Fróðskaparrit - 31.12.2000, Side 175

Fróðskaparrit - 31.12.2000, Side 175
SNIKAR A SEYðl I FØROYUM 179 tained material was examined under a stereonricroscope and any nematodes pre- sent were collected and grouped, and their total number calculated. Colon, coecum and rectum The large intestine was opened and the con- tent washed out and poured through a sieve (mesh size of 212 pm). An aliquot of 50% of the content was searched for nematodes, and their total number calculated. Lungs The lungs were examined macroscopically to confirm the possible presence of lung- worms and nodular lesions associated with nematode infection. Samples from the nodules were examined microscopically, and the nematode larvae present were iden- tified. Liver The liver was cut into two-cm slices, and soaked in lukewarm physiological saline solution for 12 hours. Then the water was poured through a sieve (mesh diameter of 106 pm), to collect any flukes present. Dif- ferent mesh sizes were used as described above to be sure to retain all possible para- sites in the respective organ, but which al- lowed other material to pass through the sieve. Abdominal cavitv The abdominal cavity was searched for Cy- sticercus tenuicollis (Taenia hydatigená). Faeces. The faecal samples were examined by the McMaster flotation method (Hansen and Perry, 1994) to determine the number of nematode eggs per gram of faeces (epg) or protozoal oocysts per gram of faeces (opg). Two grams of faeces were collected from the rectum. Twenty-eight ml of flota- tion fluid (saturated water/NaCl with glu- cose 50 g per 100 ml) were added to make approximately 30 ml in total. It was mixed thoroughly. The McMaster counting cham- ber was filled with the mixed sample (0.15 ml). After five minutes, the sample was ex- amined under a microscope at 100 times magnification, and nematode eggs and Eimeria oocysts were counted. By multi- plication of the number of eggs 'or oocysts counted in both counting chambers by 50, the estimated total number in 1 g of faeces was found. A modified Baerman analysis (Hansen and Perry, 1994) was used to isolate larvae from the faeces. Ten grams of faeces were placed on two layers of gauze. The faeces, packed in the gauze, were then dipped into a conical beaker filled with lukewarm water and were left to sediment for approximate- ly 12 hours. The faeces were discarded and the supernatant was sucked off, leaving the sediment in the bottom. The beaker was filled with water again, it was left to sedi- ment for 15 minutes and the sediment was placed on a microscope slide for examina- tion. The degree of infection was estimat- ed as low, medium and high. Muellerius capillaris: low (less than 10 larvae per g faeces), medium (10-1,000) and high (1,000 and more). Dictyocaulus filaria: low (less than 5 larvae per g faeces), medi- um (5-50) and high (50-500). The fluke egg sedimentation method was
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