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S. stercoralis is a helminthic parasite which is common in tropical and subtropical regions. It causes a persistent but often inapparent infection in humans. In the state of a protracted immunosuppression this parasite can cause a life-threatening hyperinfection syndrome. Most often the hyperinfection syndrome was found after prolonged high dose corticosteroid treatment. In HIV-infected individuals high dose corticosteroids are used for the treatment of the immune reconstitution inflammatory syndrome (IRIS) or as adjunct treatment in the treatment of meningeal or pericardial tuberculosis. Case reports from Tanzania demonstrate that Strongyloidiasis is prevalent not only in coastal regions but also in the Lake province of Tanzania. However, data on the local prevalence of S. stercoralis infection based on sensitive techniques are scanty, especially in HIV-infected individuals.
The main objective of this study is to provide data on the prevalence of S. stercoralis infections in the adult HIV-infected population attending the Bugando Medical Centre for medical care. Specific objectives of the study are the comparison of the sensitivities and specificities of five different methods in detecting S. stercoralis. Four methods to detect S. stercoralis larvae used stool samples; one method to detect S. stercoralis antibodies required blood samples. The study used the Agar-plate-culture-technique and a modified Harada-Mori-culture-technique for the direct detection of helminthic larvae in the collected faecal samples. In addition, a recently described PCR-assay from faecal specimens and an ELISA for S. stercoralis antibodies have been applied. The Faecal Parasite Concentrator (FPC) stool concentration technique was used for the differential diagnosis of other intestinal helminthic parasites. The results of the study may influence the current treatment guidelines for HIV-infected patients in case that a relevant prevalence of S. stercoralis infection is found. Then, prior to a prolonged iatrogenic immunosuppression -like the high dose corticosteroid treatment for IRIS- a prophylactic anthelminthic treatment capable to eradicate a S. stercoralis infection could be recommendable. The prevalence of a current S. stercoralis infection using the PCR as a gold standard was 5.4%. The Agar plate method showed positive results in 19 out of 278 cases (6.1%), the modified Harada Mori technique in 13 of 278 (4.7%) cases. With PCR as gold standard the sensitivity of the agar plate method was 60%, the positive predictive value 47.4%, the specificity 96.2% and the negative predictive value 97.7 %. The sensitivity of the Harada Mori technique was 36.4%, the positive predictive value 30.7% with a specificity of 96.4% and negative predictive value 97.1%. The modified Harada Mori technique allowed in principal the morphological identification of nematode larvae. Microscopic analysis showed a specificity of 100% and a sensitivity of 46.7%. Antibodies were detected in 45 of 278 cases 16.2% by ELISA, with a sensitivity of 92.9% and a specificity of 87.8%. The findings of this study show that none of the diagnostic tests can be implemented as a routine diagnostic procedure to diagnose a current infection. This leads to the conclusion that it is high time to consider the provision of a prophylactic treatment within patients who are either HIV positive patients who could develop an IRIS after receiving ART, patients with a HTLV-1 infection and the growing number of patients under iatrogenic immunosuppression for various reasons.
The StrongPaed study in the paediatric ward of a referral hospital in Mwanza in the lake region of Tanzania showed the prevalence of S. stercoralis, G. lamblia, E. histolytica and E. dispar as well as of other intestinal parasites with various diagnostic methods.
The prevalence of S. stercoralis was 2-10 % depending on the diagnostic methods used. There were no symptomatic infections but only carriage of the nematode. The positive results differed greatly depending on the performed diagnostic methods. None of the diagnostics showed satisfying results, neither in sensitivity and specificity nor in feasibility for this population in an endemic region in sub-Saharan Africa. PCR and microscopy were limited by the low amount of examined stool samples and by the resulting lack of sensitivity. Stool cultures were limited by time-consuming procedures and mainly by the problem of differentiation from hookworm and the resulting lack of specificity. ELISA was limited by the need of blood samples and also by poor specificity in the ELISA used.
The prevalence of G. lamblia was high, but mostly only carriage and not symptomatic infections was seen. No E. histolytica was detected, but 8.5 % samples were positive for E. dispar. Among the performed diagnostics, the rapid test showed sufficient results. It showed better sensitivity than microscopy and is cheaper and more feasible than PCR. Differentiation between E. histolytica and E. dispar was only possible with qPCR performed in Germany.
More children were positive for intestinal parasites from rural than from urban areas. The profession of the parents working as farmers was a risk factor for intestinal parasitic infections. Hygienic living conditions such as access to tap water and flush toilets at home were preventive for intestinal parasitic infections in children.
The present study investigates the infection rates of parasites, morbidity, and the living conditions of street children and orphans in Mwanza city, northern Tanzania. A high percentage of orphans and street children in Mwanza city is infected with one or more parasites. A significantly higher rate of infections with S. mansoni in street children as compared with orphans could be observed. The prevalence of S. mansoni determined by POC CCA test was 65.9% for orphans and 94.5% for street children. 19.2% of the orphans tested positive for S. mansoni in Kato Katz. Of the street children, 77.1% showed positive test results in Kato-Katz. Only 1.3% of the orphans stated in the questionnaire that they use the lake to wash, whereas 91.1% of the street children named the lake as at least one of their options for washing. Protozoal infections used as a marker for hygiene were at a comparable level for both groups. Microscopy showed positive results for G. intestinalis in 8.2% and for E. histolytica/dispar in 23% of orphans and 8.1% for G. intestinalis, and 23.8% for E. histolytica/dispar in street children. Through ultrasonography, we observed no signs of severe PPF and only a few mild PPF patterns. Most street children use the lake to wash and often do not have access to adequate sanitation. However, everyone in the study group indicated having access to safe drinking water. Overall, we found the general hygienic conditions for both groups to be inadequate. With the help of simple public health measures, like improve sanitation and regular mass drug administration, the overall situation would likely be considerably improved.
Even though the international combat against Neglected Tropical Diseases such as schistosomiasis or soil-transmitted helminthiases depends on reliable therapeutics, anthelminthic pharmacovigilance has been neglected on many national African drug markets. Therefore, quality and composition of 88 different batches of Albendazole, Mebendazole and Praziquantel locally collected from randomly selected facilities in Western Burkina Faso, Southeast Côte d’Ivoire, Southwest Ghana and Northwest Tanzania were analysed.
Visual examination of both packaging and samples was performed according to the WHO ‘Be Aware’ tool. Products were then screened with the GPHF Minilab, consisting of tests of mass uniformity, disintegration times and thin-layer chromatography (TLC). Confirmatory tests were performed according to international pharmacopoeiae, applying assays for dissolution profiles and high-performance liquid chromatography (HPLC).
Despite minor irregularities, appearance of the products did not hint at falsified medicines. However, 19.6 % of the brands collected in Ghana and Tanzania were not officially licensed for sale. Mass uniformity was confirmed in 53 out of 58 brands of tablets. 41 out of 56 products passed disintegration times; 10 out of the 15 failing products did not disintegrate at all.
TLC results did not reveal any falsifications or pronounced dosing errors. HPLC findings confirmed the TLC results despite shifted specification limits: ten of the 83 tested batches contained less than 90 %, none more than 110 % label claim. However, no more than 46.3 % (31 / 67) of the tablet batches assayed passed the respective criteria for dissolution.
In the four study countries, no falsified anthelminthic medicine was encountered. The active pharmaceutical ingredient was not found to either exceed or distinctively fall below specification limits. Galenic characteristics as most critical criteria however, especially dissolution profiles, revealed substantial deficits.