Veuillez utiliser cette adresse pour citer ce document : http://dspace.univ-bouira.dz:8080/jspui/handle/123456789/15985
Affichage complet
Élément Dublin CoreValeurLangue
dc.contributor.authorRai, Abdelwahab-
dc.contributor.authorAmm, Zohra-
dc.contributor.authorAnes-Boulahbal, Dahbia Leila-
dc.contributor.authorASSADI, Aymen Amin-
dc.contributor.authorAmrane, Abdeltif-
dc.contributor.authorBaaloudj, Oussama-
dc.contributor.authorMouni, Lotfi-
dc.date.accessioned2024-02-13T10:14:03Z-
dc.date.available2024-02-13T10:14:03Z-
dc.date.issued2024-
dc.identifier.urihttp://dspace.univ-bouira.dz:8080/jspui/handle/123456789/15985-
dc.description.abstractEnteroviruses (EVs) represent a major cause of viral meningitis, being responsible for nearly 1 billion infections each year worldwide. Several techniques were developed to obtain better diagnostic results of EV infections. Herein, we evaluated the efficiency of EV detection through isolation on both Rhabdomyosarcoma (RD) and Vero cell line cultures, conventional reverse transcription-polymerase chain reaction (RT-PCR) and real-time RT-PCR. Thus, 50 cerebrospinal fluid (CSF) samples belonging to patients suspected to have viral meningitis in northern Algeria were collected, anonymously numbered from 1 to 50 and subjected to the above-mentioned techniques for EV detection. Using real-time RT-PCR, 34 CSF samples were revealed to be positive for viral origin of meningitis (68%). Thirteen of them were positive when the conventional RT-PCR was used (26%), and only three samples gave positive results when the cell culture technique was used (6%). Surprisingly, two cell culture-positive CSF samples, namely, 31 and 39, were negative using RT-PCR directly on the original samples. However, they turned to be positive when amplification was carried out on their corresponding cell culture supernatant. The cell-cultured viral isolates were then identified by sequencing their viral genome’s VP1 regions. All of them were revealed to belong to the echovirus 27 strain. This investigation demonstrates that RT-PCR techniques are often more sensitive, accurate and much faster, providing reliable results within a clinically acceptable timeframe. However, viral isolation on cell cultures remains crucial to obtain enough viral load for serological tests or even to avoid the rare, but existing, false negative PCR.en_US
dc.language.isoenen_US
dc.publisherUniversité Akli M'hand Oulhadj - Bouiraen_US
dc.subjectechovirusen_US
dc.subjectviral infectionsen_US
dc.subjectcentral nervous systemen_US
dc.subjectgene amplificationen_US
dc.subjectpicornaviridaeen_US
dc.subjectrhabdomyosarcomaen_US
dc.titleMolecular Amplification and Cell Culturing Efficiency for Enteroviruses’ Detection in Cerebrospinal Fluids of Algerian Patients Suffering from Meningitisen_US
dc.typeArticleen_US
Collection(s) :Articles



Tous les documents dans DSpace sont protégés par copyright, avec tous droits réservés.