Your search keyword '"Sarcocystosis veterinary"' showing total 1,348 results

201. Sarcocystis strixi n. sp. from a Barred Owl ( Strix varia) Definitive Host and Interferon Gamma Gene Knockout Mice as Experimental Intermediate Host.

Author

Verma SK, von Dohlen AR, Mowery JD, Scott D, Cerqueira-Cézar CK, Rosenthal BM, Dubey JP, and Lindsay DS

Subjects

Animals, Cells, Cultured, Chlorocebus aethiops, DNA, Protozoan chemistry, DNA, Protozoan genetics, DNA, Protozoan isolation & purification, DNA, Ribosomal chemistry, Electron Transport Complex IV genetics, Intestines parasitology, Kidney cytology, Mice, Mice, Knockout, Phylogeny, RNA, Ribosomal, 18S genetics, RNA, Ribosomal, 28S genetics, Sarcocystis classification, Sarcocystis genetics, Sarcocystis growth & development, Sarcocystosis parasitology, Sequence Alignment veterinary, Bird Diseases parasitology, Interferon-gamma genetics, Sarcocystis isolation & purification, Sarcocystosis veterinary, Strigiformes parasitology

Abstract

Here we report a new species of Sarcocystis with a barred owl ( Strix varia) as the natural definitive host and interferon gamma gene knockout (KO) mice as an experimental intermediate host. A barred owl submitted to the Carolina Raptor Center, Huntersville, North Carolina, was euthanized because of paralysis. Fully sporulated 12.5 × 9.9 μm sporocysts were found in intestinal scrapings from the owl. Sporocysts from the barred owl were orally fed to 4 laboratory-reared outbred Swiss Webster (SW) ( Mus musculus) and 8 KO mice. All mice remained asymptomatic. Microscopic sarcocysts were found in all 5 KO mice euthanized on day 32, 59, 120, 154, and 206 post-inoculation (PI), not in KO mice euthanized on day 4, 8, and 14 PI. Sarcocysts were not found in any SW mice euthanized on day 72, 120, 206, and 210 PI. Sarcocysts were microscopic, up to 70 μm wide. By light microscopy, the sarcocyst wall < 2 μm thick had undulating, flat to conical, protrusions of varying dimensions. Numerous sarcocysts were seen in the histological sections of tongue and skeletal muscles from the abdomen, limbs, and eye but not in the heart. By transmission electron microscopy, the sarcocyst wall was "type 1j." The ground substance layer (gs) was homogenous, up to 2 μm thick, with very fine granules, and a few vesicles concentrated toward the villar projections. No microtubules were seen in the gs. Longitudinally cut bradyzoites at 206 days PI were 7.8 × 2.2 μm. Based on molecular characterization using 18S rRNA, 28S rRNA, and cox1 genes and morphology of sarcocysts, the parasite in the present study was biologically and structurally different from species so far described, and we therefore propose a new species name, Sarcocystis strixi n. sp.

Published

2017

202. Testing the Sarcocystis neurona vaccine using an equine protozoal myeloencephalitis challenge model.

Author

Saville WJA, Dubey JP, Marsh AE, Reed SM, Keene RO, Howe DK, Morrow J, and Workman JD

Subjects

Animals, Encephalomyelitis parasitology, Encephalomyelitis prevention & control, Horse Diseases parasitology, Horses, Opossums, Raccoons, Random Allocation, Sarcocystosis parasitology, Sarcocystosis prevention & control, Encephalomyelitis veterinary, Horse Diseases prevention & control, Protozoan Vaccines immunology, Sarcocystis immunology, Sarcocystosis veterinary, Vaccination veterinary

Abstract

Equine protozoal myeloencephalitis (EPM) is an important equine neurologic disorder, and treatments for the disease are often unrewarding. Prevention of the disease is the most important aspect for EPM, and a killed vaccine was previously developed for just that purpose. Evaluation of the vaccine had been hampered by lack of post vaccination challenge. The purpose of this study was to determine if the vaccine could prevent development of clinical signs after challenge with Sarcocystis neurona sporocysts in an equine challenge model. Seventy horses that were negative for antibodies to S. neurona and were neurologically normal were randomly assigned to vaccine or placebo groups and divided into short-term duration of immunity (study #1) and long-term duration of immunity (study #2) studies. S. neurona sporocysts used for the challenge were generated in the opossum/raccoon cycle isolate SN 37-R. Study #1 horses received an initial vaccination and a booster, and were challenged 34days post second vaccination. Study #2 horses received a vaccination and two boosters and were challenged 139days post third vaccination. All horses in study #1 developed neurologic signs (n=30) and there was no difference between the vaccinates and controls (P=0.7683). All but four horses in study #2 developed detectable neurologic deficits. The neurologic signs, although not statistically significant, were worse in the vaccinated horses (P=0.1559). In these two studies, vaccination with the S. neurona vaccine failed to prevent development of clinical neurologic deficits., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2017

203. Atypical fatal sarcocystosis associated with Sarcocystis neurona in a White-nosed coati (Nasua narica molaris).

Author

Dubey JP, Trupkiewicz JG, Verma SK, Mowery JD, Adedoyin G, Georoff T, and Grigg ME

Subjects

Animals, Antigens, Surface, Encephalomyelitis diagnosis, Encephalomyelitis parasitology, Encephalomyelitis pathology, Genotype, Genotyping Techniques, Male, Microsatellite Repeats genetics, Sarcocystis genetics, Sarcocystosis diagnosis, Sarcocystosis parasitology, Sarcocystosis pathology, Schizonts, Antibodies, Protozoan blood, Encephalomyelitis veterinary, Procyonidae parasitology, Sarcocystis isolation & purification, Sarcocystosis veterinary

Abstract

The protozoan parasite Sarcocystis neurona is an important cause of disease in horses (equine protozoal myeloencephalitis, EPM) and marine mammals. Isolated reports of clinical EPM-like disease have been documented in a zebra, raccoon, domestic cat, domestic dog, ferret, skunk, mink, lynx, red panda and fisher. The predominant disease is encephalomyelitis associated with schizonts in neural tissues. Here, we report highly disseminated sarcocystosis, in many tissues of a captive White-nosed coati (Nasua narica molaris). The 14year old, neutered male coati was euthanized due to progressive weakness, lethargy, and inappetence. Schizonts, including free and intracellular merozoites were detected in many cell types, and differed morphologically from S. neurona schizonts in horses. Only a few sarcocysts were seen in skeletal muscle and the myocardium. Immunohistochemically, the protozoa reacted positively to S. neurona but not to Toxoplasma gondii antibodies. Severe inflammtory disease detected in the stomach, intestine, adrenal and thyroid glands, ciliary body of eye, and urinary bladder associated with schizonts in the coati has not been reported earlier in any host with EPM. Although, a few schizonts were found in the brain, encephalitis was minimal and not the cause of clinical signs. Multilocus PCR-DNA sequencing using DNA derived from the coati lung tissue identified an S. neurona infection using the 18S, 28S and ITS-1 markers, and a novel genotype using primer pairs against antigenic surface proteins (SnSAG3, SnSAG4, SnSAG1-5-6) and microsatellite markers (MS, SN7, SN9). Although the genotype was similar to the widely distributed Type VI strain, it possessed a novel allele at SnSAG5, and a different MS combination of repeats at SN7 and SN9. Whether this severe parasitism was related to the host or the parasite needs further investigation., (Published by Elsevier B.V.)

Published

2017

204. Interobserver Variation in the Diagnosis of Neurologic Abnormalities in the Horse.

Author

Saville WJA, Reed SM, Dubey JP, Granstrom DE, Morley PS, Hinchcliff KW, Kohn CW, Wittum TE, and Workman JD

Subjects

Animals, Ataxia diagnosis, Ataxia veterinary, Coccidiosis veterinary, Dyskinesias diagnosis, Dyskinesias veterinary, Encephalomyelitis diagnosis, Encephalomyelitis parasitology, Horses, Nervous System Diseases diagnosis, Physical Examination standards, Physical Examination veterinary, Prospective Studies, Reproducibility of Results, Sarcocystosis veterinary, Encephalomyelitis veterinary, Horse Diseases diagnosis, Nervous System Diseases veterinary, Observer Variation

Abstract

Background: The diagnosis of equine protozoal myeloencephalitis (EPM) relies heavily on the clinical examination. The accurate identification of neurologic signs during a clinical examination is critical to the interpretation of laboratory results., Objective: To investigate the level of agreement between board-certified veterinary internists when performing neurologic examinations in horses., Animals: Ninety-seven horses admitted to the Veterinary Teaching Hospital at The Ohio State University from December 1997 to June 1998., Methods: A prospective epidemiologic research design was used. Horses enrolled in the study were examined by the internist responsible for care of the horse, and later by an internist who was not aware of the presenting complaint or other patient history. Data were analyzed by descriptive statistics, and kappa (K) statistics were calculated to assess interobserver agreement., Results: Ninety-seven horses were enrolled in the study. Overall, examiners, also referred to as observers, agreed that 60/97 (61.9%) were clinically abnormal, 21/97 (21.6%) were clinically normal, and the status of 16/97 (16.5%) of horses was contested. There was complete agreement among the examiners with regard to cranial nerve signs and involuntary movements. Disagreement involving severity of clinical signs occurred in 31 horses, and 25 of those horses (80.6%) were considered either normal or mildly affected by the primary observer. When examining the results of all paired clinical examinations for 11 different categories, there was wide variability in the results. When examiners rated the presence or absence of any neurologic abnormalities, lameness, or ataxia, the agreement among observers was either good or excellent for 80% of horses. When assessing truncal sway, the agreement among observers was good or excellent for 60% of the horses. When examining the horses for asymmetry of deficits, agreement was either good or excellent for 40% of the horses. Agreement among observers was excellent or good for only 20% of the horses when assessing muscle atrophy, spasticity (hypermetria), and overall assessment of the severity of neurologic abnormalities., Conclusions and Clinical Importance: This study underscores the subjectivity of the neurologic examination and demonstrates a reasonable level of agreement that may be achieved when different clinicians examine the same horse., (Copyright © 2017 The Authors. Journal of Veterinary Internal Medicine published by Wiley Periodicals, Inc. on behalf of the American College of Veterinary Internal Medicine.)

Published

2017

205. Morphological and molecular characteristics of six Sarcocystis spp. from red deer (Cervus elaphus) in Spain, including Sarcocystis cervicanis and three new species.

Author

Gjerde B, Luzón M, Alunda JM, and de la Fuente C

Subjects

Animals, Electron Transport Complex IV genetics, Microscopy, Electron, Scanning veterinary, Mitochondrial Proteins genetics, Muscles parasitology, Phylogeny, Polymerase Chain Reaction veterinary, Protozoan Proteins genetics, RNA, Ribosomal, 18S genetics, Sarcocystis genetics, Sarcocystis isolation & purification, Sarcocystis ultrastructure, Sarcocystosis parasitology, Sequence Analysis, DNA veterinary, Spain, Deer parasitology, Genetic Variation, Sarcocystis classification, Sarcocystosis veterinary

Abstract

Samples of muscle tissue from the diaphragm, oesophagus and/or heart of eight adult red deer (Cervus elaphus hispanicus) from the Quintos de Mora Park in Toledo, Central Spain, were screened for sarcocysts by means of the compression method. From positive samples, individual sarcocysts were excised and examined in wet mounts under a light microscope (LM) in order to study their basic morphology before being preserved for molecular studies. In all red deer examined, only microscopic sarcocysts were found. Those in the diaphragm and oesophagus were spindle-shaped and about 1 × 0.1 mm in size, while those in cardiac muscle were sac-like and 500-800 × 80-180 μm. By LM, the sarcocysts either had densely packed, about 8-μm-long, hair-like protrusions (type 1), sparsely distributed indistinct projections (fuzzy outline; type 2) or no visible protrusions (smooth surface; type 3). In cardiac muscle, only sarcocysts without visible protrusions were found. One of the latter sarcocysts was examined by scanning electron microscopy (SEM) and found to possess thin ribbon-like protrusions. Forty-eight sarcocysts isolated from the diaphragm, oesophagus and heart of one red deer, as well as 55 sarcocysts from the heart of three other red deer, 103 sarcocysts in total, were characterized molecularly through PCR amplification and sequencing of the partial cytochrome c oxidase subunit I gene (cox1) of the mitochondrial genome, revealing the presence of six major cox1 sequence types. Each type comprised either a single sequence (three types) or a collection of several identical or nearly identical sequences. From selected isolates possessing each of these cox1 sequence types, the complete 18S ribosomal RNA (rRNA) gene was amplified and sequenced directly and/or after cloning of the 5' end half. Supported by the sequence data from the latter gene, as well as the morphology of the sarcocysts from which the sequences originated, the six cox1 sequence types were considered to represent six separate Sarcocystis spp. Two cox1 sequence types were identified as belonging to the previously characterized species Sarcocystis hjorti (one sequence/sarcocyst) and Sarcocystis linearis (38 sequences/sarcocysts), respectively, whereas four sequence types were new. One of the latter types was assigned to the previously named species Sarcocystis cervicanis from red deer, since this sequence type was obtained from 52 sarcocysts from cardiac muscle, which matched the original morphological description (smooth surface) and habitat of this species. The remaining three sequence types were assigned to the three new species Sarcocystis iberica (one sequence/sarcocyst) Sarcocystis venatoria (10 sequences/sarcocysts) and Sarcocystis morae (one sequence/sarcocyst), respectively. The two species S. iberica and S. venatoria shared the same sarcocyst morphology (type 1) and habitat (diaphragm) and had virtually identical 18S rRNA gene sequences, but differed by 4% at cox1, which was considered sufficient to regard them as separate species. The single sarcocyst of S. morae (from the oesophagus) examined by LM had a smooth wall and this species was therefore believed to have the same type of ribbon-like protrusions (ultrastructurally) as sarcocysts of S. cervicanis and S. linearis, which were also the species most closely related to S. morae at cox1. Thus, there seems to be three species with similar ribbon-like cyst wall protrusions in red deer (S. cervicanis, S. linearis, S. morae), as well as three species with similar hair-like protrusions (S. hjorti, S. iberica, S. venatoria). Sarcocysts of S. cervicanis were only identified in cardiac muscle, whereas sarcocysts of S. linearis were found mainly in the diaphragm and oesophagus and rarely in the heart. The relative number of cox1 haplotypes was greater among sequences/isolates of S. linearis (17/38) than among isolates of S. cervicanis (7/52). Four of the species examined (S. cervicanis, S. linearis, S. iberica, S. venatoria) possessed considerable intra-isolate (intra-genomic) sequence variation (insertions/deletions, substitutions) in the 18S rRNA gene.

