1.Tick-borne rickettsial pathogens in questing ticks, removed from humans and animals in Mexico.
Carolina G SOSA-GUTIERREZ ; Margarita VARGAS-SANDOVAL ; Javier TORRES ; Guadalupe GORDILLO-PÉREZ
Journal of Veterinary Science 2016;17(3):353-360
Tick-borne rickettsial diseases (TBRD) are commonly encountered in medical and veterinary clinical settings. The control of these diseases is difficult, requiring disruption of a complex transmission chain involving a vertebrate host and ticks. The geographical distribution of the diseases is related to distribution of the vector, which is an indicator of risk for the population. A total of 1,107 ticks were collected by tick dragging from forests, ecotourism parks and hosts at 101 sites in 22 of the 32 states of Mexico. Collected ticks were placed in 1.5 mL cryovials containing 70% ethanol and were identified to species. Ticks were pooled according to location/host of collection, date of collection, sex, and stage of development. A total of 51 ticks were assayed by polymerase chain reaction (PCR) to confirm species identification using morphological methods. A total of 477 pools of ticks were assayed using PCR techniques for selected tick-borne pathogens. Anaplasma phagocytophilum was the most commonly detected pathogen (45 pools), followed by, Ehrlichia (E.) canis (42), Rickettsia (R.) rickettsii (11), E. chaffeensis (8), and R. amblyommii (1). Rhipicephalus sanguineus was the tick most frequently positive for selected pathogens. Overall, our results indicate that potential tick vectors positive for rickettsial pathogens are distributed throughout the area surveyed in Mexico.
Anaplasma phagocytophilum
;
Animals*
;
Ehrlichia
;
Ehrlichia canis
;
Ehrlichia chaffeensis
;
Ethanol
;
Forests
;
Humans*
;
Mexico*
;
Polymerase Chain Reaction
;
Rhipicephalus sanguineus
;
Rickettsia
;
Ticks*
;
Vertebrates
2.Genetic Identification and Phylogenetic Analysis of Anaplasma and Ehrlichia Species in Haemaphysalis longicornis Collected from Jeju Island, Korea.
Jae Young OH ; Bong Chun MOON ; Bo Kyoung BAE ; E Hyun SHIN ; Young Hwan KO ; Young Joo KIM ; Yong Ho PARK ; Joon Seok CHAE
Journal of Bacteriology and Virology 2009;39(4):257-267
A total of 1,395 Haemaphysalis longicornis ticks collected from Jeju Island of Korea were examined by 16S rRNA gene-based nested PCR for the presence of infection with Anaplasma and Ehrlichia species. Template DNAs to detect the tick-borne pathogens were prepared from a total 506 tick pools. Eight genera of Anaplasma and six Ehrlichia by 16S rRNA gene PCR and sequencing analysis were identified. A. phagocytophilum was the most prevalent (27 [1.9%]) by nested PCR, followed by A. bovis (5 [0.4%]), E. chaffeensis (4 [0.2%]), and A. centrale (1 [0.1%]). In the phylogenetic analysis based on 16S rRNA sequences, eight genera of Anaplasma group (> 99.4% homology) and six Ehrlichia group (> 99.5% homology) were close to deposited A. marginale strains (AF309867, AF414874, and FJ226454) and Ehrlichia sp. (DQ324547), respectively. Three Anaplasma species groups A. phagocytophilum (group A), A. bovis (group B), and A. centrale (group C) and one Ehrlichia species E. chaffeensis (group D) were determined by comparing with Anaplasma and Ehrlichia related sequences. First, twenty-eight A. phagocytophilum clones belonging to group A were divided into 7 genotypes. The sequence similarity among genotypes A1 to A4 was very high (> 99.6%). Genotype B2 was close to A. bovis from Korea (99.7%). Genotype D1 was close to known E. chaffeensis strains (M73222, AF147752, and AY350424) and their similarity value was 99.7%. In conclusion, the genera of Anaplasma/Ehrlichia, A. phagocytophilum, and E. chaffeensis identified in predominant H. longicornis ticks were ubiquitous throughout the Jeju Island. The various native groups have been found through sequence identities and phylogenetic analysis.
