| Livestock Research for Rural Development 23 (11) 2011 | Guide for preparation of papers | LRRD Newsletter | Citation of this paper |
Indigenous chickens constitute over 81% of poultry in Kenya and produce 71% of eggs and poultry meat. Ecto- and haemoparasites limit production of these birds in the rural areas. However, there exists scanty information on these parasites infection in indigenous chicken. This study was conducted to determine and document the type and prevalence of haemoparasites affecting different ages and sex groups of free range indigenous chicken from two agro ecological zones: Lower highland 1 (LH1) in Embu District and Lower Midland 5 (LM5) in Mbeere District in Eastern Province, Kenya.
Of the 144 birds examined, 79.2% were infected with haemoparasites, with 62.3% single and 37.7% mixed haemoparasitic infections. Plasmodium gallinaceum was the most prevalent haemoparasite (53.5%) followed by Leucocytozoon schoutedeni (52.1%) and Hemoproteus spp., (3.5%). Grower birds had a prevalence of 83.3% for haemoparasites compared to 81.3% of adults, and 72.9% of chicks (p> 0.05). Male birds had 83.3% prevalence, while female birds had 75.0% (p> 0.05). LH1 was found to have a slightly high prevalence of 81.9% compared to LM5, 76.4% (p> 0.05). Hemoproteus spp were isolated in chickens from LH1 but not from LM5. This study has documented a high prevalence of haemoparasites, hence further studies to determine the impact of infection on the health and productivity of these birds, and evaluation of cost benefit of various control strategies need to be undertaken.
Key words: Age, agro-ecological zones, free range, sex
Poultry production in most tropical countries is based mainly on scavenging production system. This system exposes birds to a range of parasites (Sehgal et al 2006). However, the most striking problem in relation to village poultry production is their high mortalities within the first year after hatching (Permin et al 2002).Newcastle disease, helminthosis, coccidiosis and ecto- and haemoparasites have been reported to be the main problems affecting indigenous chicken in Malawi (Njunga 2003). In Kenya, information concerning these parasites has not been recently documented. Such information will be useful in disease diagnosis and implementation of a disease control programme hence improvements in the productivity of indigenous free ranging chicken. The aim of this study was therefore to determine the type and prevalence of haemoparasites infection in indigenous free-ranging village chickens in two different agro-ecological zones in Kenya.
A total of 144 indigenous chickens with matching for age, sex and agro ecological zones were purposively randomly selected (purposive in that specific age groups, sexes and numbers were selected between each agro-ecological zones) and purchased from smallholder farms and transported alive in cages to the laboratories at the University of Nairobi, Kabete for examination. Three blood smears were prepared from each bird, processed and examined for haemoparasites. Slides were subjected to a microscopic examination and results recorded.
Two agro-ecological zones in two neighboring districts were chosen for this study. The selection was based on the availability of free-ranging village indigenous rural poultry population in the areas and contrasting agro-ecological zones.
The other study area was the lower midland 5 (LM5) in Mbeere District. This is a semi-arid area with livestock (beef cattle, sheep and goats), poultry, millet and green gram as the main agricultural activities. It has a bimodal and erratic rainfall pattern with average annual rainfall of 180mm per year. Altitude is 1200 meters above sea level and temperatures range from 20-30°C (Onduru et al 2002).
Before slaughter, each chicken was subjected to a thorough clinical examination and observation recorded. Birds were then killed by dislocation of the atlanto-occipital joint, followed by severing of the carotid arteries and jugular veins using a scalpel blade. Blood was collected in universal bottles containing Ethylenediaminetetraacetic acid (EDTA) to prevent clotting. Three blood films were prepared from each bird namely: a fresh thin blood smear, blood smear from EDTA blood and a buffy coat smear. Blood films were air-dried within 5–10 seconds after preparation. Slides were fixed in methanol for 5 minutes and then stained with 10% Giemsa for 15 minutes, washed with tap water, blotted and examined under the microscope for haemoparasites (Nemi 1986).
Examination of Giemsa stained blood smears and buffy coat smears was carried out as described by Nemi (1986). Blood films were examined for 10–15 minutes at low magnifications of X40, X63 and then 100 fields were studied at high magnification (X100). The haemoparasites detected were identified according to Soulsby (1982) and Valkiūnas (2005) and recorded.
The prevalence of haemoparasitic infection was defined as the total number of birds infested with a particular parasite group/ species divided by the number of chicken examined at a point in time (Margolis et al 1982). A Kruskal Wallis one-way analysis of variance (Genstat® Discovery Edition 3) was used to analyze the influence of three age and two sex groups and two agro-ecological zones on the prevalence. A critical probability of 0.05 was adopted throughout as a cut-off point for statistical significance between groups compared.