Published

2017

206. Phosphorylated neurofilament H (pNF-H) as a potential diagnostic marker for neurological disorders in horses.

Author

Intan-Shameha AR, Divers TJ, Morrow JK, Graves A, Olsen E, Johnson AL, and Mohammed HO

Subjects

Animals, Biomarkers blood, Biomarkers cerebrospinal fluid, Cross-Sectional Studies, Encephalomyelitis blood, Encephalomyelitis cerebrospinal fluid, Encephalomyelitis diagnosis, Encephalomyelitis veterinary, Enzyme-Linked Immunosorbent Assay veterinary, Horse Diseases blood, Horse Diseases cerebrospinal fluid, Horses, Nervous System Diseases blood, Nervous System Diseases cerebrospinal fluid, Nervous System Diseases diagnosis, Phosphorylation, Sarcocystis isolation & purification, Sarcocystosis blood, Sarcocystosis cerebrospinal fluid, Sarcocystosis diagnosis, Sarcocystosis veterinary, Cervical Vertebrae abnormalities, Horse Diseases diagnosis, Nervous System Diseases veterinary, Neurofilament Proteins blood, Neurofilament Proteins chemical synthesis

Abstract

The current study aimed at the investigating the potential use of phosphorylated neurofilament H (pNF-H) as a diagnostic biomarker for neurologic disorders in the horse. Paired serum and cerebrospinal fluid (CSF) samples (n=88) and serum only (n=30) were obtained from horses diagnosed with neurologic disorders and clinically healthy horses as control. The neurologic horses consisted of equine protozoal myeloencephalitis (EPM) (38 cases) and cervical vertebral malformation (CVM) (23 cases). Levels of pNF-H were determined using an ELISA. The correlation between CSF and serum concentrations of pNF-H was evaluated using Spearman's Rank test and the significance of the difference among the groups was assessed using a nonparametric test. Horses had higher pNF-H levels in the CSF than serum. Horses afflicted with EPM had significantly higher serum pNF-H levels in comparison to controls or CVM cases. The correlation between CSF and serum pNF-H levels was poor in both the whole study population and among subgroups of horses included in the study. There was significant association between the likelihood of EPM and the concentrations of pNF-H in either the serum or CSF. These data suggest that pNF-H could be detected in serum and CSF samples from neurologic and control horses. This study demonstrated that pNF-H levels in serum and CSF have the potential to provide objective information to help in the early diagnosis of horses afflicted with neurologic disorders., (Published by Elsevier Ltd.)

Published

2017

207. Morphological and molecular identification of Sarcocystis arctica sarcocysts in three red foxes (Vulpes vulpes) from the Czech Republic.

Author

Pavlásek I and Máca O

Subjects

Animals, Animals, Wild parasitology, Coinfection epidemiology, Coinfection parasitology, Czech Republic epidemiology, Microscopy, Electron, Transmission, Phylogeny, Polymerase Chain Reaction, RNA, Ribosomal, 18S genetics, Sarcocystis cytology, Sarcocystis genetics, Sarcocystosis diagnosis, Sarcocystosis epidemiology, Sarcocystosis parasitology, Sequence Analysis, DNA, Trichinella isolation & purification, Trichinellosis epidemiology, Trichinellosis parasitology, Trichinellosis veterinary, Foxes parasitology, Muscles parasitology, Sarcocystis isolation & purification, Sarcocystosis veterinary

Abstract

Muscular sarcocystosis by Sarcocystis arctica was found for the first time in the Czech Republic, in different muscles of red fox (Vulpes vulpes). Cysts were slim, elongated, thread-like, whitish, 1-7mm long, and 206-270μm wide; bradyzoites were 7.9×2.7μm in unstained wet mounts and 9.2×2.9μm in cyst Giemsa-stained smears. The cyst wall was thin, with short villi-like protrusions, and no host response was observed in the histological sections. Examination of the distribution and intensity of sarcocysts in 17 different muscle groups revealed that the highest intensity was in the cranial tibial muscle (>15 cysts in compressoria), followed by the diaphragm, forearm, and other groups (with intensities of 3-15 cysts in compressoria). Sarcocysts were detected in 3 out of 86 foxes. Genetic characterization at 18S rRNA, 28S rRNA, ITS1 and cox1, consistently showed that the species was identical with S. arctica. Interestingly, this protozoan was also detected as a co-infection in 3 foxes with the nematode Trichinella spp. for the first time., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2017

208. Sarcocystis pantherophisi n. sp., from Eastern Rat Snakes (Pantherophis alleghaniensis) as Definitive Hosts and Interferon Gamma Gene Knockout Mice as Experimental Intermediate Hosts.

Author

Verma SK, Lindsay DS, Mowery JD, Rosenthal BM, and Dubey JP

Subjects

Animals, Biological Assay, Brain parasitology, DNA, Protozoan chemistry, DNA, Protozoan isolation & purification, Gastrointestinal Contents parasitology, Interferon-gamma genetics, Mice, Mice, Knockout, Microscopy, Electron, Transmission veterinary, Muscle, Skeletal parasitology, Oocysts, Phylogeny, RNA, Ribosomal, 18S chemistry, RNA, Ribosomal, 18S genetics, Sarcocystis classification, Sarcocystis genetics, Sarcocystis isolation & purification, Sarcocystosis parasitology, Colubridae parasitology, Sarcocystis physiology, Sarcocystosis veterinary

Abstract

Here, we report a new species, Sarcocystis pantherophisi n. sp., with the Eastern rat snake (Pantherophis alleghaniensis) as natural definitive host and the interferon gamma gene knockout (KO) mouse as the experimental intermediate host. Sporocysts (n = 15) from intestinal contents of the snake were 10.8 × 8.9 μm. Sporocysts were orally infective to KO mice but not to laboratory-raised albino outbred house mice (Mus musculus). The interferon gamma KO mice developed schizont-associated neurological signs, and schizonts were cultivated in vitro from the brain. Mature sarcocysts were found in skeletal muscles of KO mice examined 41 days postinoculation (PI). Sarcocysts were slender, up to 70 μm wide and up to 3.5 mm long. By light microscopy, sarcocysts appeared thin-walled (<1 μm) without projections. By transmission electron microscopy, the sarcocyst wall was a variant of "type 1" (type 1i, new designation). The parasitophorous vacuolar membrane (pvm) had approximately 100-nm-wide × 100-nm-long bleb-like evaginations interspersed with 100-nm-wide × 650-nm-long elongated protrusions at irregular distances, and invaginations into the ground substance layer (gs) for a very short distance (6 nm). The gs was smooth, up to 500 nm thick, without tubules, and contained a few vesicles. Longitudinally cut bradyzoites at 54 days PI were banana-shaped, 7.8 × 2.2 μm (n = 5). Molecular characterization using 18S rRNA, 28S rRNA, ITS-1, and cox1 genes indicated a close relationship with other Sarcocystis parasites that have snake-rodent life cycles. The parasite in the present study was molecularly and biologically similar to a previously reported isolate (designated earlier as Sarcocystis sp. ex Pantherophis alleghaniensis) from P. alleghaniensis, and it was structurally different from other Sarcocystis species so far described.

Published

2017

209. Sarcocystis jamaicensis n. sp., from Red-Tailed Hawks (Buteo jamaicensis) Definitive Host and IFN-γ Gene Knockout Mice as Experimental Intermediate Host.

Author

Verma SK, von Dohlen AR, Mowery JD, Scott D, Rosenthal BM, Dubey JP, and Lindsay DS

Subjects

Animals, Biological Assay veterinary, DNA, Protozoan chemistry, Female, Interferon-gamma genetics, Intestines parasitology, Male, Mice, Mice, Knockout, Microscopy, Electron, Transmission veterinary, Muscle, Skeletal parasitology, Oocysts ultrastructure, Phylogeny, Sarcocystis genetics, Sarcocystis isolation & purification, Sarcocystosis parasitology, Sequence Analysis, DNA veterinary, Bird Diseases parasitology, Hawks parasitology, Sarcocystis classification, Sarcocystosis veterinary

Abstract

Here, we report a new species of Sarcocystis with red-tailed hawk (RTH, Buteo jamaicensis) as the natural definitive host and IFN-γ gene knockout (KO) mice as an experimental intermediate host in which sarcocysts form in muscle. Two RTHs submitted to the Carolina Raptor Center, Huntersville, North Carolina, were euthanized because they could not be rehabilitated and released. Fully sporulated 12.5 × 9.9-μm sized sporocysts were found in intestinal scrapings of both hawks. Sporocysts were orally fed to laboratory-reared outbred Swiss Webster mice (SW, Mus musculus) and also to KO mice. The sporocysts were infective for KO mice but not for SW mice. All SW mice remained asymptomatic, and neither schizonts nor sarcocysts were found in any SW mice euthanized on days 54, 77, 103 (n = 2) or 137 post-inoculation (PI). The KO mice developed neurological signs and were necropsied between 52 to 68 days PI. Schizonts/merozoites were found in all KO mice euthanized on days 52, 55 (n = 3), 59, 61 (n = 2), 66, and 68 PI and they were confined to the brain. The predominant lesion was meningoencephalitis characterized by perivascular cuffs, granulomas, and necrosis of the neural tissue. The schizonts/merozoites were located in neural tissue and were apparently extravascular. Brain homogenates from infected KO mice were infective to KO mice by subcutaneous inoculation and when seeded on to CV-1 cells. Microscopic sarcocysts were found in skeletal muscles of 5 of 8 KO mice euthanized between 55-61 days PI. Only a few sarcocysts were detected. Sarcocysts were microscopic, up to 3.5 mm long. When viewed with light microscopy, the sarcocyst wall appeared thin (<1 μm thick) and smooth. By transmission electron microscopy, the sarcocyst wall classified as "type 1j" (new designation). Molecular characterization using 18S rRNA, 28S rRNA, ITS-1, and cox1 genes revealed a close relationship with Sarcocystis microti and Sarcocystis glareoli; both species infect birds as definitive hosts. The parasite in the present study was biologically and molecularly different from species so far described in RTHs and we therefore propose a new species name, Sarcocystis jamaicensis n. sp.

Published

2017

210. Molecular characterization of Sarcocystis spp. in intestine mucosal scrapings and fecal samples of Pampas fox (Lycalopex gymnocercus).

Author

Scioscia NP, Gos ML, Denegri GM, and Moré G

Subjects

Animals, Animals, Wild parasitology, Birds parasitology, Female, Host Specificity, Intestine, Small parasitology, Male, Oocysts genetics, Oocysts isolation & purification, Polymerase Chain Reaction methods, Prevalence, Sarcocystosis epidemiology, Sarcocystosis parasitology, Feces parasitology, Foxes parasitology, Intestinal Mucosa parasitology, Sarcocystis genetics, Sarcocystosis veterinary

Abstract

Sarcocystis spp. are obligatory intracellular protozoan parasites which can infect humans and animals. Most of Sarcocystis species were identified based on the detection of muscle cysts in different intermediate hosts (IH). Regarding to natural infection in definitive host, there are few reports which have reached to determining species of Sarcocystis. The present work was aimed to studying the occurrence of Sarcocystis spp. (oocysts and sporocysts) in mucosal scrapings of small intestine and fecal samples of one the most abundant wild canids from South America, Lycalopex gymnocercus (Pampas fox), and to identify the Sarcocystis spp. using molecular tools. A total of 131 free-living L. gymnocercus were sampled in rural areas located in several departments from Buenos Aires province, Argentina. Fecal samples from all the animals and 33 small intestines were analyzed. Fecal and mucosal scrapings samples were analyzed by sugar flotation method and once oocysts or sporocysts were detected, sedimentation was performed and DNA extracted with a commercial kit. A PCR was conducted using primers targeting a fragment of the 18S rRNA gene and the amplicons were purified and sequenced. Of the total Pampas foxes analyzed, 23 (17.6%) had Sarcocystis spp. oocysts/sporocysts in fecal and/or mucosal samples. Sarcocystis spp. sporocysts were detected in 13.0% (17/131) of fecal samples and in 39.4% (13/33) of mucosal samples by the initial sugar flotation. Twenty one L. gymnocercus samples were processed by DNA extraction and PCR. Molecular identification of Sarcocystis spp. infection was successfully achieved in 14 foxes and was distributed as follows: 4.6% S. cruzi (6/131), 3.8% Sarcocystis spp. using birds as IH (S. albifronsi and S. anasi among others, 5/131), 0.8% S. tenella (1/131) and 1.5% (2/131) with low homology (97%) with S. miescheriana. In one fecal sample with spherical oocysts, the sequencing results showed a 100% sequence identity with Hammondia heydorni. The results show that the mucosal scrapings are the eligible sample to identify prevalence and to proceed with species identification. Lycalopex gymnocercus is suggested as definitive host for S. cruzi, S. tenella and probably various Sarcocystis spp. using birds as intermediate hosts as well as for H. heydorni., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2017

211. Morphology, Molecular Characteristics, and Demonstration of a Definitive Host for Sarcocystis rommeli from Cattle (Bos taurus) in China.

