Stray dogs are carriers of several zoonotic diseases such as leishmaniasis and canine monocytic ehrlichiosis (CME) as a result of poor nutrition, low hygienic conditions and lack of veterinary care. Thus, the Veterinary Research Institute (VRI) conducted a survey to determine the parasite pathogens such as blood protozoans, gastrointestinal parasites and ectoparasites in stray dogs with the collaboration of the Kuala Lumpur City Council Pest Control Unit. Skin, organ, faecal and blood samples were analysed and results indicate that Babesia canis, Babesia gibsoni, Ehrlichia canis, Hepatozoon canis and microfilaria of Dirofilaria immittis are the common parasites species found in the blood and organ samples in 2014. The faecal floatation technique showed the presence ofhelminth ova such as Trichuris, Ancylostoma and Toxocara species. All skin samples were positive for Rhipicephalus sanguineus ticks. As strays are closely linked to human habitats such as market and housing areas, it is vital that stray population control is strategically implemented to safeguard these common zoonotic infections from spreading to humans.

A study was conducted inthe Teaching Veterinary Clinical Complex,College of Veterinary Animal Sciences,Mannuthy to evaluate the efficacy ofclindamycin as potential monotherapytreatment plan for Babesia gibsoni infectionin dogs during the period from January2013 to March 2014. Dogs of variousbreeds and age groups belonging to bothsexes diagnosed of having Babesia gibsoniinfection by blood smear examination andconfirmed by PCR were selected for thestudy. These animals were treated withclindamycin @ 11mg/kg bw IV q24hr for10 days and supported with haematinics.All animals showed clinical cure withimprovement in appetite and physicalactivity, increase in haematologicalparameters including platelet count andimprovement in serum chemistry values.

In the present study, we employed flow cytometry to evaluate the level of parasitemia of Babesia gibsoni infecting canine erythrocytes in vivo and in vitro by using fluorescent nucleic acid staining. Peripheral blood samples from a B. gibsoni-infected dog and cultured B. gibsoni parasitizing in canine erythrocytes were stained with a membrane-permeable fluorescent nucleic acid stain, SYTO16. In this study, we utilized normal canine erythrocytes (LK erythrocytes) and canine erythrocytes containing high concentrations of potassium, reduced glutathione, and some free amino acids (HK erythrocytes) as host cells for culture. In vivo parasitized cells were discriminated completely from unparasitized cells and a correlation (r=0.998) between the percentage of SYTO16-positive cells and parasitemia in vivo was observed. On the other hand, in vitro erythrocytes could not be divided clearly into parasitized and unparasitized cells. However, when LK erythrocytes were used as host cells, the percentage of SYTO16-positive cells was the almost same as, and was well correlated (r=0.932) with the level of parasitemia. When HK erythrocytes were used as host cells, the percentage of SYTO16-positive cells was almost half of, but was correlated (r=0.982) with the level of parasitemia. Therefore, we attempted to observe the changes in the percentage of parasitized cells after treatment with antiprotozoal drug or mitochondria inhibitors by using flow cytometry. The changes in the percentage of SYTO16-positive cells corresponded well with the changes of the level of parasitemia when the parasites in HK erythrocytes were cultured with each compound. The present results suggest that flow cytometric detection using SYTO16 is a rapid and reliable method for monitoring parasitemia both in vivo and in vitro.