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Home / Equine Research Bank / J Parasitol / Experimental infection of ponies with Sarcocystis fayeri and...
The Journal of parasitology2005; 90(6); 1487-1491; doi: 10.1645/GE-313

Experimental infection of ponies with Sarcocystis fayeri and differentiation from Sarcocystis neurona infections in horses.

Abstract: Sarcocystis neurona and Sarcocystis fayeri infections are common in horses in the Americas. Their antemortem diagnosis is important because the former causes a neurological disorder in horses, whereas the latter is considered nonpathogenic. There is a concern that equine antibodies to S. fayeri might react with S. neurona antigens in diagnostic tests. In this study, 4 ponies without demonstrable serum antibodies to S. neurona by Western immunoblot were used. Three ponies were fed 1 x 10(5) to 1 x 10(7) sporocysts of S. fayeri obtained from dogs that were fed naturally infected horse muscles. All ponies remained asymptomatic until the termination of the experiment, day 79 postinoculation (PI). All serum samples collected were negative for antibodies to S. neurona using the Western blot at the initial screening, just before inoculation with S. fayeri (day 2) and weekly until day 79 PI. Cerebrospinal fluid samples from each pony were negative for S. neurona antibodies. Using the S. neurona agglutination test, antibodies to S. neurona were not detected in 1:25 dilution of sera from any samples, except that from pony no. 4 on day 28; this pony had received 1 X 10(7) sporocysts. Using indirect immunofluorescence antibody tests (IFATs), 7 serum samples were found to be positive for S. neurona antibodies from 1:25 to 1:400 dilutions. Sarcocystis fayeri sarcocysts were found in striated muscles of all inoculated ponies, with heaviest infections in the tongue. All sarcocysts examined histologically appeared to contain only microcytes. Ultrastructurally, S. fayeri sarcocysts could be differentiated from S. neurona sarcocysts by the microtubules (mt) in villar protrusions on sarcocyst walls; in S. fayeri the mt extended from the villar tips to the pellicle of zoites, whereas in S. neurona the mt were restricted to the middle of the cyst wall. Results indicate that horses with S. fayeri infections may be misdiagnosed as being S. neurona infected using IFAT, and further research is needed on the serologic diagnosis of S. neurona infections.
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Publication Date: 2005-02-18 PubMed ID: 15715250DOI: 10.1645/GE-313Google Scholar: Lookup
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Summary

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The research study evaluates the effects of experimental infection of Sarcocystis fayeri in ponies, its differentiation from Sarcocystis neurona, and any misinterpretations that may occur in diagnostic tests due to similarities between the two parasites. The findings revealed horses infected with S. fayeri could be incorrectly diagnosed with S. neurona, if using the indirect fluorescent antibody test (IFAT).

Research Method

The research experiment involved the following steps:

  • Four ponies with no discernable serum antibodies to S. neurona were selected for the experiment.
  • Three of these ponies were fed sporocysts of S. fayeri obtained from dogs that were fed naturally infected horse muscles. The sporocysts amounts varied from 1 x 10(5) to 1 x 10(7).
  • The ponies were kept in observation until the termination of the experiment at day 79 post-inoculation (PI).
  • Throughout the time period, weekly serum samples were collected for testing.

Findings

Researchers observed the following:

  • All ponies remained symptomless throughout the experiment duration.
  • Serum samples demonstrated no antibodies to S. neurona using the Western blot at any time instance.
  • Cerebrospinal fluid tests also established the absence of S. neurona antibodies.
  • A substantial number of serum samples tested positive for S. neurona antibodies but only through IFATs.
  • Sarcocysts from S. fayeri were found in the striated muscles of all the inoculated ponies, most heavily in the tongue.
  • A differentiation between S. fayeri and S. neurona sarcocysts could be accomplished by examining microtubules in the sarcocyst walls using ultrastructure.

Conclusion

The research data demonstrated a potential issue in the serologic diagnosis of S. neurona infections, as there is a considerable risk of horses with S. fayeri infections being misdiagnosed with S. neurona using IFATs. Therefore, the researchers have highlighted the need for further studies on the serologic diagnosis of S. neurona infections to eliminate such cross-reactions.