Author

Hu JJ, Huang S, Wen T, Esch GW, Liang Y, and Li HL

Subjects

Animals, Cat Diseases parasitology, Cats, Cattle, China, Cloning, Molecular, DNA, Protozoan chemistry, DNA, Protozoan isolation & purification, Electron Transport Complex IV genetics, Feces parasitology, Intestine, Small parasitology, Life Cycle Stages, Microscopy, Electron, Transmission veterinary, Mitochondria enzymology, Phylogeny, Polymerase Chain Reaction veterinary, RNA, Ribosomal, 18S genetics, Sarcocystis classification, Sarcocystis growth & development, Sarcocystosis parasitology, Sequence Alignment veterinary, Sequence Analysis, DNA, Cattle Diseases parasitology, Sarcocystis genetics, Sarcocystis ultrastructure, Sarcocystosis veterinary

Abstract

Sarcocysts of Sarcocystis rommeli were found for the first time in 6 of 34 (17.6%) cattle (Bos taurus) in China. With light microscopy, sarcocysts of S. rommeli were up to 1,130 μm long, with a striated, 4-8-μm-thick cyst wall. Using transmission electron microscopy, the villar protrusions (vp) were 4.7-5.2 × 0.2-0.3 μm, and 0.3-0.5 μm apart from each other. The vp contained microtubules extending from the top of the vp to the middle of the ground substance layer (gsl). A BLAST search of the near full-length 18S rRNA and partial mitochondrial cox1 sequences of S. rommeli revealed 98.7% identity and 99.2% identity with sequences of Sarcocystis bovini in GenBank, respectively. Two domestic cats (Felis catus) fed sarcocysts of S. rommeli shed oocysts/sporocysts in their feces with a prepatent period of 14 to 15 days; the partial mitochondrial cox1 sequences of these oocysts/sporocysts shared the high identities, that is, 99.4% and 99.5%, with cox1 sequences of S. rommeli sarcocysts and S. bovini sarcocysts, respectively. This is the first demonstration of a definitive host for S. rommeli.

Published

2017

212. Parasitemia due to Sarcocystis neurona-like infection in a clinically ill domestic cat.

Author

Zitzer NC, Marsh AE, Burkhard MJ, Radin MJ, Wellman ML, Jugan M, and Parker V

Subjects

Animals, Cat Diseases blood, Cat Diseases pathology, Cats, Chronic Disease, Male, Parasitemia parasitology, Parasitemia pathology, Sarcocystosis blood, Sarcocystosis parasitology, Sarcocystosis pathology, Cat Diseases parasitology, Parasitemia veterinary, Sarcocystis, Sarcocystosis veterinary

Abstract

An 8-year-old, 6-kg, male neutered Domestic Shorthair cat was presented to The Ohio State University Veterinary Medical Center (OSU-VMC) for difficulty breathing. Physical examination and thoracic radiographs indicated pneumonia, a soft-tissue mass in the left caudal lung lobe, and diffuse pleural effusion. The effusion was classified as modified transudate. Rare extracellular elongated (~5-7 μm × 1-2 μm) zoites with a central round to oval-shaped purple to deep purple vesicular nucleus with coarsely stippled chromatin and light blue cytoplasm were seen on a peripheral blood smear. Serum IgG and IgM were positive for Sarcocystis sp. antibodies and negative for Toxoplasma gondii antibodies, suggesting that the infection was acute rather than a recrudescence of prior infection. This organism was most consistent with either Sarcocystis neurona or Sarcocystis dasypi based on DNA sequence analysis of PCR products using COC ssRNA, ITS-1, snSAG2, and JNB25/JD396 primer sets. This is the first report to visualize by light microscopy circulating Sarcocystis sp. merozoites in the peripheral blood of a domestic cat. Therefore, Sarcocystis should be considered as a differential diagnosis in cats with suspected systemic protozoal infection., (© 2017 American Society for Veterinary Clinical Pathology.)

Published

2017

213. Molecular detection of Sarcocystis lutrae in the European badger (Meles meles) in Scotland.

Author

Lepore T, Bartley PM, Chianini F, Macrae AI, Innes EA, and Katzer F

Subjects

Animals, DNA, Ribosomal, DNA, Ribosomal Spacer genetics, Molecular Diagnostic Techniques, Phylogeny, Polymerase Chain Reaction, Sarcocystis classification, Sarcocystosis diagnosis, Sarcocystosis epidemiology, Sarcocystosis parasitology, Scotland epidemiology, Sequence Analysis, DNA, DNA, Protozoan genetics, Mustelidae parasitology, Sarcocystis genetics, Sarcocystis isolation & purification, Sarcocystosis veterinary

Abstract

Neck samples from 54 badgers and 32 tongue samples of the same badgers (Meles meles), collected in the Lothians and Borders regions of Scotland, were tested using polymerase chain reactions (PCRs) directed against the 18S ribosomal DNA and the internal transcribed spacer (ITS1) region of protozoan parasites of the family Sarcocystidae. Positive results were obtained from 36/54 (67%) neck and 24/32 (75%) tongue samples using an 18S rDNA PCR. A 468 base pair consensus sequence that was generated from the 18S rDNA PCR amplicons (KX229728) showed 100% identity to Sarcocystis lutrae. The ITS1 PCR results revealed that 12/20 (60%) neck and 10/20 (50%) tongue samples were positive for Sarcocystidae DNA. A 1074 bp consensus sequence was generated from the ITS1 PCR amplicons (KX431307) and showed 100% identity to S. lutrae. Multiple sequence alignments and phylogenetic analysis support the finding that the rDNA found in badgers is identical to that of S. lutrae. This parasite has not been previously reported in badgers or in the UK. Sarcocystis lutrae has previously only been detected in tongue, skeletal muscle and diaphragm samples of the Eurasian otter (Lutra lutra) in Norway and potentially in the Arctic fox (Vulpes lagopus).

Published

2017

214. Sarcocystis neurona and Neospora caninum in Brazilian opossums (Didelphis spp.): Molecular investigation and in vitro isolation of Sarcocystis spp.

Author

Gondim LSQ, Jesus RF, Ribeiro-Andrade M, Silva JCR, Siqueira DB, Marvulo MFV, Aléssio FM, Mauffrey JF, Julião FS, Savani ESMM, Soares RM, and Gondim LFP

Subjects

Animals, Biological Assay veterinary, Brazil epidemiology, Coccidiosis epidemiology, Coccidiosis parasitology, Melopsittacus, Mice, Phylogeny, Sarcocystis genetics, Sarcocystosis epidemiology, Sarcocystosis parasitology, Coccidiosis veterinary, Didelphis parasitology, Neospora isolation & purification, Sarcocystis isolation & purification, Sarcocystosis veterinary

Abstract

Sarcocystis neurona and Neospora spp. are protozoan parasites that induce neurological diseases in horses and other animal species. Opossums (Didelphis albiventris and Didelphis virginiana) are definitive hosts of S. neurona, which is the major cause of equine protozoal myeloencephalitis (EPM). Neospora caninum causes abortion in cattle and infects a wide range of animal species, while N. hughesi is known to induce neurologic disease in equids. The aims of this study were to investigate S. neurona and N. caninum in tissues from opossums in the northeastern Brazil, and to isolate Brazilian strains of Sarcocystis spp. from wild opossums for comparison with previously isolated strains. Carcasses of 39 opossums from Bahia state were available for molecular identification of Sarcocystis spp. and N. caninum in their tissues, and for sporocyst detection by intestinal scraping. In addition, Sarcocystis-like sporocysts from nine additional opossums, obtained in São Paulo state, were tested. Sarcocystis DNA was found in 16 (41%) of the 39 opossums' carcasses; N. caninum DNA was detected in tissues from three opossums. The sporocysts from the nine additional opossums from São Paulo state were tested by bioassay and induced infection in nine budgerigars, but in none of the gamma-interferon knockout mice. In vitro isolation was successful using tissues from all nine budgerigars. The isolated strains were maintained in CV-1 and Vero cells. Three of nine isolates presented contamination in cell culture and were discarded. Analysis of six isolates based on five loci showed that these parasites were genetically different from each other and also distinct from S. neurona, S. falcatula, S. lindsayi, and S. speeri. In conclusion, opossums in the studied regions were infected with N. caninum and Sarcocystis spp. and represent a potential source of infection to other animals. This is the first report of N. caninum infection in tissues from black-eared opossum (D. aurita or D. marsupialis) and white-eared opossum (D. albiventris). Brazilian opossums are probably infected by different Sarcocystis spp. distinct from S. neurona and S. falcatula, or present a high level of genetic recombination., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2017

215. Molecular characterization of the ribosomal DNA unit of Sarcocystis singaporensis, Sarcocystis zamani and Sarcocystis zuoi from rodents in Thailand.

Author

Watthanakaiwan V, Sukmak M, Hamarit K, Kaolim N, Wajjwalku W, and Muangkram Y

Subjects

Animals, DNA, Protozoan genetics, DNA, Protozoan isolation & purification, Phylogeny, RNA, Protozoan genetics, RNA, Ribosomal, 28S genetics, Rodent Diseases epidemiology, Rodentia, Sarcocystis classification, Sarcocystis isolation & purification, Sarcocystosis epidemiology, Sarcocystosis parasitology, Thailand epidemiology, Rodent Diseases parasitology, Sarcocystis genetics, Sarcocystosis veterinary

Abstract

Sarcocystis species are heteroxenous cyst-forming coccidian protozoan parasites with a wide host range, including rodents. In this study, Sarcocystis spp. samples were isolated from Bandicota indica, Rattus argentiventer, R. tiomanicus and R. norvegicus across five provinces of Thailand. Two major groups of Sarcocystis cysts were determined in this study: large and small cysts. By sequence comparisons and phylogenetic analyses based on the partial sequences of 28S ribosomal DNA, the large cysts showed the highest identity value (99%) with the S. zamani in GenBank database. While the small cysts could be divided into 2 groups of Sarcocystis: S. singaporensis and presupposed S. zuoi. The further analysis on 18S rDNA supported that the 2 isolates (S2 and B6 no.2) were as identified as S. singaporensis shared a high sequence identity with the S. singaporensis in GenBank database and the unidentified Sarcocystis (4 isolates, i.e., B6 no.10, B6 no.12, B10 no.4 and B10 no.7) showed 96.3-99.5% identity to S. zuoi as well as high distinct identity from others Sarcocystis spp. (≤93%). The result indicated that these four samples should be S. zuoi. In this study, we provided complete sequence of internal transcribed spacer 1 (ITS1), 5.8S rDNA and internal transcribed spacer 2 (ITS2) of these three Sarcocystis species and our new primer set could be useful to study the evolution of Sarcocystis.

Published

2017

216. Sarcocystis dehongensis n. sp. (Apicomplexa: Sarcocystidae) from water buffalo (Bubalus bubalis) in China.

Author

Chen X, Wen T, Hu J, Liu T, Esch GW, Liang Y, Li H, and Huang S

Subjects

Animals, China, DNA, Mitochondrial chemistry, DNA, Ribosomal chemical synthesis, DNA, Ribosomal genetics, Microscopy, Electron, Transmission veterinary, Phylogeny, RNA, Ribosomal, 18S genetics, Sarcocystis genetics, Sarcocystis isolation & purification, Sarcocystis ultrastructure, Sarcocystosis parasitology, Buffaloes parasitology, Sarcocystis classification, Sarcocystosis veterinary

Abstract

Water buffalo (Bubalus bubalis) is the intermediate host for at least four species of Sarcocystis: S. fusiformis, S. buffalonis, S. levinei, and S. sinensis/S. dubeyi. Here, a new species, Sarcocystis dehongensis, is reported in 51 of 756 (6.7%) water buffaloes in China. By light microscopy, the cysts of S. dehongensis were macroscopic, up to 18.5 mm long and 95 μm in diameter; 4.9-11.9 μm villous protrusions extended beyond the sarcocyst wall. Using transmission electron microscopy, the sarcocyst wall had lancet- or leaf-like protrusions in longitudinal section, but the cross section showed that the protrusions appeared as mushroom-like in shape with a core of tightly packed microtubules, similar to "type 24." BLAST searches revealed that S. dehongensis shared the most similarities with the 18S rDNA sequence of S. hardangeri (92.4%) and mitochondrial cox1 gene sequence of S. ovalis (81.0%), whereas no sequences in GenBank were found to be significantly similar to the ITS-1 region of S. dehongensis. A phylogenetic analysis based on 18S rDNA and mitochondrial cox1 gene sequences suggested that S. dehongensis was closely related to Sarcocystis species from cervids that employ corvids as definitive hosts.

Published

2017

217. Morphological and molecular characterization of Sarcocystis arctica-like sarcocysts from the Arctic fox (Vulpes lagopus) from Alaska, USA.

