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Comparative detection of trypanosomal DNA by loop-mediated isothermal amplification and PCR from flinders technology associates cards spotted with patient blood. | LitMetric

Comparative detection of trypanosomal DNA by loop-mediated isothermal amplification and PCR from flinders technology associates cards spotted with patient blood.

J Clin Microbiol

Department of Veterinary Parasitology and Microbiology, Faculty of Veterinary Medicine, Makerere University, P.O. Box 7062, Kampala, Uganda.

Published: June 2010

AI Article Synopsis

  • The study evaluated the effectiveness of loop-mediated isothermal amplification (LAMP) methods for detecting trypanosomal DNA from blood samples of human African trypanosomiasis (HAT) patients in Uganda and Tanzania, comparing them to traditional PCR techniques.
  • LAMP methods showed significantly higher sensitivity than PCR, with RIME-LAMP detecting DNA in 95.3% of 128 samples, while the more established SRA-PCR detected DNA in only 78.9% of cases.
  • There was a strong correlation between RIME-LAMP and SRA-LAMP results, suggesting that LAMP could be a more efficient diagnostic tool for monitoring HAT, particularly in areas where the disease is prevalent.

Article Abstract

We analyzed DNA eluted from FTA (Flinders Technology Associates) cards spotted with blood from human African trypanosomiasis (HAT) patients admitted at Lwala Hospital in eastern Uganda and Kaliua Health Centre in northwestern Tanzania. The aims were to evaluate loop-mediated isothermal amplification (LAMP) for detection of trypanosomal DNA in clinical samples and to characterize the infecting trypanosomes to the subspecies level. LAMP targeting the Trypanozoon conserved random inserted mobile element (RIME-LAMP) and that for the serum resistance-associated (SRA) gene (SRA-LAMP) were performed. For comparison, PCRs for the SRA gene specific for Trypanosoma brucei rhodesiense (SRA-PCR) and that to amplify the Trypanosoma brucei gambiense-specific surface glycoprotein (TgSGP-PCR) were done. Out of 128 samples analyzed, SRA-PCR was positive in 101 samples (78.9% sensitivity; 95% confidence interval [CI], 71.1 to 85.1%), SRA-LAMP was positive in 120 (93.8%; 95% CI, 88.2 to 96.8%), while RIME-LAMP revealed signals in 122 (95.3%; 95% CI, 90.2 to 97.8%). RIME-LAMP and SRA-LAMP were each significantly more sensitive than SRA-PCR (P values of 0.000 and 0.001, respectively; Fisher's exact test). There was poor agreement between RIME-LAMP and SRA-LAMP and the SRA-PCR, yielding kappa values of 0.31 and 0.40, respectively. Agreement between SRA-LAMP and RIME-LAMP was almost perfect (kappa value, 0.85; 95% CI, 0.64 to 1). All the 128 field samples were negative by TgSGP-PCR. Blood spots from three T. b. gambiense HAT cases from northwestern Uganda were positive by TgSGP-PCR and RIME-LAMP. PCR took five times longer to execute than LAMP. LAMP may be useful to monitor emerging HAT foci or to test travelers returning from countries where HAT is endemic. It should be evaluated in a case-control study to determine its utility as a HAT diagnostic.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC2884477PMC
http://dx.doi.org/10.1128/JCM.00101-10DOI Listing

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