Cite This Article

APA
Saville WJ, Dubey JP, Oglesbee MJ, Sofaly CD, Marsh AE, Elitsur E, Vianna MC, Lindsay DS, Reed SM. (2005). Experimental infection of ponies with Sarcocystis fayeri and differentiation from Sarcocystis neurona infections in horses. J Parasitol, 90(6), 1487-1491. https://doi.org/10.1645/GE-313

Publication

The Journal of parasitology
ISSN: 0022-3395
NlmUniqueID: 7803124
Country: United States
Language: English
Volume: 90
Issue: 6
Pages: 1487-1491

Researcher Affiliations

Saville, W J A
  • Department of Veterinary Preventive Medicine, College of Veterinary Medicine, Ohio State University, Columbus, Ohio 43210-1092, USA. saville.4@osu.edu
Dubey, J P
    Oglesbee, M J
      Sofaly, C D
        Marsh, A E
          Elitsur, E
            Vianna, M C
              Lindsay, D S
                Reed, S M

                  MeSH Terms

                  • Agglutination Tests / veterinary
                  • Animals
                  • Antibodies, Protozoan / blood
                  • Blotting, Western / veterinary
                  • Diagnosis, Differential
                  • Dogs
                  • Fluorescent Antibody Technique, Indirect / veterinary
                  • Horse Diseases / diagnosis
                  • Horse Diseases / parasitology
                  • Horses
                  • Immunohistochemistry / veterinary
                  • Male
                  • Microscopy, Electron, Transmission / veterinary
                  • Microtubules / ultrastructure
                  • Microvilli / ultrastructure
                  • Random Allocation
                  • Sarcocystis / classification
                  • Sarcocystis / immunology
                  • Sarcocystis / ultrastructure
                  • Sarcocystosis / diagnosis
                  • Sarcocystosis / parasitology
                  • Sarcocystosis / veterinary
                  • Tongue / parasitology
                  • Tongue / ultrastructure

                  Citations

                  This article has been cited 5 times.
                  1. Marques C, da Silva B, Nogueira Y, Bezerra T, Tavares A, Borges-Silva W, Gondim L. Brazilian Horses from Bahia State Are Highly Infected with Sarcocystis bertrami.. Animals (Basel) 2022 Dec 10;12(24).
                    doi: 10.3390/ani12243491pubmed: 36552411google scholar: lookup
                  2. Zhang M, Wei K, Wu Z, Sun J, Hu J, Deng S, Tao J. Morphological and molecular characterization of a Sarcocystis species infecting donkeys from China.. Parasitol Res 2022 Oct;121(10):2917-2926.
                    doi: 10.1007/s00436-022-07616-2pubmed: 35941324google scholar: lookup
                  3. Dubey JP, Howe DK, Furr M, Saville WJ, Marsh AE, Reed SM, Grigg ME. An update on Sarcocystis neurona infections in animals and equine protozoal myeloencephalitis (EPM).. Vet Parasitol 2015 Apr 15;209(1-2):1-42.
                    doi: 10.1016/j.vetpar.2015.01.026pubmed: 25737052google scholar: lookup
                  4. Miller MA, Barr BC, Nordhausen R, James ER, Magargal SL, Murray M, Conrad PA, Toy-Choutka S, Jessup DA, Grigg ME. Ultrastructural and molecular confirmation of the development of Sarcocystis neurona tissue cysts in the central nervous system of southern sea otters (Enhydra lutris nereis).. Int J Parasitol 2009 Oct;39(12):1363-72.
                    doi: 10.1016/j.ijpara.2009.04.014pubmed: 19527725google scholar: lookup
                  5. Hoane JS, Morrow JK, Saville WJ, Dubey JP, Granstrom DE, Howe DK. Enzyme-linked immunosorbent assays for detection of equine antibodies specific to Sarcocystis neurona surface antigens.. Clin Diagn Lab Immunol 2005 Sep;12(9):1050-6.
                    doi: 10.1128/CDLI.12.9.1050-1056.2005pubmed: 16148170google scholar: lookup
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