Author

Cerqueira-Cézar CK, Thompson PC, Verma SK, Mowery J, Calero-Bernal R, Antunes Murata FH, Sinnett DR, Van Hemert C, Rosenthal BM, and Dubey JP

Subjects

Alaska epidemiology, Animals, DNA, Ribosomal genetics, Microscopy, Electron, Transmission, Muscles parasitology, Phylogeny, Sarcocystis genetics, Sarcocystis isolation & purification, Sarcocystis ultrastructure, Sarcocystosis epidemiology, Sarcocystosis parasitology, Sequence Analysis, DNA veterinary, Tongue parasitology, Foxes parasitology, Sarcocystis classification, Sarcocystosis veterinary

Abstract

The muscles of herbivores commonly harbor sarcocysts of parasites belonging to species in the genus Sarcocystis, but such muscle parasites are rare in carnivores. Here, we report Sarcocystis arctica-like sarcocysts in muscles of Arctic foxes (Vulpes lagopus) from Alaska, USA, for the first time. The tongues of 56 foxes were examined for Sarcocystis infection using several methods. Sarcocystis bradyzoites were detected in pepsin digests of 13 (23.2%), and sarcocysts were found in histological sections stained with hematoxylin and eosin (HE) of 9 (16.0%). By light microscopy, sarcocysts were up to 4 mm long and up to 245 μm wide. In HE-stained sections, the sarcocyst wall appeared smooth and up to 1.5 μm thick without visible protrusions. By transmission electron microscopy, the sarcocyst wall had a wavy parasitophorous vacuolar membrane (pvm) folded as pleomorphic villar protrusions (vp), sometimes with anastomoses of villar tips. The vp and the ground substance (gs) layer were smooth and without microtubules. The gs was up to 2.0 μm thick. The total width of the wall including vp and the gs was up to 4.0 μm. The vp were up to 3.0 μm long and most closely resembled "type 9c." All sarcocysts were mature and contained numerous 8.1 × 2.1 μm sized bradyzoites. Molecular characterization (at 18S rDNA, 28S rDNA, ITS-1, and cox1) showed the highest affinity for S. arctica of the Arctic fox (V. lagopus) from Norway. In the present investigation, we provide evidence that sarcocysts are common in tongues of Alaskan Arctic foxes suggesting that these carnivores are serving as intermediate hosts, and we also provide ultrastructure of S. arctica from the Arctic fox for the first time.

Published

2017

218. Molecular confirmation of Sarcocystis fayeri in a donkey.

Author

Coultous RM, Raftery AG, Shiels BR, Sutton DGM, and Weir W

Subjects

Animals, Equidae blood, Phylogeny, Polymerase Chain Reaction methods, Sarcocystosis diagnosis, Sarcocystosis parasitology, Serologic Tests methods, DNA, Protozoan genetics, Equidae parasitology, Polymerase Chain Reaction veterinary, Sarcocystis genetics, Sarcocystosis veterinary, Serologic Tests veterinary

Abstract

Sarcocystis fayeri is a canine protozoan parasite with an equine intermediate host. Historically classified as an incidental pathogen, recent literature has described the toxic effects of Sarcocystis fayeri in human food poisoning, and highlighted potential involvement in equine neuromuscular disease. Until now, horses were believed to be the exclusive intermediate host. This study reports the first molecular confirmation of S. fayeri in a donkey, and gives rise to the consideration of donkeys being a potential reservoir for the parasite. This finding is of particular importance in understanding the epidemiology of this disease., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2017

219. Seroprevalences of anti-Sarcocystis neurona and anti-Neospora hughesi antibodies among healthy equids in the United States.

Author

James KE, Smith WA, Conrad PA, Packham AE, Guerrero L, Ng M, and Pusterla N

Subjects

Animals, Antibodies, Protozoan blood, Coccidiosis epidemiology, Coccidiosis parasitology, Cross-Sectional Studies, Encephalomyelitis epidemiology, Encephalomyelitis parasitology, Female, Horse Diseases blood, Horse Diseases parasitology, Horses, Male, Neospora immunology, Prevalence, Risk Factors, Sarcocystis immunology, Sarcocystosis epidemiology, Sarcocystosis parasitology, United States epidemiology, Coccidiosis veterinary, Encephalomyelitis veterinary, Horse Diseases epidemiology, Neospora isolation & purification, Sarcocystis isolation & purification, Sarcocystosis veterinary

Abstract

OBJECTIVE To describe the general seroprevalence of anti-Sarcocystis neurona and anti-Neospora hughesi antibodies among healthy equids by use of indirect fluorescent antibody tests and determine potential risk factors for seropositivity. DESIGN Cross-sectional study. SAMPLE Whole blood samples collected from 5,250 equids (1 sample/animal) across 18 states in the United States during October 2013. PROCEDURES Information regarding potential risk factors (geographic region, breed, primary use, sex, and age) was collected along with the blood samples. For each equid, an indirect fluorescent antibody test was used to determine serum titers of antibody against each of the 2 protozoal parasites. Mixed-effects logistic regression models were created to determine ORs for seropositivity. RESULTS The overall seroprevalence of anti-S neurona and anti-N hughesi antibodies in the tested equids was 78% and 34%, respectively. Of the equids, 31% were seropositive and 18% were seronegative for antibodies against both parasites. Factors associated with equids being seropositive for anti-S neurona antibodies were residence in the South, warmblood breed, and age > 5 years. Seroprevalence of anti-N hughesi antibodies did not differ among equids in different states across the country, but warmblood breed and age > 5 years were associated with seropositivity. CONCLUSIONS AND CLINICAL RELEVANCE With regard to risk factors for S neurona and N hughesi exposure and antibody response among tested equids, older age was not unexpected; however, the influences of warmblood breed and geographic location on seropositivity for anti-S neurona antibody but not for anti-N hughesi antibody deserve further investigation.

Published

2017

220. Pampas fox (Lycalopex gymnocercus) new intermediate host of Sarcocystis svanai (Apicomplexa: Sarcocystidae).

Author

Scioscia NP, Olmos L, Gorosábel A, Bernad L, Pedrana J, Hecker YP, Gual I, Laura Gos M, Denegri GM, Moore DP, and Moré G

Subjects

Animals, Foxes anatomy & histology, Microscopy, Electron, Transmission, Phylogeny, Polymerase Chain Reaction, RNA, Ribosomal, 18S genetics, Sarcocystis genetics, Sarcocystis ultrastructure, Sarcocystosis parasitology, Sarcocystosis physiopathology, Sarcocystosis transmission, South America, Tongue parasitology, Foxes parasitology, Muscle, Skeletal parasitology, Sarcocystis isolation & purification, Sarcocystis physiology, Sarcocystosis veterinary

Abstract

Several Sarcocystis spp. have carnivores as definitive host and sarcocysts are common in muscles of herbivores (intermediate host). However, sarcocysts have been found in muscles of wild and domestic carnivores suggesting they are intermediate host for some Sarcocystis spp. Here, we report mature sarcocysts in the muscles of Pampas fox (Lycalopex gymnocercus). A total of 36 free-living foxes were analyzed. Different skeletal muscles were assessed by microscopic and molecular methods. Cysts and/or DNA of Sarcocystis sp. were detected in 61.1% (22/36) foxes. Histopathology revealed the presence of sarcocysts in 52.8% (19/36) foxes. The tongue and masseter were the muscles more frequently infected. Of all the samples processed by homogenization of pooled muscles of each animal, 45.4% (10/22) evidenced muscle cysts and 68.2% (15/22) resulted positives by PCR. Individual cysts obtained from the ten positive samples in direct microscopic examination were all positive by PCR. Five amplicons from individual cysts from different samples were selected for sequencing together with four PCR products obtained from the pooled muscles. All nine sequences shared a high identity among them (99.8-100%) and showed the highest identity by BLAST (99%) with a S. svanai sequence (KM362428) from a North American dog. By transmission electron microscopy, the sarcocyst wall was thin (<1μm), had minute undulations, with tiny evaginations and without evident villar protrusions. The cyst wall type is referred as "type 1". Sarcocystis svanai infects L. gymnocercus with a high prevalence and the presence of mature sarcocysts suggests the role of the Pampas fox as natural intermediate host. The definitive host of S. svanai remains unknown., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2017

221. Sarcocystis neurona manipulation using culture-derived merozoites for bradyzoite and sporocyst production.

Author

Chaney SB, Marsh AE, Lewis S, Carman M, Howe DK, Saville WJ, and Reed SM

Subjects

Animals, Cryopreservation, Mice, Muscle, Skeletal parasitology, Sarcocystosis parasitology, Merozoites physiology, Oocysts physiology, Raccoons parasitology, Sarcocystis physiology, Sarcocystosis veterinary

Abstract

Equine protozoal myeloencephalitis (EPM) remains a significant central nervous system disease of horses in the American continents. Sarcocystis neurona is considered the primary causative agent and its intermediate life stages are carried by a wide host-range including raccoons (Procyon lotor) in North America. S. neurona sarcocysts mature in raccoon skeletal muscle and can produce central nervous system disease in raccoons, mirroring the clinical presentation in horses. The study aimed to develop laboratory tools whereby the life cycle and various life stages of S. neurona could be better studied and manipulated using in vitro and in vivo systems and compare the biology of two independent isolates. This study utilized culture-derived parasites from S. neurona strains derived from a raccoon or from a horse to initiate raccoon infections. Raccoon tissues, including fresh and cryopreserved tissues, were used to establish opossum (Didelphis virginiana) infections, which then shed sporocyts with retained biological activity to cause encephalitis in mice. These results demonstrate that sarcocysts can be generated using in vitro-derived S. neurona merozoites, including an isolate originally derived from a naturally infected horse with clinical EPM. This study indicates the life cycle can be significantly manipulated in the laboratory without affecting subsequent stage development, allowing further purification of strains and artificial maintenance of the life cycle., (Published by Elsevier B.V.)

Published

2017

222. Therapeutics for Equine Protozoal Myeloencephalitis.

Author

Pusterla N and Tobin T

Subjects

Animals, Encephalomyelitis drug therapy, Encephalomyelitis parasitology, Horses, Neospora isolation & purification, Sarcocystis isolation & purification, Sarcocystosis drug therapy, Sarcocystosis parasitology, Antiprotozoal Agents therapeutic use, Encephalomyelitis veterinary, Horse Diseases drug therapy, Horse Diseases parasitology, Sarcocystosis veterinary

Abstract

Equine protozoal myeloencephalitis is an infectious disease of the central nervous system caused by Sarcocystis neurona or Neospora hughesi. Affected horses routinely present with progressive and asymmetrical neurologic deficits. The diagnosis relies on the presence of neurologic signs, ruling out other neurologic disorders, and the detection of intrathecally derived antibodies to either S neurona and/or N hughesi. Recommended treatment is use of an FDA-approved anticoccidial drug formulation. Medical and supportive treatment is provided based on the severity of neurologic deficits and complications. This article focuses on recent data related to diagnosis, pharmacologic treatment, and prevention., (Copyright © 2016 Elsevier Inc. All rights reserved.)

Published

2017

223. Morphological and molecular characterization of four Sarcocystis spp., including Sarcocystis linearis n. sp., from roe deer (Capreolus capreolus) in Italy.

Author

Gjerde B, Giacomelli S, Bianchi A, Bertoletti I, Mondani H, and Gibelli LR

Subjects

Animals, Genetic Variation, Italy, Microscopy, Electron, Scanning, Muscles, Phylogeny, Polymerase Chain Reaction veterinary, RNA, Ribosomal, 18S genetics, Sarcocystis cytology, Sarcocystosis parasitology, Species Specificity, Deer, Sarcocystis genetics, Sarcocystosis veterinary

Abstract

Fresh (frozen/thawed) muscle samples from four 2-12-year-old roe deer (Capreolus capreolus) from the Sondrio province in north-eastern Italy were examined under a dissecting microscope, and about 180 sarcocysts were isolated and identified to morphological type in wet mounts by light microscopy (LM). Seventy-seven of these sarcocysts were subsequently examined by molecular methods, comprising polymerase chain reaction (PCR) amplification and sequencing of the partial cytochrome c oxidase subunit I gene (cox1) of all isolates, as well as PCR amplification, cloning and sequencing of the complete18S ribosomal RNA (rRNA) gene of two isolates of each species found. By LM, three major sarcocyst types were recognised: spindle-shaped sarcocysts, 0.5-3 mm long, either with no clearly recognisable protrusions (thin-walled) or with finger-like protrusions (thick-walled); and slender, thread-like sarcocysts, 2-3 mm long, with hair-like protrusions. Sequencing of cox1 revealed that the sarcocysts belonged to four different species. Those with no visible protrusions either belonged to Sarcocystis gracilis (n = 24) or to a Sarcocystis taeniata-like species (n = 19), whereas those with finger- and hair-like protrusions belonged to Sarcocystis silva (n = 27) and Sarcocystis capreolicanis (n = 7), respectively. The 19 cox1 sequences of the S. taeniata-like species, comprising five haplotypes, differed from each other at 0-16 of 1038 nucleotide positions (98.5-100% identity). They differed from 25 previous cox1 sequences of S. taeniata from moose and sika deer (with 98.0-100% intraspecific identity), at 33-43 nucleotide positions (95.9-96.8% interspecific identity), and there were 20 fixed nucleotide differences between the two populations. In the phylogenetic analysis based on cox1 sequences, the two populations formed two separate monophyletic clusters. The S. taeniata-like species in roe deer was therefore considered to represent a separate species, which was named Sarcocystis linearis n. sp. At the 18S rRNA gene, however, the two species could not be clearly separated from each other. Thus, there was considerable intraspecific sequence variation in the 18S rRNA gene of S. linearis (98.1-99.9% identity between 24 sequences), which was similar both in magnitude and nature to the variation previously found in this gene of S. taeniata. The new 18S rRNA gene sequences of S. linearis shared an identity of 97.9-99.6% with those of S. taeniata (overlap between intra- and interspecific identity), and in the phylogenetic tree, sequences of the two species were interspersed. By scanning electron microscopy (SEM), the sarcocysts of S. linearis were found to possess regularly spaced, thin and narrow ribbon-like cyst wall protrusions (about 2.8-3.2 μm long, 0.3-0.4 μm wide and about 0.02-0.03 μm thick), terminating in a plate-like structure of the same thickness but with an elliptic outline (about 0.3-0.4 μm wide and 0.7-0.9 μm long). The terminal plates were connected in the middle with the band-like portion of the protrusions like the board of a seesaw (tilting board). The terminal plates of adjacent protrusions were neatly arranged in a hexagonal pattern resembling tiles on a roof. Together, they formed an outer roof-like layer facing the surrounding cytoplasm of the host cell and completely covering the band-like proximal portion of the protrusions, which overlapped and were stacked in three to four layers close to the cyst surface. The sarcocyst morphology of S. linearis was consistent with that of an unnamed Sarcocystis sp. in roe deer previously found by transmission electron microscopy in several countries, including Italy. A few sarcocysts of S. gracilis and S. silva were also examined by SEM, confirming the presence of regularly distributed, short knob-like protrusions in S. gracilis (as seen in previous SEM studies) and revealing tightly packed, erect 6-7-μm-long villus-like protrusions having regularly distributed round depressions on their surface in S. silva. The sequencing of cox1 of 7, 24 and 27 new isolates of S. capreolicanis, S. gracilis and S. silva, respectively, recovered 7, 11 and 10 new haplotypes from each of the three species and expanded our knowledge on the intraspecific sequence variation at this marker. Similarly, the study revealed a more extensive intragenomic sequence variation at the 18S rRNA gene of S. capreolicanis and S. silva than known from previous studies and confirmed a near absence of such variation in the 18S rRNA gene of S. gracilis.