Out of 144 birds examined, 114 (79.2%) were infected with haemoparasites. Three species of haemoparasites were found during this study. These were Plasmodium spp., Leucocytozoon spp., and Haemoproteus spp. Plasmodium gallinaceum, 53.7% (77/144) was the most prevalent haemoparasite, followed closely by Leucocytozoon schoutedeni, 52.1% (75/144) and lastly Haemoproteus spp., 3.5% (5/144). Of the 114 infected birds, 71 (62.3%) had single infection, while 43 (37.7%) had more than one genera of haemoparasites (Table 1).
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| Figure 1. Blood smear showing a red blood cell (R) infected with a “signet-ring” merozoites (M) of Plasmodium gallinaceum (Giemsa stain, magnification X 1000). |
Figure 2. Blood smear
showing a red blood cell infected with Plasmodium gallinaceum (arrow) (Giemsa-stained, Magnification X 1000). |
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Figure 3 and 4. Chicken
blood smears showing football-like Leucocytozoon schoutedeni (cytoplasm of host cell- chc; nucleus of host cell-nhc; cytoplasm of parasite cell- cpc; nucleus of parasite- npc) (Giemsa-stained, magnification X1000) |
Figure 5. A Chicken blood
smear showing an elongated host cell nucleus (arrow) forming a long thin dark crescent band along one side of parasitized cell (Giemsa stained, magnification X 1000) |
The occurrence rate of Plasmodium was the same (56.3%) in adult and grower birds, but slightly lower in chicks (47.9%). Males had a slightly higher rate of infection with Plasmodium (56.9%) compared to female birds, 50%. Between the agro ecological zones, Lower highland 1 was found to have a slightly higher rate of infection. 61.1% (44/72) than the Lower midland zone 5, 45.8% (33/72). The difference in the rate of occurrence of Plasmodium gallinaceum among the bird age groups and sexes, and between the agro ecological zones was not statistically significant.
Out of the 114 birds infected with haemoparasites, 75 (65.8%) had Leucocytozoon schoutedeni. This parasite was found to infect the leukocytes. Parasites were spherical, ovoid or spindle-shaped containing one to four elongated deeply staining structures called host cell nucleus or lateral bars. Gametocytes caused marked enlargement and distortion of the infected cell producing a football-like appearance (Figure 3 and 4). Nucleus of the host cell was elongate and formed a long thin dark crescent along one side of parasitized cell (Figure 5). Macrogametes stained dark blue with Giemsa, and the nucleus was compact and had several vacuoles occurring in darkly stained cytoplasm. Microgametes were slightly smaller than macrogametes, their cytoplasm stained less deeply, usually pale blue in color, and the nucleus was diffuse and stained pale pink.
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Table 1. Prevalence of haemoparasites in birds (single or mixed infection) |
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Haemoparasite occurrence in birds |
Number of birds infected with haemoparasites (x) |
Percentage prevalence rate (x/144) |
|
Plasmodium species |
34 |
29.8 |
|
Leucocytozoon species |
36 |
31.6 |
|
Haemoproteus species |
1 |
0.9 |
|
Plasmodium species and Leucocytozoon species |
39 |
34.2 |
|
Plasmodium species and Hemoproteus species |
4 |
3.5 |
|
Leucocytozoon species and Hemoproteus species |
0 |
0.0 |
Results obtained from examination of blood smears revealed the presence of three haemoparasites (Plasmodium spp, Leucocytozoon spp and Haemoproteus spp) that were found to infect poultry in the study zones. Mixed infections with two of these haemoparasites were encountered. The findings of this study are consistent with the study by Sadiq et al (2003) in Ibadan, Nigeria, who reported the same three haemoparasites (Plasmodium spp, Leucocytozoon spp and Haemoproteus spp) during their study. In other studies in Malawi, Njunga (2003) reported the occurrence of Plasmodium gallinaceum, P. juxtanucleare and Aegyptinella pullorum. However, observation on haemoparasitism indicated that the indigenous chicken samples examined in this study lacked Aegyptinella spp., which is frequently encountered in birds in Africa (Poulsen et al 2000, Permin et al 2002 and Njunga 2003).
