reverse primers, respectively. Amplification of the pap31 gene was performed in a 25[micro]L final volume reaction as described above. PCR conditions for pap31 gene amplification were a single hot-start cycle at 95[degrees]C for 5 min, followed by 45 cycles of denaturing at 94[degrees]C for 45 s, annealing at 58[degrees]C for 45 s, and extension at 72[degrees]C for 45 s. Amplification was completed by an additional cycle at 72[degrees]C for 5 min. Products were analyzed by electrophoresis on 2% agarose gels and detected by staining with ethidium bromide and viewing under UV light. Amplicons were sequenced to identify specific strains. Cloning and Sequencing of ITS and pap31 Gene Amplicons Bartonella ITS and pap31 DNA sequencing was performed for 2 positive amplicons for both the ITS and pap31 gene to confirm the Bartonella species and strain. The amplified PCR products were cloned into the Plasmid pGEM-T Easy Vector System (Promega, Madison, WI, USA). Recombinants (white colonies) were selected on the basis of the right size of the insert in the plasmid using a plasmid miniprep procedure (Qiagen). Sequencing of plasmid inserts was done by Davis Sequencing, Inc. (Davis, CA, USA). Sequence analysis and alignment with GenBank sequences were performed by using AlignX software (Vector NTI Suite 6.0, InforMax, Inc., Frederick, MD, USA) to identify bacteria at species and strain level. Results Blood and Preenrichment Blood Culture Real-Time PCR Following direct extraction from blood, Bartonella DNA was amplified from 1 (MLC 001) of the 2 porpoises. Real-time PCR amplification of Bartonella DNA was possible from the harbor porpoise stranded along the North Carolina coast, but not from the porpoise (AAH 009) that was captured and released until after the 7-day BAPGM enrichment period. Using a multiplex real-time PCR assay developed in the Vector-Borne Disease Diagnostic Laboratory at North Carolina State University History
Cloning and Sequencing The Bartonella species was confirmed by cloning and sequencing the 16S-23S ITS region and the pap31 gene. The ITS and pap31 DNA sequences from both porpoises were consistent with that of B. henselae strain San Antonio 2 (GenBank accession no. AF369529). The 16S-23S ITS sequence matches were 675/677 bp (99.7%) for MLC 001 and 676/677 bp (99.8%) for AAH 009. The ITS sequence from MLC 001 contained 2 bp insertions (a C and a T), at positions 45 and 675, respectively, when compared with the ITS GenBank sequences for B. henselae SA2. Sequences from AAH 009 contained only a C insertion at position 45. The pap31 gene sequences derived from both porpoises matched 540/540 bp (100%) with B. henselae SA2 (GenBank accession no. AF308168). Discussion We report the first detection of a Bartonella species from the blood of a cetacean cetacean Any of the exclusively aquatic placental mammals constituting the order Cetacea. They are found in oceans worldwide and in some freshwater environments. Modern cetaceans are grouped in two suborders: about 70 species of toothed whales (Odontoceti) and 13 species of , the detection of B. henselae from a nonterrestrial animal. This study was initiated by a request to use molecular diagnostic to evaluate blood from a stranded sick porpoise and from a porpoise captured out of its natural habitat. MLC 001, a yearling female that was stranded in a remote location, may have been stranded for many hours before it could safely be reached and humanely killed. There was no evidence of fisheries interaction. The animal was thin, and necropsy showed no food in its stomach. Few obvious gross lesions and parasites were noted. The degree of postmortem autolysis autolysis /au·tol·y·sis/ (aw-tol´i-sis) 1. spontaneous disintegration of cells or tissues by autologous enzymes, as occurs after death and in some pathologic conditions. 2. was more than would be expected in a freshly killed animal. This finding, with signs of cranial epaxial epaxial /ep·ax·i·al/ (ep-ak´se-il) situated upon or above an axis. ep·ax·i·al adj. Located above or behind an axis, such as the spinal axis or the axis of a limb. and caudal abdominal muscle hemorrhages and the friable condition of the muscle, suggests that the animal's condition likely deteriorated during stranding. Results of histopathologic examination were unremarkable and lesions known to be consistent with bartonellosis were not found. AAH 009, found swimming in a low-salinity canal, had 2 lacerations (2.5 and 5 cm long) over the left dorsal trunk cranial to the dorsal fin, 1 of which extended the full thickness through the blubber, but was not bleeding. In addition, [approximately equal to] 8 clusters of pinpoint lesions were observed slightly cranial and dorsal to the lacerations, which may have been due to punctures or viral skin lesions. Assessment of the porpoise's behavior, body condition, and hematologic hematological, hematologic pertaining to or emanating from blood cells. hematological tests total and differential white cell counts, hematocrit estimation, erythrocyte count. parameters indicated that it was not debilitated despite its unusual location. It was then tagged and released into the ocean. Molecular evidence of Bartonella infection was obtained by direct PCR on