Published

2017

224. Isolation, molecular characterization, and in vitro schizogonic development of Sarcocystis sp. ex Accipiter cooperii from a naturally infected Cooper's hawk (Accipiter cooperii).

Author

Lindsay DS, Verma SK, Scott D, Dubey JP, and von Dohlen AR

Subjects

Animals, Cell Line, Chlorocebus aethiops, Cloning, Molecular, Cyclooxygenase 1 genetics, DNA, Ribosomal genetics, Microscopy, Electron, Transmission, Oocysts ultrastructure, Phylogeny, Polymerase Chain Reaction veterinary, RNA, Ribosomal genetics, Reproduction, Asexual physiology, Sarcocystis classification, Sarcocystis growth & development, Sarcocystosis parasitology, Schizonts growth & development, Schizonts ultrastructure, Sequence Analysis, DNA, Bird Diseases parasitology, Hawks parasitology, Sarcocystis genetics, Sarcocystis isolation & purification, Sarcocystosis veterinary

Abstract

Raptors serve as the definitive host for several Sarcocystis species. The complete life cycles of only a few of these Sarcocystis species that use birds of prey as definitive hosts have been described. In the present study, Sarcocystis species sporocysts were obtained from the intestine of a Cooper's hawk (Accipiter cooperii) and were used to infect cell cultures of African green monkey kidney cells to isolate a continuous culture and describe asexual stages of the parasite. Two clones of the parasite were obtained by limiting dilution. Asexual stages were used to obtain DNA for molecular classification and identification. PCR amplification and sequencing were done at three nuclear ribosomal DNA loci; 18S rRNA, 28S rRNA, and ITS-1, and the mitochondrial cytochrome c oxidase subunit 1 (cox1) locus. Examination of clonal isolates of the parasite indicated a single species related to S. columbae (termed Sarcocystis sp. ex Accipiter cooperii) was present in the Cooper's hawk. Our results document for the first time Sarcocystis sp. ex A. cooperii occurs naturally in an unknown intermediate host in North America and that Cooper's hawks (A. cooperii) are a natural definitive host., (Copyright © 2016 Elsevier Ireland Ltd. All rights reserved.)

Published

2017

225. Identification of Macroscopic Sarcocysts of Sarcocystis cameli from One-Humped Camel ( Camelus dromedarius ) in Iraq.

Author

Dubey JP, A'aiz NN, Mowery JD, Verma SK, and Calero-Bernal R

Subjects

Animals, Esophagus parasitology, Iraq, Microscopy, Electron, Transmission veterinary, Muscles parasitology, Sarcocystis classification, Sarcocystis ultrastructure, Sarcocystosis parasitology, Camelus parasitology, Sarcocystis isolation & purification, Sarcocystosis veterinary

Abstract

There is considerable confusion concerning the identity of macroscopic Sarcocystis species in camels. Currently 2 species, Sarcocystis cameli and Sarcocystis ippeni, are recognized from 1-humped camel ( Camelus dromedarius ), and sarcocysts of both species are microscopic. Here, we report the identity of macroscopic sarcocysts from the C. dromedarius in Iraq as S. cameli. Five sarcocysts from the muscle of 2 adult camels collected in 1999 and stored in 10% formalin were studied by transmission electron microscopy (TEM). Sarcocysts were 1.5-5.0 mm long and 200-400 μm wide. By TEM, all 5 sarcocysts had thin sarcocyst walls. Ultrastructurally, the sarcocyst wall had "type 9j" villar protrusions similar to those of S. cameli. This is the first confirmation of macroscopic sarcocysts from 1-humped camel as S. cameli.

Published

2017

226. Acute fatal sarcocystosis hepatitis in an Indo-Pacific bottlenose dolphin (Tursiops aduncus) in Hong Kong.

Author

Calero-Bernal R, Mauroo NF, Hui SW, Kuiken T, van de Bildt MW, de Jong AW, Osterhaus AD, Sims L, Gendron-Fitzpatrick A, Carmena D, Cerqueira-Cézar CK, Rosenthal BM, and Dubey JP

Subjects

Acute Disease, Animals, Fatal Outcome, Hepatitis, Animal diagnosis, Hong Kong, Liver parasitology, Liver pathology, Liver ultrastructure, Male, Phylogeny, Polymorphism, Single Nucleotide genetics, Sarcocystis classification, Sarcocystis genetics, Sarcocystis ultrastructure, Sarcocystosis diagnosis, Sarcocystosis parasitology, Schizonts, Sequence Analysis, DNA veterinary, Bottle-Nosed Dolphin parasitology, Hepatitis, Animal parasitology, Sarcocystis isolation & purification, Sarcocystosis veterinary

Abstract

Unlike most species in the genus Sarcocystis, Sarcocystis canis has a broad intermediate host range. Its life cycle is incompletely known and most reports are from the USA. Here we report fatal hepatitis in a 4year old male Indo-Pacific bottlenose dolphin (Tursiops aduncus) from Hong Kong associated with a S. canis-like infection. Diagnosis was made based on clinical presentation, histopathology, transmission electron microscopy (TEM), and molecular characterization. Microscopically, S. canis-like like infection was confined to the liver. Immature and mature schizonts were found in hepatocytes and the parasite was associated with generalized hepatic necrosis. By TEM, schizonts divided by endopolygeny, and merozoites lacked rhoptries. Molecular characterization of parasites present in liver and brain tissues at the cox1 gene showed a high degree of identity (97-98%) and clustered together with Sarcocystis canis, S. lutrae, S. arctica, S. speeri, S. turdusi, and S. rileyi in a phylogenetic study. This is the first report of S. canis-like infection from Asia., (Published by Elsevier B.V.)

Published

2017

227. Meningoencephalitis caused by pathogenic Sarcocystis species in a naturally infected sheep in Turkey.

Author

Alasonyalilar-Demirer A, Kahraman MM, Akkoç A, Erturkuner SP, Guzel EE, Kul O, and Ipek V

Subjects

Animals, Central Nervous System Protozoal Infections diagnosis, Central Nervous System Protozoal Infections pathology, Cerebellum parasitology, Cerebellum pathology, Cerebrum parasitology, Cerebrum pathology, Diagnosis, Differential, Heart parasitology, Myocardium pathology, Sarcocystis isolation & purification, Sarcocystis ultrastructure, Sarcocystosis diagnosis, Sarcocystosis pathology, Sheep, Sheep Diseases parasitology, Sheep Diseases pathology, Turkey, Central Nervous System Protozoal Infections veterinary, Sarcocystis pathogenicity, Sarcocystosis veterinary, Sheep Diseases diagnosis

Abstract

A 3-year-old sheep was examined after an acute onset of hind limb paralysis and ataxia. At necropsy, central nervous system, pulmonary and intestinal hyperaemia and ecchymoses in the aortic arch were observed. Main microscopic lesions were confined to the heart, cerebrum and cerebellum. There were a multifocal mild myocarditis and nonsuppurative meningoencephalitis together with protozoal cysts in the heart and the brain. Protozoal cystic structures were observed within many of the myocardial fibers as well as in the cerebrum and cerebellum. Using light microscopy it could not be morphologically determined whether these organisms were Toxoplasma (T.) gondii or Neospora (N.) caninum. Additional diagnostic methods like immunohistochemistry and polymerase chain reaction provided differentiation of Sarcocystis from T. gondii and N. caninum. Transmission electron microscopy demonstrated characteristic features of Sarcocystis sp. as previously described. This is the first confirmed diagnosis of Sarcocystis sp. in the central nervous system of a sheep from Turkey.

Published

2017

228. Necrotizing meningoencephalitis caused by Sarcocystis falcatula in bare-faced ibis (Phimosus infuscatus).

Author

Konradt G, Bianchi MV, Leite-Filho RV, da Silva BZ, Soares RM, Pavarini SP, and Driemeier D

Subjects

Alleles, Animals, Bird Diseases diagnosis, Bird Diseases pathology, Birds, Brain parasitology, Brain pathology, Brazil, Cytochromes b genetics, Male, Meningoencephalitis diagnosis, Meningoencephalitis parasitology, Meningoencephalitis pathology, Necrobiotic Disorders, Sarcocystis genetics, Sarcocystosis diagnosis, Sarcocystosis parasitology, Sarcocystosis pathology, Sequence Analysis, DNA veterinary, Bird Diseases parasitology, Meningoencephalitis veterinary, Sarcocystis isolation & purification, Sarcocystosis veterinary

Abstract

The infection by S. falcatula is commonly associated with respiratory disease in captive psittacine birds, with a few case reports of this protozoan causing encephalitis in wild birds. We describe the clinical, pathological, and molecular aspects of an infection by S. falcatula in a bare-faced ibis (Phimosus infuscatus). Clinically, wing paralysis and mild motor incoordination were observed. At necropsy, the telencephalic cortex showed multifocal to coalescing yellowish soft areas. Histologically, multifocal to coalescent nonsuppurative necrotizing meningoencephalitis of telencephalic cortex, cerebellum, and brainstem was observed. Necrotic areas showed multiple protozoan organism characteristics of Sarcocystis sp. schizonts in the cytoplasm of endothelial cells or lying free in the neuropil. Partial genetic sequences of the gene encoding cytochrome b (CYTB), the gene encoding the beta subunit of RNA polymerase (RPOB) and the first internal transcribed spacer (ITS-1) from Sarcocystis sp. schizonts revealed that the parasite had ITS-1 sequences that were 100% identical to the homologous alleles from Sarcocystis sp. shed by Didelphis albiventris in Brazil. RPOB and CYTB sequences were 100% identical to homologous of S. falcatula available in Genbank. Thus, this is the first report of necrotizing meningoencephalitis caused by S. falcatula in bare-faced ibis (P. infuscatus).

Published

2017

229. Environmental Persistence Influences Infection Dynamics for a Butterfly Pathogen.

Author

Satterfield DA, Altizer S, Williams MK, and Hall RJ

Subjects

Animals, Asclepias parasitology, Plant Leaves parasitology, Population Density, Sarcocystis physiology, Sarcocystosis transmission, Sarcocystosis veterinary, Spores, Protozoan pathogenicity, Spores, Protozoan physiology, Butterflies parasitology, Host-Parasite Interactions, Sarcocystis pathogenicity

Abstract

Many pathogens, including those infecting insects, are transmitted via dormant stages shed into the environment, where they must persist until encountering a susceptible host. Understanding how abiotic conditions influence environmental persistence and how these factors influence pathogen spread are crucial for predicting patterns of infection risk. Here, we explored the consequences of environmental transmission for infection dynamics of a debilitating protozoan parasite (Ophryocystis elektroscirrha) that infects monarch butterflies (Danaus plexippus). We first conducted an experiment to observe the persistence of protozoan spores exposed to natural conditions. Experimental results showed that, contrary to our expectations, pathogen doses maintained high infectivity even after 16 days in the environment, although pathogens did yield infections with lower parasite loads after environmental exposure. Because pathogen longevity exceeded the time span of our experiment, we developed a mechanistic model to better explore environmental persistence for this host-pathogen system. Model analysis showed that, in general, longer spore persistence led to higher infection prevalence and slightly smaller monarch population sizes. The model indicated that typical parasite doses shed onto milkweed plants must remain viable for a minimum of 3 weeks for prevalence to increase during the summer-breeding season, and for 11 weeks or longer to match levels of infection commonly reported from the wild, assuming moderate values for parasite shedding rate. Our findings showed that transmission stages of this butterfly pathogen are long-lived and indicated that this is a necessary condition for the protozoan to persist in local monarch populations. This study provides a modeling framework for future work examining the dynamics of an ecologically important pathogen in an iconic insect., Competing Interests: The authors have declared that no competing interests exist.