Prevalence of haemoparasites in birds in this study was found to be 79.2%. This high prevalence of blood parasites is comparable to the studies done by Valkiūnas et al (2005) who reported the prevalence of avian blood parasites in Uganda to be 61.9%, while Njunga (2003) in Malawi found the prevalence of haemoparasites in chicken to be 71%. There were no differences in occurrences among bird age groups, and across sexes and agro ecological zones. Findings among age groups were consistent with the findings of Permin et al (2002), who compared the prevalence between young and adult free range birds. All infected chickens in Zimbabwe (Permin et al 2002) had a low parasitaemia (<1% of erythrocytes were infected). However, there were no documented studies on the comparisons between sexes, and agro ecological zones. The reason for similar prevalence between bird’s age groups and across sexes and agro ecological zones were not clear hence should be studied further.
Plasmodium gallinaceum occurred in 77 of 144 birds (53.7%) examined and was the most prevalent haemoparasite encountered during our study. This high prevalence was in contrast to results found in a study in Zimbabwe where, 14 of 94 chickens (14.9%) harbored Plasmodium gallinaceum (Permin et al 2002), and that in Ghana where 27 of 100 birds (27.0%) harbored Plasmodium juxtanucleare (Poulsen et al 2000). This variation can be adequately attributed to variation between agro climatic conditions Fallis et al (1973), Adene and Dipeolu, (1975) and Permin et al (2002) indicated that Leucocytozoon spp. may be the most common hematozoan in these birds in Africa. This was however in contrast to the findings of the current study and that by Sadiq et al (2003), where Plasmodium spp., was found to be the most prevalent.
Of the three haemoparasites encountered, Plasmodium gallinaceum is the most pathogenic. Soulsby (1982) cited progressive emaciation, anaemia, enlargement of spleen and liver. Paralysis may be observed where there are massive numbers of exoerythrocytic forms in the endothelia cells of the brain capillaries and death in untreated cases. In Zimbabwe, Permin et al (2002) found that the differences in prevalence of Plasmodium gallinaceum were not significantly different between the bird’s ages (young and adult). This report was similar to our findings. However, there were no previous reports on comparison of occurrences of Plasmodium spp. between bird’s sexes and agro ecological zones. The differences in prevalence of Plasmodium spp. in this study is most likely connected to abundance and variations in appearance of vectors (Permin et al 2002).
Leucocytozoon schoutedeni was found in 75 (52.1%) of 144 birds examined. This prevalence was comparable to studies by Fallis et al (1973) who reported that of 150 chickens tested in Tanzania, more than 50% were infected with L. schoutedeni. Sehgal et al (2006) in their studies in Uganda found that the prevalence of L. schoutedeni was 31.0%, a prevalence that was lower than these findings. In Zimbabwe, 4 of 94 (4.3%) chickens’ harbored Leucocytozoon sabrazesi, but in Ghana, no Leucocytozoon infection was detected (Poulsen et al 2000). Earlier studies showed Leucocytozoon spp. infected 55 of 163 (34%) examined chickens in Ibadan, Nigeria (Adene and Dipeolu 1975). This variation in prevalence and distribution of various Leucocytozoon spp. can be attributed to agro climatic variation which affects vector distribution and adaptation of the Leucocytozoon spp., in different agro climatic zones. Leucocytozoon spp infection causes anaemia, thickened oral discharge and paralysis of legs (Sadiq et al 2003).
On the other hand, Haemoproteus was the least found haemoparasite during this study. This haemoparasite was found to infect birds from LH1 zone only, and has not been recently reported in other African countries. Variation in prevalence between LH1 and LM5 is likely due to a difference in geographical and climatic factors between the study areas. Haemoproteus infection is not particularly pathogenic in domestic chicken (Soulsby 1982).
This study revealed that there is a high prevalence of haemoparasitic infection in healthy looking indigenous chicken. However, there is a need to do further studies to assess the intensity of this infection and subsequent levels that can cause clinical disease. Predisposing factors to haemoparasite infection need to be examined. Also, the only test used in this study was microscopy which has a very low specificity and therefore more invasive tests need to be used as such can reveal a higher level of prevalence than the one reported here.
We acknowledge the chairman and technical staff of the Department of Veterinary Pathology, Microbiology and Parasitology, Kabete for their assistance during the setting up and running of laboratory work. Local guides and smallholder farmers from various villages in Embu and Mbeere where the study birds were purchased are appreciated for their indefatigable support and cooperation while sourcing for the study material. The study was financed by Danish International Development Agency (DANIDA) through the ENRECA program “Productivity and Health of Smallholder Livestock in East Africa (PHSL) and University of Nairobi grant no. 500-661-202.
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Received 17 December 2010; Accepted 1 October 2011; Published 4 November 2011