Single-tube and nested reverse transcriptase–polymerase chain reaction for detection of Rift Valley fever virus in human and animal sera

Rift Valley fever (RVF) is an anthropozoonosis caused by a Phlebovirus (Bunyaviridae family) that has re-emerged recently in East and West Africa in 1997–1998. This emphasizes the need for early and rapid detection of the virus and an efficient surveillance system. To this goal, a single tube or a n...

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Published inJournal of virological methods Vol. 91; no. 1; pp. 85 - 92
Main Authors Sall, A.A., Thonnon, J., Sene, O.K., Fall, A., Ndiaye, M., Baudez, B., Mathiot, C., Bouloy, M.
Format Journal Article
LanguageEnglish
Published London Elsevier B.V 2001
Amsterdam Elsevier
New York, NY
Subjects
Africa
Animals
Biological and medical sciences
Bunyaviridae
Diagnosis
Fundamental and applied biological sciences. Psychology
Humans
Mice
Microbiology
Phlebovirus
Reverse Transcriptase Polymerase Chain Reaction
Rift Valley Fever - diagnosis
Rift Valley fever virus
Rift Valley fever virus - isolation & purification
RNA, Viral - blood
Sensitivity and Specificity
Sheep
Bunyaviridae
Diagnosis
Phlebovirus
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Summary:Rift Valley fever (RVF) is an anthropozoonosis caused by a Phlebovirus (Bunyaviridae family) that has re-emerged recently in East and West Africa in 1997–1998. This emphasizes the need for early and rapid detection of the virus and an efficient surveillance system. To this goal, a single tube or a nested reverse transcriptase–polymerase chain reaction (RT–PCR) method focusing on the NSs coding region of the S segment was developed and used to detect the RVF virus (RVFV) genome, resulting respectively in the synthesis of 810 and 662 bp DNA amplimers. The assay was specific for RVFV and did not amplify any other phleboviruses known to circulate in sub-Saharan Africa. When serial dilutions of RVFV were artificially mixed with human normal serum, the minimal detection limits were 50 and 0.5 plaque forming units respectively using the simple and the nested RT–PCR. The RT–PCR method was efficient for the detection of RVFV RNA in the blood from experimentally RVFV-infected mice and lamb and the nested RT–PCR was found more sensitive than the virus isolation method. Additionally, this detection method was applied successfully for the diagnosis of human cases during the 1998 Mauritanian outbreak.
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ISSN:0166-0934
1879-0984
DOI:10.1016/S0166-0934(00)00252-4