Published

2017

230. Sarcocystis entzerothi n. sp. from the European roe deer (Capreolus capreolus).

Author

Prakas P, Rudaitytė E, Butkauskas D, and Kutkienė L

Subjects

Animals, DNA, Protozoan genetics, DNA, Ribosomal genetics, Lithuania, Microscopy, Electron, Transmission, Phylogeny, Sarcocystis classification, Sarcocystis genetics, Sarcocystosis parasitology, Deer parasitology, Sarcocystis isolation & purification, Sarcocystosis veterinary

Abstract

In the present study, we describe Sarcocystis entzerothi n. sp. from the European roe deer (Capreolus capreolus) based on the microscopical and DNA analysis. By light microscopy (LM), cysts of S. entzerothi were spindle-shaped with pointed tips, 950-1900 × 70-150 μm in size and had 5-6 μm long finger-like cyst wall protrusions. Cyst wall of S. entzerothi by transmission electron microscopy (TEM) was type 10a-like; villar protrusions were up to 1.2 μm wide, densely packed, lying about 0.1 μm between each other, had profuse microgranules and microfilaments, parasitophorous vacuolar membrane had many minute invaginations, and the ground substance layer measured up to 0.4 μm. This species is morphologically similar to Sarcocystis silva, previously found in the roe deer and the moose (Alces alces). By LM, cysts of S. silva were cigar-shaped with blunted tips, measured 1000-1500 × 130-184 μm, and had 7-8 μm long finger-like cyst wall protrusions. Under TEM, S. silva had no clear differences from S. entzerothi in their cyst wall ultrastructure. Having examined six roe deer hunted in Lithuania, cysts of S. entzerothi and S. silva were identified in four and two animals, respectively. These two Sarcocystis species could be morphologically differentiated according to the shape of the cysts and the length of protrusions. The species examined showed 95.6-96.1 % and 85.6-86.9 % sequence identity within 18S ribosomal DNA (rDNA) and cox1, respectively, and therefore they could be clearly distinguished by means of molecular methods. It should be noted that in the 18S rDNA phylogenetic tree, S. entzerothi from the roe deer was placed together with one sequence of Sarcocystis sp. from the Lithuanian red deer (Cervus elaphus) demonstrating the same species. Based on 18S rDNA and cox1 sequences, S. entzerothi was more closely related to Sarcocystis species transmitted via felids than canids.

Published

2017

231. Antibodies against Apicomplexa protozoa and absence sarcocysts in heart tissues from horses in southern Brazil.

Author

Portella LP, Cadore GC, Sangioni LA, Pellegrini LF, Fighera R, Ramos F, and Vogel FS

Subjects

Animals, Brazil, Coccidiosis veterinary, Horse Diseases immunology, Horses, Myocardium immunology, Sarcocystosis veterinary, Seroepidemiologic Studies, Antibodies, Protozoan analysis, Heart parasitology, Horse Diseases parasitology, Neospora immunology, Sarcocystis immunology, Toxoplasma immunology

Abstract

Sarcocystis spp., Neospora spp., and Toxoplasma gondii are Apicomplexa protozoa that can infect horses. This study aimed to investigate the occurrence of antibodies against Sarcocystis spp., Neospora spp., and T. gondii in horses slaughtered in southern Brazil. The presence of histological lesions, tissue cysts, and Sarcocystis spp. DNA in the hearts of these horses was also investigated. A total of 197 paired serum and heart samples were evaluated by serology and direct microscopic examination; 50 of these samples were subjected to histopathological and PCR analyses. Antibodies against at least one of the protozoa were detected in 146 (74.1%) of the serum samples. The frequencies of positive serology were: 36% (71/197) against Sarcocystis spp., 39.1% (77/197) against Neospora spp., and 47.2% (93/197) against T. gondii. No cysts, Sarcocystis spp. DNA, or histopathological lesions were observed in myocardial tissue samples. The frequencies of antibody seropositivity against Sarcocystis spp., Neospora spp., and T. gondii showed that horses are frequently infected by these parasites in southern Brazil. The absence of sarcocysts in horse tissues is compatible with their role as aberrant/accidental hosts in the life cycle of Sarcocystis spp..

Published

2017

232. Sarcocystis spp. in domestic sheep in Kunming City, China: prevalence, morphology, and molecular characteristics.

Author

Hu JJ, Huang S, Wen T, Esch GW, Liang Y, and Li HL

Subjects

Animals, China epidemiology, DNA, Protozoan chemistry, DNA, Protozoan isolation & purification, DNA, Ribosomal Spacer genetics, Electron Transport Complex IV genetics, Genetic Markers, Microscopy, Electron, Transmission veterinary, Mitochondria enzymology, Muscles parasitology, Phylogeny, Prevalence, RNA, Ribosomal, 18S genetics, RNA, Ribosomal, 28S genetics, Sarcocystis classification, Sarcocystis genetics, Sarcocystis ultrastructure, Sarcocystosis epidemiology, Sarcocystosis parasitology, Sheep, Sheep Diseases epidemiology, Sarcocystis isolation & purification, Sarcocystosis veterinary, Sheep Diseases parasitology

Abstract

Sheep (Ovis aries) are intermediate hosts for at least six named species of Sarcocystis: S. tenella, S. arieticanis, S. gigantea, S. medusiformis, S. mihoensis, and S. microps. Here, only two species, S. tenella and S. arieticanis, were found in 79 of 86 sheep (91.9%) in Kunming, China, based on their morphological characteristics. Four genetic markers, i.e., 18S rRNA gene, 28S rRNA gene, mitochondrial cox1 gene, and ITS-1 region, were sequenced and characterized for the two species of Sarcocystis. Sequences of the three former markers for S. tenella shared high identities with those of S. capracanis in goats, i.e., 99.0%, 98.3%, and 93.6%, respectively; the same three marker sequences of S. arieticanis shared high identities with those of S. hircicanis in goats, i.e., 98.5%, 96.5%, and 92.5%, respectively. No sequences in GenBank were found to significantly resemble the ITS-1 regions of S. tenella and S. arieticanis. Identities of the four genetic markers for S. tenella and S. arieticanis were 96.3%, 95.4%, 82.5%, and 66.2%, respectively., (© J.-J. Hu et al., published by EDP Sciences, 2017.)

Published

2017

233. Seroepidemiology of Sarcocystis neurona and Neospora hughesi infections in domestic donkeys (Equus asinus) in Durango, Mexico.

Author

Alvarado-Esquivel C, Howe DK, Yeargan MR, Alvarado-Esquivel D, Alfredo Zamarripa-Barboza J, and Dubey JP

Subjects

Age Distribution, Animals, Antibodies, Protozoan blood, Coccidiosis epidemiology, Coccidiosis immunology, Cross-Sectional Studies, Enzyme-Linked Immunosorbent Assay veterinary, Female, Male, Mexico epidemiology, Sarcocystosis epidemiology, Sarcocystosis immunology, Seroepidemiologic Studies, Coccidiosis veterinary, Equidae parasitology, Neospora immunology, Sarcocystis immunology, Sarcocystosis veterinary

Abstract

There is currently no information regarding Sarcocystis neurona and Neospora hughesi infections in donkeys in Mexico. Here, we determined the presence of antibodies against S. neurona and N. hughesi in donkeys in the northern Mexican state of Durango. Serum samples of 239 domestic donkeys (Equus asinus) were assayed for S. neurona and N. hughesi antibodies using home-made enzyme-linked immunoassays; six (2.5%) of the 239 donkeys tested seropositive for S. neurona. The seroprevalence of S. neurona infection was comparable among donkeys regardless of their origin, health status, or sex. Multivariate analysis showed that seropositivity to S. neurona was associated with increased age (OR = 2.95; 95% CI: 1.11-7.82; p = 0.02). Antibodies to N. hughesi were found in two (0.8%) of the 239 donkeys. Both exposed donkeys were healthy, 3- and 6-year-old females. This is the first evidence of S. neurona and N. hughesi infections in donkeys in Mexico., (© C. Alvarado-Esquivel et al., published by EDP Sciences, 2017.)

Published

2017

234. First molecular detection and characterization of Sarcocystis species in slaughtered cattle in North-West Tunisia.

Author

Amairia S, Amdouni Y, Rjeibi MR, Rouatbi M, Awadi S, and Gharbi M

Subjects

Animals, Cattle Diseases epidemiology, Cattle Diseases parasitology, Meat, Polymerase Chain Reaction veterinary, Polymorphism, Restriction Fragment Length, Prevalence, Sarcocystis classification, Sarcocystis genetics, Tunisia epidemiology, Cattle parasitology, Red Meat parasitology, Sarcocystis isolation & purification, Sarcocystosis epidemiology, Sarcocystosis veterinary

Abstract

Sarcocystis spp. is one of the most prevalent foodborne parasites infecting both animals and humans. Consumption of raw or undercooked infected meat is a risk factor of human intestinal sarcocystosis. The present study aimed to estimate the prevalence of Sarcocystis species infecting slaughtered Tunisian cattle in North-West Tunisia (Béja governorate). DNA was extracted from 150 beef meat samples and a PCR-restriction fragment length polymorphism was used for identification. The overall infection prevalence of Sarcocystis spp. was 38% (57/150). Two species were identified, namely S. hominis (25%; 39/150) and S. cruzi (12%; 18/150). For both species, the highest prevalence was in Thibar locality (52.9 and 17.6% for S. hominis and S. cruzi, respectively). The molecular prevalence of S. cruzi was significantly higher in animals aged between two and eight years (19.2%; 10/52). This is the first molecular identification of Sarcocystis species in Tunisian cattle. Further studies in both human and animal Tunisian populations are needed to rank this parasitic disease among others., (Copyright © 2016 Elsevier Ltd. All rights reserved.)

Published

2016

235. Prevalance, Morphology, and Molecular Characterization of Sarcocystis heydorni Sarcocysts from Cattle (Bos Taurus) in China.

Author

Hu JJ, Wen T, Chen XW, Liu TT, Esch GW, and Huang S

Subjects

Animals, Cattle, Cattle Diseases epidemiology, Cattle Diseases transmission, China epidemiology, Cyclooxygenase 1 genetics, DNA, Mitochondrial chemistry, DNA, Protozoan chemistry, DNA, Ribosomal chemistry, Genetic Markers, Humans, Microscopy, Electron, Transmission, Phylogeny, Prevalence, RNA, Protozoan genetics, RNA, Ribosomal, 18S genetics, Sarcocystis genetics, Sarcocystis ultrastructure, Sarcocystosis epidemiology, Sarcocystosis parasitology, Sarcocystosis transmission, Cattle Diseases parasitology, Sarcocystis classification, Sarcocystosis veterinary

Abstract

Cattle are intermediate hosts for 2 zoonotic species of Sarcocystis, Sarcocystis hominis and Sarcocystis heydorni. Here we report S. heydorni from cattle for the first time in China. Sarcocysts of S. heydorni were found in muscle from 173 of 1,630 (10.6%) cattle in abattoirs (9.7% in skeletal muscles, 3.4% esophagus, 2.5% diaphragm, and 0.1% tongue; heart muscle was negative). By means of light microscopy, S. heydorni sarcocysts were thin-walled (<1 μm). Using transmission electron microscopy, the sarcocyst wall had short (0.3-0.5 × 0.5-0.9 μm) stubby protrusions, the tips of which contained electron-dense, disk-shaped plaques, similar to the sarcocyst wall type 29b. In preliminary transmission attempts, a human volunteer did not excrete sporocysts in feces after ingesting 579 sarcocysts S. heydorni isolated from cattle. Phylogenetic analysis using the 2 molecular markers (18S rRNA gene and mitochondrial cox1 gene) indicated S. heydorni shared the closest affinity with species of Sarcocystis, which employ ruminants as intermediate hosts and canids as definitive hosts.

Published

2016

236. DNA extraction methods and multiple sampling to improve molecular diagnosis of Sarcocystis spp. in cattle hearts.

Author

Bräunig P, Portella LP, Cezar AS, Libardoni F, Sangioni LA, Vogel FS, and Gonçalves PB

Subjects

Animals, Cattle, Cattle Diseases diagnosis, DNA, Protozoan genetics, DNA, Ribosomal genetics, DNA, Ribosomal isolation & purification, Heart parasitology, Polymerase Chain Reaction veterinary, Reproducibility of Results, Sarcocystis genetics, Sarcocystosis diagnosis, Sarcocystosis parasitology, Cattle Diseases parasitology, DNA, Protozoan isolation & purification, Sarcocystis isolation & purification, Sarcocystosis veterinary, Specimen Handling veterinary

Abstract

Molecular detection of Sarcocystis spp. in tissue samples can be useful for experimental and diagnostic purposes. However, the parasite spreads unevenly through tissues, forming tissue cysts, and the cystic wall is an obstacle in DNA extraction protocols. Therefore, adequate sampling and effective disruption of the cysts are essential to improve the accuracy of DNA detection by PCR. The aims of this study were to evaluate the suitability of four protocols for DNA extraction from cysts of Sarcocystis spp. present in bovine myocardium samples or after their harvest in phosphate-buffered saline (PBS) solution as well as determine the effects of single or multiple sampling on the accuracy of molecular diagnosis of sarcocystosis in cattle hearts. Cysts and myocardium samples from nine bovine hearts were randomly distributed to four DNA extraction protocols: kit, kit with modification, DNAzol, and cetyl-trimethyl ammonium bromide (CTAB). Samples were submitted to DNA extraction and PCR as replicates of each heart (simplicate, duplicate, and triplicate), and the probability of a true positive diagnostic was calculated. Among the protocols tested, the kit with modification was determined to be the most suitable for DNA extraction from cysts in PBS solution (92.6 % of DNA detection by PCR); DNAzol resulted in higher DNA detection frequency from bovine myocardium samples (48.1 %). Multiple sampling improved the molecular diagnosis of Sarcocystis spp. infection in cattle hearts, increasing at 22.2 % the rate of true positive diagnostic.