Anaplasma
;
Anaplasma phagocytophilum
;
Clone Cells
;
DNA
;
Ehrlichia
;
Ehrlichia chaffeensis
;
Genes, rRNA
;
Genotype
;
Korea
;
Polymerase Chain Reaction
;
Ticks
3.Anaplasma marginale and A. platys Characterized from Dairy and Indigenous Cattle and Dogs in Northern Vietnam
Nguyen Thi Hong CHIEN ; Thi Lan NGUYEN ; Khanh Linh BUI ; Tho VAN NGUYEN ; Thanh Hoa LE
The Korean Journal of Parasitology 2019;57(1):43-47
Anaplasma marginale and A. platys were detected and characterized (16S rDNA sequence analysis) from dairy and indigenous cattle, and the latter in domestic dogs in Vietnam. A phylogenetic tree was inferred from 26 representative strains/species of Anaplasma spp. including 10 new sequences from Vietnam. Seven of our Vietnamese sequences fell into the clade of A. marginale and 3 into A. platys, with strong nodal support of 99 and 90%, respectively. Low genetic distances (0.2–0.4%) within each species supported the identification. Anaplasma platys is able to infect humans. Our discovery of this species in cattle and domestic dogs raises considerable concern about zoonotic transmission in Vietnam. Further systematic investigations are needed to gain data for Anaplasma spp. and members of Anaplasmataceae in animal hosts, vectors and humans across Vietnam.
Anaplasma marginale
;
Anaplasma
;
Anaplasmataceae
;
Animals
;
Asian Continental Ancestry Group
;
Cattle
;
DNA, Ribosomal
;
Dogs
;
Humans
;
Phylogeny
;
Trees
;
Vietnam
4.Detection and molecular characterization of Hepatozoon canis, Babesia vogeli, Ehrlichia canis, and Anaplasma platys in dogs from Metro Manila, Philippines.
Davin Edric V ADAO ; Charles Michael T HERRERA ; Luiza H GALARION ; Nicole R BOLO ; Rhodora S CARLOS ; Enrique T CARLOS ; Sixto S CARLOS ; Windell L RIVERA
Korean Journal of Veterinary Research 2017;57(2):79-88
The study of canine vector-borne diseases in the Philippines started in the 1970s but only gained interest in the past decade. Characterization of such diseases in the Philippines remains incomplete, thus, it is necessary to obtain additional information on the prevalence and diversity of canine tick-borne diseases in the country. In this study, blood samples were obtained at two veterinary clinics in Metro Manila, Philippines from 114 dogs suspected of having canine tick-borne pathogens. Polymerase chain reaction (PCR) was performed on whole blood DNA extracts followed by sequencing, and the following pathogens were detected: Hepatozoon (H.) canis (5.26%), Babesia (B.) vogeli (5.26%), Ehrlichia (E.) canis (4.39%), and Anaplasma platys (3.51%). Additionally, a set of multiplex PCR primers were developed to detect H. canis, Babesia spp. (B. canis and B. vogeli), and E. canis in canine blood. Multiplex and conventional single-reaction PCR results for the 114 dog blood samples were similar, except for one H. canis sample. Multiplex PCR is, therefore, a useful tool in screening infected dogs in veterinary clinics. This study's results, together with those of previous studies in the country, show that canine vector-borne pathogens are an emerging veterinary concern in the Philippines.
Anaplasma*
;
Animals
;
Babesia*
;
DNA
;
Dogs*
;
Ehrlichia canis*
;
Ehrlichia*
;
Hospitals, Animal
;
Mass Screening
;
Multiplex Polymerase Chain Reaction
;
Philippines*
;
Polymerase Chain Reaction
;
Prevalence
;
Tick-Borne Diseases
5.Serological investigation of vector-borne disease in dogs from rural areas of China.
Shiwen WANG ; Jing HE ; Lijuan ZHANG
Asian Pacific Journal of Tropical Biomedicine 2012;2(2):102-103
OBJECTIVETo evaluate the Anaplasma phagocytophilum (A. phagocytophilum), Ehrlichia canis (E. canis), Dirofilaria immitis (D. immitis) (canine heartworm), Borrelia burgdorferi (B. burgdorferi) infections in countryside dogs from Yunnan, Hainan and Anhui provinces.
METHODSSerum samples were collected from 26 dogs in Yunnan, Hainan and Anhui provinces. The samples were tested using a commercial ELISA rapid diagnostic assay kit (SNAP(®) 4Dx(®); IDEXX Laboratories, Inc. U.S.A.). Meanwhile, indirect immunofluorescence assay (IFA) recommended by WHO was conducted to detect IgG to A. phagocytophilum. Two methods were analyzed and compared.
