Rapid detection of HIV-1 viral RNA by real-time transcription mediated amplification assay

Message:
Abstract:
Background
Several different molecular methods have been developed that are capable of detecting HIV-1 in clinical specimens with different levels of sensitivity and specificity. This article describes the results of a reliability study on the development and application of a new real-time TMA method for isothermal detection of HIV-1.
Materials And Methods
In this ex Primental study, the molecular beacon primer and probe set were designed for a 176-base-pair region of HIV-1 pol gene using a specialized software. Logarithmic serial dilutions from 10-107 copies of an in-vitro transcribed RNA were used for determination of the analytical sensitivity of the assay. Clinical specimens that had previously been evaluated positive or negative by a valid commercial assay were used for assessing the clinical sensitivity and specificity of the assay.
Results
The analytical and clinical sensitivities of the assay were determined 500 copies/ml and 93.3%, respectively. The primers and the probe were HIV-1 specific and no cross-reaction was observed with other blood-borne viruses and human genome bioinformatically. The clinical specificity of the developed real-time TMA assay was examined experimentally using 20 negative samples and determined to be 100%.
Conclusion
The developed real-time TMA assay can be used as an appropriate tool for the rapid and isothermal detection of HIV-1 in patient's blood and plasma samples.
Language:
Persian
Published:
Journal of Arak University of Medical Sciences, Volume:15 Issue: 4, 2012
Pages:
18 to 25
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