whole blood from MLC 001, and by using a recently improved diagnostic method that combines preenrichment blood culture (24) and real-time PCR in samples from AAH 009. An isolate was not obtained from either porpoise after application of the preenrichment BAPGM blood culture onto a blood agar plate. Recently, various emerging or reemerging infectious diseases or infections of serious epizootic ep·i·zo·ot·ic adj. Affecting a large number of animals at the same time within a particular region or geographic area. Used of a disease. ep or zoonotic potential have been described in marine mammals (28-32). These include morbillivirus Morbillivirus /Mor·bil·li·vi·rus/ (-vi?rus) measles-like viruses; a genus of viruses of the family Paramyxoviridae, including the agents of measles and canine distemper. Mor·bil·li·vi·rus n. infection, brucellosis brucellosis (br  'səlō`sĭs) or Bang's disease, infectious disease of farm animals that is sometimes transmitted to humans. , toxoplasmosis, sarcocystosis, papillomavirus infection, and West Nile virus West Nile virus, microorganism and the infection resulting from it, which typically produces no symptoms or a flulike condition. The virus is a flavivirus and is related to a number of viruses that cause encephalitis. infection (29,31,33). As was the case for brucellosis, recognized as an emerging disease in a marine mammal in 1994 (34,35), bartonellosis may become an important emerging marine mammal infectious disease. Current evidence indicates that all known Bartonella species are vector transmitted, with bites or scratches (cat scratch disease cat scratch disease n. An infectious disease that may follow the scratch or bite of a cat, producing localized inflammation of lymph nodes and a low-grade fever. Also called benign inoculation lymphoreticulosis, cat scratch fever. ) providing an alternative means of transmission for B. henselae (2,20). The B. henselae SA2 sequence deposited in GenBank was amplified from an isolate derived from a human lymph node aspiration sample (9). Although exposed to rose thorns and cats, the patient did not recall an animal bite or scratch, and illness developed after a recent tick bite, which was attributed to Amblyomma americanum, based on the location and time of the year. Since the mode of infection was not established in these porpoises, the potential role of trauma, as induced by tooth raking, or transmission by biting marine invertebrates should be investigated. As for many fastidious pathogens, difficulties associated with Bartonella detection and isolation have compromised efforts to define the role of these organisms in disease causation. Enhancement of organism-specific DNA detection and isolation through the use of an optimized isolation medium such as BAPGM can aid in evaluating serodiagnostic assays and may advance understanding the diversity, adaptation, and epidemiology of this genus (24,36). Based on the recent use of BAPGM in the North Carolina State University Vector-Borne Disease Diagnostic Laboratory, we believe that chronic infection with Bartonella species can contribute to subtle clinical abnormalities or vague symptoms in companion and wild animals or in humans. Angiomatosis, an important pathologic manifestation of Bartonella infection in immunocompromised persons (8,21), has been previously reported in bottlenose dolphins (37). Since angiomatous an·gi·o·ma·tous adj. Relating to or resembling an angioma. lesions are unusual pathologic lesions and B. henselae is a recently recognized cause of vasoproliferative lesions in humans (8,15), examination of angiomatous lesions from cetaceans for the presence of B. henselae should be a priority in future studies. In addition, the involvement of Bartonella species in disorders of the central nervous system and neurologic dysfunction in animals and humans (4-7) suggests that this genus should be considered in stranding events. Although Bartonella infection in the vasculature of reservoir hosts is generally not accompanied by pathologic changes, Bartonella spp. may become pathogenic in combination with severe stress, malnutrition, increased exposure to toxins, and concurrent infection with other organisms. PCR amplification directly from an extracted blood sample or from a preenrichment blood culture showed that both porpoises in this study were infected with B. henselae SA2. Since infection with Bartonella spp. has been documented in a marine mammal, the clinical impact, mode of transmission, pathology, and epidemiology are areas for additional inquiry. Acknowledgments We thank Gregory A. Lewbart for helpful discussions and review of this manuscript; Robert George, Larry J. Hansen, and Gretchen N. Lovewell for facilitating blood collection and testing; and the Virginia Aquarium and Marine Science Stranding Program and the University of North Carolina Wilmington Marine Mammal Stranding Program for assistance during the study. This research was supported by the state of North Carolina. Funding for stranding responses and sample collection was provided in part by National Oceanic and Atmospheric Administration Noun 1. National Oceanic and Atmospheric Administration - an agency in the Department of Commerce that maps the oceans and conserves their living resources; predicts changes to the earth's environment; provides weather reports and forecasts floods and hurricanes and Fisheries John H. Prescott Marine Mammal Rescue Assistance Grant Program awards to D. Ann Pabst, William A. McLellan (NA03NMFS4390411), and Craig A. Harms (NA04NMF NMF An abbreviation for "no meaningful figure". 