RESULTSThe number of serologically positive dogs for IgG to A. phagocytophilum was only 2 which was from Hainan province and none of the 26 dogs responded positive for E. canis, D. immitis (canine heartworm), and B. burgdorferi by ELISA rapid diagnostic method. The number of serologically positive dogs for IgG to A. phagocytophilum was 13 (50%) by IFA method. Data of the two methods were analyzed by statistical software and the difference was statistically significant (P=0.002).
CONCLUSIONSIt can be concluded that IFA method was more sensitive than ELISA rapid diagnostic method. However, we need conduct further and intensive epidemiology survey on tick-born diseases pathogens including A. phagocytophilum, E. canis, D. immitis (canine heartworm), and B. burgdorferi which have public health significance.
Anaplasma phagocytophilum ; immunology ; Animals ; Borrelia burgdorferi ; immunology ; China ; epidemiology ; Dirofilaria immitis ; immunology ; Dirofilariasis ; blood ; epidemiology ; immunology ; Disease Vectors ; Dog Diseases ; epidemiology ; Dogs ; Ehrlichia canis ; immunology ; Ehrlichiosis ; blood ; epidemiology ; immunology ; Enzyme-Linked Immunosorbent Assay ; methods ; Fluorescent Antibody Technique, Indirect ; methods ; Immunoglobulin G ; blood ; Lyme Disease ; blood ; epidemiology ; immunology ; Tick-Borne Diseases ; epidemiology
6.Molecular and phylogenetic analysis of Anaplasma spp. in sheep and goats from six provinces of China.
Yan ZHANG ; Yali LV ; Feifei ZHANG ; Wenjing ZHANG ; Jinhong WANG ; Yanyan CUI ; Rongjun WANG ; Fuchun JIAN ; Longxian ZHANG ; Changshen NING
Journal of Veterinary Science 2016;17(4):523-529
Members of the genus Anaplasma are important emerging tick-borne pathogens in both humans and animals in tropical and subtropical areas. Here, we investigated the presence of Anaplasma spp. in 621 sheep and 710 goats from six provinces of China. Polymerase chain reaction (PCR) and DNA sequencing were conducted to determine the prevalence of Anaplasma (A.) phagocytophilum, A. ovis and A. bovis targeting the 16S ribosomal RNA or the major surface protein 4 gene. PCR revealed Anaplasma in 39.0% (240/621) of sheep and 45.5% (323/710) of goats. The most frequently detected species was A. ovis (88/621, 14.2% for sheep; 129/710, 18.2% for goats), followed by A. bovis (60/621, 9.7% for sheep; 74/710, 10.4% for goats) and A. phagocytophilum (33/621, 5.3% for sheep; 15/710, 2.1% for goats). Additionally, eight sheep and 20 goats were found to be infected with three pathogens simultaneously. DNA sequencing confirmed the presence of these three Anaplasma species in the investigated areas, and phylogenetic analysis indicated that there was geographic segregation to a certain extent, as well as a relationship between the host and cluster of A. ovis. The results of the present study provide valuable data that helps understand the epidemiology of anaplasmosis in ruminants from China.
Anaplasma ovis
;
Anaplasma phagocytophilum
;
Anaplasma*
;
Anaplasmosis
;
Animals
;
China*
;
Epidemiology
;
Goats*
;
Humans
;
Polymerase Chain Reaction
;
Prevalence
;
RNA, Ribosomal, 16S
;
Ruminants
;
Sequence Analysis, DNA
;
Sheep*
8.Development of Rickettsia Specific Nested PCR Method Based on groEL Gene Sequences.
Jung Hee LEE ; Hyo Soon PARK ; Eun Ju JEONG ; Jung Eun KIM ; Won Jong JANG ; Kyung Hee PARK ; Bum Joon KIM ; Yoon Hoh KOOK ; Seung Hyun LEE
Journal of Bacteriology and Virology 2003;33(4):301-306
To detect Rickettsia, we have developed a nested PCR method amplifying the groEL gene. Rickettsia strains were successfully amplified by this PCR method but the microorganisms causing other febrile diseases, such as Orientia tsutsugamushi, Coxiella burnetii, Ehrlichia sennetsu, Borrelia burgdorferi sensu lato, Borrelia hermsii, and Leptospira interrogans were not amplified. This PCR assay was applied to detect Rickettsia DNA from 100 ticks. Sixteen Haemaphysalis longicornis ticks were positive by this PCR assay. These results suggest that the new nested PCR method might be sensitive and useful for discrimination between Rickettsia and other febrile disease-causing microorganisms.