Published

2016

237. Prevalence, morphology, and molecular characteristics of Sarcocystis spp. in domestic goats (Capra hircus) from Kunming, China.

Author

Hu JJ, Liu TT, Liu Q, Esch GW, Chen JQ, Huang S, and Wen T

Subjects

Animals, China epidemiology, Cyclooxygenase 1 genetics, DNA, Protozoan chemistry, DNA, Protozoan genetics, DNA, Ribosomal chemistry, DNA, Ribosomal genetics, Goat Diseases parasitology, Goats, Mitochondria enzymology, Muscles parasitology, Phylogeny, Prevalence, Protozoan Proteins genetics, Sarcocystis enzymology, Sarcocystis genetics, Sarcocystis ultrastructure, Sarcocystosis epidemiology, Sarcocystosis parasitology, Sequence Analysis, DNA veterinary, Genetic Variation, Goat Diseases epidemiology, Sarcocystis classification, Sarcocystosis veterinary

Abstract

Despite the importance of worldwide goat production, little is known about the prevalence of Sarcocystis spp. in domestic goats (Capra hircus) in China. The aims of the present study were to determine prevalence of Sarcocystis spp. in domestic goats in Kunming, China, as well as to identify parasite species based on morphological characteristics and DNA sequence analysis. Only microscopic sarcocysts of Sarcocystis spp. were detected in 174 of 225 goats (77.3 %). By light and transmission electron microscopy, two species, i.e., Sarcocystis capracanis and Sarcocystis hircicanis, were identified. Two sarcocysts from each of the two species were randomly selected for DNA extraction; the 18S rRNA gene (18S rRNA), the 28S rRNA gene (28S rRNA), and the mitochondrial cytochrome c oxidase subunit 1 (cox1) were amplified by the polymerase chain reaction (PCR) and subsequently sequenced. The results were compared with other previously sequenced Sarcocystis species retrieved from GenBank. There was little sequence variation between two isolates of the same species. S. capracanis was most closely related with Sarcocystis tenella; 18S rRNA, 28S rRNA, and mitochondrial cox1 sequences shared identities of 95.7-99.1, 95.3, and 92.3-93.2 % with those of S. tenella, respectively. Thus, mitochondrial cox1 sequences seem to perform better than 18S rRNA sequences or 28S rRNA sequences for identification of the two species. S. hircicanis was most closely related to Sarcocystis arieticanis, i.e., 18S rRNA and 28S rRNA sequences of the former species shared 97.2-97.4 and 95.6-96.1 % identities with those of latter, respectively. Phylogenetic analysis inferred from the three genetic markers yielded similar results and indicated the two species were within a group of Sarcocystis species with canines as known, or presumed, definitive hosts.

Published

2016

238. Detection and Molecular Identification of Sarcocystis rileyi (Apicomplexa: Sarcocystidae) From a Northern Shoveler (Anas clypeata) in Mexico.

Author

Padilla-Aguilar P, Romero-Callejas E, Osorio-Sarabia D, Ramírez-Lezama J, Cigarroa-Toledo N, Machain-Williams C, Manterola C, and Zarza H

Subjects

Animals, Mexico, Phylogeny, Sarcocystis pathogenicity, Sarcocystosis veterinary, Ducks microbiology, Sarcocystis isolation & purification

Abstract

We detected macroscopic Sarcocystis cysts in a Northern Shoveler ( Anas clypeata ) in the Lerma Marshes, State of Mexico, Mexico in February 2014. The 5.0×2.0-mm macrocysts in the breast muscle of the duck were ovoid and yellow. Using an optical microscope, we saw parasitic forms of a Sarcocystis sp. among muscular fibers; the cysts measured 3.5×1.1 mm. The external wall had a smooth surface and the internal wall had a spongy texture. We identified the macrocysts as Sarcocystis rileyi according to sequences of the 18S rRNA gene, 28S rRNA gene, and ITS-1 region. Sarcocystosis should be considered in similar assessments in wild waterfowl in Mexico. Awareness of S. rileyi among anatids in the Lerma Marshes will contribute to more-effective conservation and management actions.

Published

2016

239. Protozoal-related mortalities in endangered Hawaiian monk seals Neomonachus schauinslandi.

Author

Barbieri MM, Kashinsky L, Rotstein DS, Colegrove KM, Haman KH, Magargal SL, Sweeny AR, Kaufman AC, Grigg ME, and Littnan CL

Subjects

Animals, Female, Hawaii epidemiology, Male, Protozoan Infections, Animal epidemiology, Protozoan Infections, Animal pathology, Sarcocystosis epidemiology, Sarcocystosis mortality, Sarcocystosis parasitology, Toxoplasmosis, Animal epidemiology, Toxoplasmosis, Animal parasitology, Protozoan Infections, Animal mortality, Sarcocystosis veterinary, Seals, Earless parasitology, Toxoplasmosis, Animal mortality

Abstract

Protozoal infections have been widely documented in marine mammals and may cause morbidity and mortality at levels that result in population level effects. The presence and potential impact on the recovery of endangered Hawaiian monk seals Neomonachus schauinslandi by protozoal pathogens was first identified in the carcass of a stranded adult male with disseminated toxoplasmosis and a captive monk seal with hepatitis. We report 7 additional cases and 2 suspect cases of protozoal-related mortality in Hawaiian monk seals between 2001 and 2015, including the first record of vertical transmission in this species. This study establishes case definitions for classification of protozoal infections in Hawaiian monk seals. Histopathology and immunohistochemistry were the primary diagnostic modalities used to define cases, given that these analyses establish a direct link between disease and pathogen presence. Findings were supported by serology and molecular data when available. Toxoplasma gondii was the predominant apicomplexan parasite identified and was associated with 100% of mortalities (n = 8) and 50% of suspect cases (n = 2). Incidental identification of sarcocysts in the skeletal muscle without tissue inflammation occurred in 4 seals, including one co-infected with T. gondii. In 2015, 2 cases of toxoplasmosis were identified ante-mortem and shared similar clinical findings, including hematological abnormalities and histopathology. Protozoal-related mortalities, specifically due to toxoplasmosis, are emerging as a threat to the recovery of this endangered pinniped and other native Hawaiian taxa. By establishing case definitions, this study provides a foundation for measuring the impact of these diseases on Hawaiian monk seals.

Published

2016

240. Prevalence and first molecular identification of Sarcocystis species in cattle and water buffaloes in India.

Author

Daptardar M, Singh BB, Aulakh RS, and Gill JP

Subjects

Animals, Buffaloes parasitology, Cattle parasitology, Cattle Diseases epidemiology, China, India epidemiology, Phylogeny, Polymerase Chain Reaction, Sarcocystis classification, Sarcocystosis epidemiology, Sarcocystosis parasitology, Cattle Diseases parasitology, Sarcocystis genetics, Sarcocystis isolation & purification, Sarcocystosis veterinary

Abstract

The importance of Sarcocystis hominis in causing zoonotic infections is well known. Recently, S. hominis like cysts have been reported from water buffalo in China. Previous studies indicate prevalence of Sarcocystis species in bovine populations in India but molecular evidence is required for proper species differentiation. We examined two hundred and ninety six cardiac tissue samples of Indian water buffaloes and cattle from northern and western parts of the country. Tissues were examined for Sarcocystis using intact cyst isolation method, pepsin acid digestion method and Sarcocystis 18S rRNA PCR. The combination of primers was used for 18S rRNA PCR amplification followed by sequencing. Twenty five representative samples were sent for sequencing and 19 readable sequences were obtained for phylogenetic analysis. Overall, the Sarcocystis cysts/zoites were recorded in 44% (95% CI 38-49%), 58% (95% CI 53-64%) and 68% (95% CI 63-73%) from both cattle and buffalo samples using intact cyst isolation, pepsin-HCl digestion method and conventional PCR, respectively. The results indicate that pepsin-HCl digestion method and conventional PCR are more sensitive than intact cyst isolation for detection of Sarcocystis species in tissue samples. The prevalence of Sarcocystis species was high in buffalo as compared to cattle intermediate hosts. Phylogenetic analysis indicated that more than one Sarcocystis species are circulating in cattle and water buffaloes in India. The results further indicate that experimental transmission studies are required to re-confirm the identities and host ranges of the Sarcocystis species in cattle and water buffaloes in India.

Published

2016

241. Detection of Zoonotic Protozoa Toxoplasma gondii and Sarcocystis suihominis in Wild Boars from Spain.

Author

Calero-Bernal R, Pérez-Martín JE, Reina D, Serrano FJ, Frontera E, Fuentes I, and Dubey JP

Subjects

Animals, Female, Male, Sarcocystosis epidemiology, Sarcocystosis parasitology, Seroepidemiologic Studies, Spain epidemiology, Swine, Swine Diseases epidemiology, Swine Diseases parasitology, Toxoplasmosis, Animal epidemiology, Zoonoses, Sarcocystis isolation & purification, Sarcocystosis veterinary, Sus scrofa, Toxoplasma isolation & purification, Toxoplasmosis, Animal parasitology

Abstract

Food safety regulations require the control of the presence of protozoa in meats destined for human consumption. Wild boar (Sus scrofa) meat may constitute a source of zoonoses. A 23.8% (688/2881) seroprevalence of anti-Toxoplasma gondii antibodies and 72.2% (662/910) Sarcocystis sarcocysts prevalence were detected among wild boars hunted in Southwestern areas of Spain. Identity of Sarcocystis spp. was performed by RFLP-PCR and sequencing, detecting S. miescheriana (7/8) and the zoonotic S. suihominis (1/8). Risk assessment studies of these coccidian in meats destined to human consumption are needed., (© 2015 Blackwell Verlag GmbH.)

Published

2016

242. Morphological and molecular characterization of Sarcocystis taeniata and Sarcocystis pilosa n. sp. from the sika deer (Cervus nippon) in Lithuania.

Author

Prakas P, Butkauskas D, Rudaitytė E, Kutkienė L, Sruoga A, and Pūraitė I

Subjects

Animals, Lithuania, Microscopy, Electron, Transmission, Phylogeny, RNA, Ribosomal, 18S genetics, Sarcocystosis parasitology, DNA, Ribosomal genetics, Deer parasitology, Electron Transport Complex IV genetics, Sarcocystis classification, Sarcocystis genetics, Sarcocystosis veterinary

Abstract

The diaphragm muscles of eight sika deer (Cervus nippon) bred in Lithuania were examined for Sarcocystis cysts. Two Sarcocystis species, Sarcocystis taeniata, which were previously reported in Canadian moose (Alces alces) and Argentinean red deer (Cervus elaphus), and Sarcocystis pilosa n. sp. were described using light microscopy (LM), transmission electron microscopy (TEM), 18S ribosomal DNA (rDNA), and subunit I of cytochrome c oxidase (cox1) sequences analysis. By LM, cysts of S. taeniata were 424.8 × 57.9 (200-837 × 30-100) μm in size and had a thin (up to 1 μm) and smooth cyst wall, while short ribbon-like protrusions arising from broadened cone-shaped bases were seen under TEM. Cysts of S. pilosa (by LM) were ribbon-shaped, measured 848.5 × 63.8 (350-1700 × 30-125) μm and had thin 7-8-μm long hair-like protrusions. By TEM, cyst wall was type 7a-like; protrusions arose from 0.3 μm wide dome-shaped base with minute indentations of the parasitophorous vacuolar membrane near it, the surface of protrusions seemed to be smooth, and the ground substance layer was thin (0.18-0.22 μm). The 18S rDNA, in contrast to the cox1, lacked variability to discriminate S. pilosa from closely related Sarcocystis hjorti from the red deer and moose. S. taeniata, but not S. pilosa, showed a considerable intraspecific variation in both genes analyzed. The phylogenetic analyses based on 18S rDNA and cox1 sequences suggest that canids are definitive hosts of both S. taeniata and S. pilosa. This paper represents the first identification of Sarcocystis species in the sika deer by morphological and molecular methods.

Published

2016

243. Domestic cats (Felis catus) are definitive hosts for Sarcocystis sinensis from water buffaloes (Bubalus bubalis).

Author

Gjerde B and Hilali M

Subjects

Animals, Cat Diseases transmission, Cats, Cattle, Cyclooxygenase 1 genetics, DNA, Protozoan analysis, Disease Reservoirs parasitology, Host-Parasite Interactions, Life Cycle Stages, Sarcocystis enzymology, Sarcocystis genetics, Sarcocystis physiology, Sarcocystosis transmission, Buffaloes parasitology, Cat Diseases parasitology, Disease Reservoirs veterinary, Sarcocystis isolation & purification, Sarcocystosis veterinary

Abstract

The definitive hosts of Sarcocystis sinensis in water buffaloes have hitherto been unknown, but the close similarity of this species to the cat-transmitted Sarcocystis bovifelis in cattle suggested they were felids. In a previous study, two domestic cats were fed macroscopic sarcocysts of Sarcocystis fusiformis contained within or dissected from the esophageal muscles of water buffaloes, while no microscopic sarcocysts of S. sinensis were noticed. Both cats started shedding small numbers of sporocysts 8-10 days post infection (dpi) and were euthanized 15 dpi. Using a PCR-based molecular assay targeting the mitochondrial cox1 gene of S. fusiformis, both cats were shown to act as definitive hosts for this species. In the present study, DNA samples derived from oocysts/sporocysts in the intestinal mucosa of both cats were further examined by PCR for the presence of S. sinensis using 2 newly designed primers selectively targeting the cox1 gene of this species. All 6 DNA samples examined from each cat tested positive for S. sinensis. A 1,038-bp-long portion of cox1 was amplified and sequenced as 2 overlapping fragments from 5 of these DNA samples. The 5 sequences shared 99.3-100% identity with 7 previous cox1 sequences of S. sinensis obtained from sarcocysts in water buffaloes. Additionally, amplification of the ITS1 region with primers targeting various Sarcocystis spp., yielded amplicons of 2 different lengths, corresponding to those obtained from sarcocyst isolates of S. sinensis and S. fusiformis, respectively. This is the first study to show that cats act as definitive hosts for S. sinensis.

