Observations have been made over a 15-month period on the frequency distribution of human faecal deposits and infective larvae of Necator americanus in a hookworm endemic area. The agestructure of infective larvae in a field population and their vertical distribution in soils were determined. These studies were undertaken to examine the hypothesis that hookworm transmission in the tropics is discontinuous and limited mainly to the rainy season. The distribution of larvae was found to be overdispersed statistically and in general much greater numbers of L3s were recovered during the rainy season. The degree of overdispersion was also reduced during this season, and there was a tendency for larvae to be confined to the surface/topsoil. The implications of these findings have been discussed in relation to human hookworm parasitism in endemic areas of the tropics.
The pattern of transmission of human schistosomiasis was studied in Amagunze Village, eastern Nigeria, during 1986–1987. The prevalence of Schistosoma haematobium in 119 schoolboys aged 5–12 years was 79%. The geometric mean of intensity of infection was 49 eggs/10 ml urine and the frequency of visible haematuria was 25·2%. No S. mansoni infections were demonstrated. A marked seasonality in population density of Bulinus truncatus, B. forskalii and Biomphalaria pfeifferi was demonstrated with reduced densities during the late rainy and early dry seasons. Schistosoma sp. infected B. truncatus were found in the late dry and early rainy seasons in 2 out of 7 major human water contact sites studied. Seasonality and focality of transmission of S. haematobium and its high endemicity in the area were thus demonstrated.
Laboratory studies were undertaken to evaluate the role of environmental factors on the development of free-living stages of the cat hookworm Ancylostoma tubaeforme. An index of development calculated from the proportion of eggs that developed to the infective stage and the reciprocal of the development period, has suggested that the absence of 'high' temperatures (26 degrees - 30 degrees C) would significantly affect the L3 population in contaminated soils. There were, however, no significant differences in the size and lipid content of L3 that had developed at the different temperatures.
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