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From the discovery of the Malta fever's agent to the discovery of a marine mammal reservoir, brucellosis has continuously been a re-emerging zoonosis Zoonosis Definition Zoonosis, also called zoonotic disease refers to diseases that can be passed from animals, whether wild or domesticated, to humans. . Vet Res. 2005;36:313-26. (30.) Dubey JP, Zarnke R, Thomas NJ, Wong SK, van Bonn W, Briggs M, et al. Toxoplasma gondii, Neospora caninum, Sarcocystis neurona, and Sarcocystis canis-like infections in marine mammals. Vet Parasitol. 2003; 116:275-96. (31.) Dubey JP. Toxoplasmosis: a waterborne zoonosis. Vet Parasitol. 2004;126:57-72. (32.) Foster G, Jahans KL, Reid RJ, Ross HM. Isolation of Brucella Brucella /Bru·cel·la/ (broo-sel´ah) a genus of schizomycetes (family Brucellaceae). B. abor´tus causes infectious abortion in cattle and is the most common cause of brucellosis in humans. B. species from cetaceans, seals and an otter. Vet Rec. 1996;138:583-6. (33.) Harvell CD, Kim K, Burkholder JM, Colwell RR, Epstein PR, Grimes DJ, et al. Emerging marine diseases: climate links and anthropogenic factors. Science. 1999;285:1505-10. (34.) Ross HM, Jahans KL, MacMillan AP, Reid RJ, Thompson PM, Foster G. Brucella species infection in North Sea seal and cetacean populations. Vet Rec. 1996;138:647-8. (35.) Ewalt DR, Payeur JB, Martin BM, Cummins DR, Miller WG. Characteristics of a Brucella species from a bottlenose dolphin (Tursiops truncatus). J Vet Diagn Invest. 1994;6:448-52. (36.) LaScola B, Raoult D. Culture of Bartonella quintana and Bartonella henselae from human samples: a 5-year experience (1993-1998). J Clin Microbiol. 1999;37:1899-1905. (37.) Turnbull BS, Cowan DF. Angiomatosis, a newly recognized disease in Atlantic bottlenose dolphins (Tursiops truncatus) from the Gulf of Mexico Noun 1. Gulf of Mexico - an arm of the Atlantic to the south of the United States and to the east of Mexico Golfo de Mexico Atlantic, Atlantic Ocean - the 2nd largest ocean; separates North and South America on the west from Europe and Africa on the east . Vet Pathol. 1999;36:28-34. Ricardo G. Maggi, * Craig A. Harms, * ([dagger]) Aleta A. Hohn, ([double dagger]) D. Ann Pabst, ([section]) William A. McLellan, ([section]) Wendy J. Walton, ([paragraph]) David S. Rotstein, (#) and Edward B. Breitschwerdt * * North Carolina State University College of Veterinary Medicine, Raleigh, North Carolina For other uses of this name, see Raleigh. Raleigh (IPA: /ˈrɑli/, ral-ee) is the capital of the State of North Carolina and the county seat of Wake County. , USA; ([dagger]) Center for Marine Sciences and Technology, Morehead City, North Carolina ''This article or section is being rewritten at  This article's grammar usage needs improvement. , USA: ([double dagger]) National Marine Fisheries Service The U.S. National Marine Fisheries Service (NMFS) is a United States federal agency. A division of the National Oceanic and Atmospheric Administration (NOAA) and the Department of Commerce, NMFS is responsible for the stewardship and management of the nation's living marine , Beaufort, North Carolina Beaufort (pronounced "BO-furt" / IPA: ˈbo.fɚt) is a town in Carteret County, North Carolina, United States. , USA; ([section]) University of North Carolina Wilmington, Wilmington, North Carolina For other places with the same name, see Wilmington (disambiguation).Wilmington is a city in New Hanover County, North Carolina, United States. The population was estimated at 100,000 as of 2006;[1] , USA; ([paragraph]) Virginia Aquarium and Marine Science Center, Virginia Beach, Virginia Virginia Beach is an independent city located in the South Hampton Roads area in the Commonwealth of Virginia, on the shores of the Chesapeake Bay and the Atlantic Ocean. It is the most populous city in Virginia and the 41st largest city in the United States, with an estimated , USA; and (#) University of Tennessee The University of Tennessee (UT), sometimes called the University of Tennessee at Knoxville (UT Knoxville or UTK), is the flagship institution of the statewide land-grant University of Tennessee public university system in the American state of Tennessee. College of Veterinary Medicine, Knoxville, Tennessee, USA Address for correspondence: Edward B. Breitschwerdt, Department of Clinical Sciences, College of Veterinary Medicine, North Carolina State University, 4700 Hillsborough St, Raleigh, NC 27606, USA; fax: 919-513-6336; email: ed_breitschwerdt@ncsu.edu Dr Maggi is a research postdoctoral associate in the Intracellular Pathogens Laboratory at North Carolina State University, College of Veterinary Medicine. His research interests include development of novel/improved molecular, diagnostic, and culture methods for detection of Bartonella infections in humans and animals. |
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