Published

2016

244. Accipiter hawks (Accipitridae) confirmed as definitive hosts of Sarcocystis turdusi, Sarcocystis cornixi and Sarcocystis sp. ex Phalacrocorax carbo.

Author

Mayr SL, Maier K, Müller J, Enderlein D, Gruber AD, and Lierz M

Subjects

Animals, DNA, Intergenic genetics, DNA, Protozoan genetics, Feces parasitology, Germany, Polymerase Chain Reaction, Sarcocystis genetics, Sarcocystis isolation & purification, Sarcocystosis parasitology, Species Specificity, Bird Diseases parasitology, Hawks parasitology, Intestines parasitology, Oocysts cytology, Sarcocystis classification, Sarcocystosis veterinary

Abstract

Sarcocystis is a large genus of protozoan parasites with complex heteroxenous life cycles. For many species, either the intermediate or the definitive host is still unknown. In this study, 116 Accipiter hawks (Eurasian sparrowhawks and northern goshawks) were investigated for the presence of Sarcocystis spp. in their intestinal tract or their faeces. To gain a wide distribution, samples were collected throughout Germany within 2 years. It was possible to detect Sarcocystis-like oocysts in 65 samples. Sequencing of the ITS region or species-specific PCR identified 33 samples as Sarcocystis turdusi/Sarcocystis sp. ex A. nisus (18), Sarcocystis calchasi (6), Sarcocystis columbae (3), Sarcocystis cornixi (3) and Sarcocystis sp. ex Phalacrocorax carbo (3). Besides the known infestation with S. columbae, S. sp. ex A. nisus and S. calchasi the Accipiter hawks were thereby confirmed as definitive host of S. turdusi, S. cornixi and S. sp. ex Phalacrocorax carbo for the first time.

Published

2016

245. Comments on "Prevalence of Sarcocystis spp. and Hammondia spp. microcysts in esophagus tissue of sheep and cattle, emphasized on their morphological differences, Parasitol Res. 2014 Oct;113(10):3801-5.".

Author

Razmi GR

Subjects

Animals, Cattle, Cattle Diseases, Esophagus, Prevalence, Sarcocystidae, Sheep, Sheep Diseases, Sarcocystis, Sarcocystosis veterinary

Published

2016

246. Molecular detection of Sarcocystis aucheniae in the blood of llamas from Argentina.

Author

Martin M, Decker Franco C, Romero S, Carletti T, Schnittger L, and Florin-Christensen M

Subjects

Animals, Argentina epidemiology, Base Sequence, DNA, Protozoan genetics, DNA, Ribosomal genetics, Meat parasitology, Molecular Sequence Data, Parasitemia epidemiology, Parasitemia parasitology, RNA, Protozoan genetics, RNA, Ribosomal, 18S genetics, Sarcocystis classification, Sarcocystis genetics, Sarcocystosis blood, Sarcocystosis epidemiology, Sarcocystosis parasitology, Sensitivity and Specificity, Sequence Alignment, Sequence Homology, Nucleic Acid, Species Specificity, Camelids, New World parasitology, Livestock parasitology, Parasitemia veterinary, Parasitology methods, Ribotyping methods, Sarcocystis isolation & purification, Sarcocystosis veterinary

Abstract

Sarcocystis aucheniae are apicomplexan protozoa that infect South American camelids (SACs), giving rise to macroscopic cysts similar to rice grains in skeletal muscles. Visual detection of macrocysts in slaughtered animals hampers commercialization of SAC meat, a highly relevant economic exploitation for Andean rural families. Importantly, the consumption of undercooked S. aucheniae-infested meat causes gastroenteritis. A carnivore definitive host, possibly the dog, acquires the parasite when feeding on infected SAC meat, and later eliminates infective oocysts in its feces. The parasite cycle is completed when SACs ingest contaminated water or pastures. We hypothesized that parasite DNA can be detected in SAC blood using molecular methods. In order to test this hypothesis, a seminested PCR format was specifically designed to target the hypervariable 18S rRNA gene region of S. aucheniae. PCR conditions were optimized using genomic DNA extracted from macrocyst bradyzoites. A detection limit of up to 1 parasite in 10μl of llama blood was established based on DNA samples extracted from aliquots of S. aucheniae bradyzoite-spiked non-infected llama blood. The seminested PCR allowed to detect natural infections of S. aucheniae in llama blood samples originating in the Andean flatlands of Argentina. Specific amplification of S. aucheniae DNA was corroborated by amplicon sequencing. This is the first report of S. aucheniae detection in llama blood, which provides a valuable diagnostic tool for epidemiological studies and for the evaluation of the efficacy of control measures for this parasitosis., (Copyright © 2016 Asociación Argentina de Microbiología. Publicado por Elsevier España, S.L.U. All rights reserved.)

Published

2016

247. Molecular differentiation of bovine sarcocysts.

Author

Akhlaghi M, Razavi M, and Hosseini A

Subjects

Animals, Base Sequence, Cattle, Iran, Molecular Typing, Neospora classification, Neospora genetics, Polymerase Chain Reaction methods, Polymerase Chain Reaction veterinary, Polymorphism, Restriction Fragment Length, Prevalence, Cattle Diseases parasitology, Sarcocystis classification, Sarcocystosis veterinary

Abstract

Cattle are common intermediate hosts of Sarcocystis, and the prevalence in adult bovine muscle is close to 100 % in most regions of the world. Three Sarcocystis spp. are known to infect cattle as intermediate hosts, namely, S. cruzi, S. hirsuta, and S. hominis. The aim of the present study was the molecular identification and differentiation of these three species, Neospora caninum and Besnoitia by PCR and RFLP methods. Tissue samples were obtained from diaphragmatic muscle of 101 cattle slaughtered in Shiraz, Fars Province, Iran, for both smear preparation and DNA extraction. The samples were digested by Pepsin, washed three times with PBS solution before taking smears, fixed in absolute methanol and stained with 10 % Giemsa. The slides were examined microscopically for Sarcocystis bradyzoites and DNA was extracted from 100 mg of Sarcocystis-infected meat samples. Since the primers also bind to 18S rRNA gene of some tissue cyst-forming coccidian protozoa, DNA was also extracted from 100 μl of tachyzoite-containing suspension of N. caninum and Besnoitia isolated from goat to compare RFLP pattern. Polymerase chain reaction (PCR) was performed on DNA of samples which were microscopically positive for Sarcocystis. Five restriction enzymes Dra1, EcoRV, RsaI, AvaI, and SspI were used for RFLP and DNA of one sample from protozoa was sequenced. Based on the RFLP results, 87 (98.9 %) DNA samples were cut with DraI, indicating infection by S. cruzi. One sample (1.1 %) of PCR products of infected samples was cut only with EcoRV which showed S. hominis infection. Forty-eight samples (53.3 %) of PCR products were cut with both DraI, EcoRV, or with DraI, EcoRV, and RsaI while none of them was cut with SspI, which shows the mixed infection of both S. cruzi and S. hominis and no infection with S. hirsuta. It seems by utilizing these restriction enzymes, RLFP could be a suitable method not only for identification of Sarcocystis species but also for differentiating them from N. caninum and Besnoitia.

Published

2016

248. Sarcocystis arctica (Apicomplexa: Sarcocystidae): ultrastructural description and its new host record, the Alaskan wolf (Canis lupus).

Author

Calero-Bernal R, Cerqueira-Cézar CK, Verma SK, Mowery J, Carmena D, Beckmen K, and Dubey JP

Subjects

Alaska, Animals, DNA, Protozoan chemistry, DNA, Protozoan genetics, DNA, Ribosomal chemistry, DNA, Ribosomal genetics, Male, Microscopy, Electron, Transmission veterinary, Muscles parasitology, Phylogeny, Sarcocystosis diagnosis, Sarcocystosis parasitology, Sequence Analysis, DNA veterinary, Sarcocystis classification, Sarcocystis genetics, Sarcocystis isolation & purification, Sarcocystis ultrastructure, Sarcocystosis veterinary, Wolves parasitology

Abstract

Sarcocystis sarcocysts are common in muscles of herbivores but are rare in muscles of carnivores. Here, we report sarcocysts in the muscles of a gray wolf (Canis lupus) from Alaska, USA, for the first time. Sarcocysts extracted from the tongue of the wolf were up to 900 μm long and slender and appeared to have a relatively thin wall by light microscope. By transmission electron microscopy, the sarcocyst wall most closely resembled "type 9c," and had a wavy parasitophorous vacuolar membrane folded as pleomorphic villar protrusions (vp), with anastomoses of tips. The vp and the ground substance (gs) layer were smooth without tubules or granules. The gs was up to 2.0 μm thick. The total width of the wall including vp and the gs was 3.5 μm. The vp were up to 1.5 μm long. Mature sarcocysts contained numerous bradyzoites and few metrocytes. The bradyzoites were 9.5 μm long and 1.5 μm wide, and contained all organelles found in Sarcocystis bradyzoites with at least two rhoptries. Molecular characterization showed the highest identity for 18S rRNA, 28S rRNA, ITS-1, and cox1 sequences of Sarcocystis arctica of the Arctic fox (Vulpes lagopus) from Norway. The ultrastructure of S. arctica from the fox is unknown. Here, we provide ultrastructure of S. arctica from the Alaskan wolf for the first time. The definitive host of S. arctica remains unknown.

Published

2016

249. Pathology, immunohistochemistry, and ultrastructural findings associated with neurological sarcocystosis in cattle.

Author

Dubey JP, Calero-Bernal R, Verma SK, and Mowery JD

Subjects

Animals, Brain parasitology, Brain pathology, Cattle, Central Nervous System Diseases parasitology, Central Nervous System Diseases pathology, Male, Paraffin Embedding, Sarcocystosis pathology, Cattle Diseases parasitology, Central Nervous System Diseases veterinary, Sarcocystosis veterinary

Abstract

Paraffin-embedded blocks of brain of a nine months old bull calf that died of neurological signs in 1982 in Germany were restudied. Numerous schizonts and merozoites were found associated with extensive but focal necrosis and severe meningoencephalitis. Developing stages of schizonts as well as free merozoites were identified. The schizonts were primarily in perivascular areas. Ultrastructurally, schizonts were seen both in capillaries and in extravascular space. Merozoites were often concentrated in adventitial layers of capillaries. Schizonts divided by endopolygeny, the nucleus became multi-lobed, and at the terminal stage nuclear lobes were incorporated into budding merozoites. Individual merozoites were seen in neurons, astrocytes, oligodendrocytes, leukocytes, and vascular endothelial cells. Occasionally merozoites were present in the nucleus of mononuclear cells. Individual merozoites were ovoid, 3-5×2-3μm in size, and contained a prominent nucleus, numerous micronemes, a conoid, but no rhoptries. Schizonts and merozoites did not react to polyclonal rabbit Neospora caninum, Toxoplasma gondii, and Sarcocystis neurona antibodies but did react to Sarcocystis cruzi antibodies. Because of morphological characteristics and the type of lesions, the parasite was likely due to an unidentified Sarcocystis species, different from S. cruzi., (Published by Elsevier B.V.)

Published

2016

250. Seroepidemiology of Sarcocystis neurona, Toxoplasma gondii and Neospora spp. among horses in the south of the state of Minas Gerais, Brazil.

Author

Ribeiro MJ, Rosa MH, Bruhn FR, Garcia Ade M, Rocha CM, and Guimarães AM

Subjects

Animals, Antibodies, Protozoan, Brazil epidemiology, Coccidiosis epidemiology, Fluorescent Antibody Technique, Indirect veterinary, Horse Diseases microbiology, Horse Diseases parasitology, Horses, Neospora, Sarcocystis, Sarcocystosis epidemiology, Seroepidemiologic Studies, Toxoplasma, Coccidiosis veterinary, Horse Diseases epidemiology, Sarcocystosis veterinary, Toxoplasmosis, Animal epidemiology

Abstract

The present study used the indirect fluorescent antibody test (IFAT) to determine the seroprevalence of Sarcocystis neurona, Toxoplasma gondii and Neospora spp., and evaluated the variables associated with these infections among 506 apparently healthy horses, reared in the south of the state of Minas Gerais, Brazil. This study was conducted between April 2012 and October 2013. Among the horses, the true prevalence of S. neurona was 26% (95% CI: 22.0-30.4%), T. gondii 19.9% (95% CI: 15.5-24.8%) and Neospora spp. 23.9% (95% CI: 19.9-28.1%); and among the farms, 88.3% (95% CI: 74.4-91.6%), 71.6% (95% CI: 41-92.8%) and 85% (95% CI: 70.7-96.1%), respectively. Regarding mixed infection, 17 horses (3.4%) were seropositive for both S. neurona and T. gondii, 16 (3.2%) for T. gondii and Neospora spp. and 14 (2.8%) for S. neurona and Neospora spp. The associations between seropositivity and variables relating to the structure of the farm, management and health were analyzed using the logistic regression analysis, through the generalized estimating equations (GEE). The results suggest that the south of Minas Gerais is an enzootic area for S. neurona, T. gondii and Neospora spp. among horses, with prevalence of asymptomatic subclinical or chronic infections.

Published

2016