Borrelia
;
Borrelia burgdorferi Group
;
Coxiella burnetii
;
Discrimination (Psychology)
;
DNA
;
Leptospira interrogans
;
Neorickettsia sennetsu
;
Orientia tsutsugamushi
;
Polymerase Chain Reaction*
;
Rickettsia*
;
Ticks
9.Serological Analysis of Ehrlichiosis in Korean from 1990 to 1992.
Won Jong JANG ; Kwang Don JUNG ; Jong Hyun KIM ; Seung Hyun LEE ; Ik Sang KIM ; Myung Sik CHOI ; Kyung Hee PARK
Journal of Bacteriology and Virology 2002;32(3):255-261
Ehrlichia sennetsu is the causative agent of human Sennetsu ehrlichiosis. Ehrlichiosis is an acute and occasionally chronic infectious disease caused by obligate intracellular bacteria in the family Rickettsiaceae. To understand the seroepidemiological patterns of ehrlichiosis in Korea, a total of 2,625 patients with acute febrile episode reported from 1990 to 1992 were surveyed using an indirect fluorescent antibody assay (IFA). The result was as follows. Seropositivity for ehrlichiosis was 3.23% by excluding highly cross-reacted sera with other rickettsial antigens. Sera reacted to E. sennetsu showed the cross reaction with other rickettsia as in the order of R. typhi 49.6%, R. conorii 31.6%, R. japonica 28.1%, C. burnetii 26.4%, R. sibirica 25.8%, O. tsutsugamushi 25.8%, R. akari 25.4%, and R. prowazekii 25.4%. Sexual difference in the seropositivity was not noted. The age groups of fifties and under the tenth showed higher prevalence than others. Seropositivity was most prevalent in July and August. As for regional distribution, Chonbuk (10.5%) showed the highest seropositive rate. Geographical distribution of the seropositivity covered most area except Cheju province in Korea.
Bacteria
;
Communicable Diseases
;
Cross Reactions
;
Ehrlichiosis*
;
Humans
;
Jeju-do
;
Jeollabuk-do
;
Korea
;
Neorickettsia sennetsu
;
Prevalence
;
Rickettsia
;
Rickettsiaceae
10.Sequence and phylogenetic analysis of the gp200 protein of Ehrlichia canis from dogs in Taiwan.
Chia Chia HUANG ; Yu Chen HSIEH ; Chau Loong TSANG ; Yang Tsung CHUNG
Journal of Veterinary Science 2010;11(4):333-340
Ehrlichia (E.) canis is a Gram-negative obligate intracellular bacterium responsible for canine monocytic ehrlichiosis. Currently, the genetic diversity of E. canis strains worldwide is poorly defined. In the present study, sequence analysis of the nearly full-length 16S rDNA (1,620 bp) and the complete coding region (4,269 bp) of the gp200 gene, which encodes the largest major immunoreactive protein in E. canis, from 17 Taiwanese samples was conducted. The resultant 16S rDNA sequences were found to be identical to each other and have very high homology (99.4~100%) with previously reported E. canis sequences. Additionally, phylogenetic analysis of gp200 demonstrated that the E. canis Taiwanese genotype was genetically distinct from other reported isolates obtained from the United States, Brazil, and Israel, and that it formed a separate clade. Remarkable variations unique to the Taiwanese genotype were found throughout the deduced amino acid sequence of gp200, including 15 substitutions occurring in two of five known species-specific epitopes. The gp200 amino acid sequences of the Taiwanese genotype bore 94.4~94.6 identities with those of the isolates from the United States and Brazil, and 93.7% homology with that of the Israeli isolate. Taken together, these results suggest that the Taiwanese genotype represents a novel strain of E. canis that has not yet been characterized.
Amino Acid Sequence
;
Animals
;
Bacterial Proteins/chemistry/*genetics
;
Dogs
;
Ehrlichia canis/*classification/*genetics
;
Genotype
;
Molecular Sequence Data
;
*Phylogeny
;
RNA, Ribosomal, 16S/genetics
;
Sequence Alignment
;
Sequence Analysis, Protein
;
Taiwan