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Polymerase chain reaction method for the rapid detection of virulent Shigella spp. | ||
| International Journal of Molecular and Clinical Microbiology | ||
| مقاله 5، دوره 2، شماره 1، مهر 2012، صفحه 134-137 اصل مقاله (250.17 K) | ||
| نوع مقاله: Research Article | ||
| نویسندگان | ||
| Majid Alipour* 1؛ Maryam Talebjannat2؛ Mohammad Nabiuni3 | ||
| 1Department of microbiology, Islamic Azad University (IAU) - Babol Branch, Babol, Iran | ||
| 2Science and research branch, Islamic Azad University,Tehran, Iran | ||
| 3Department of Biological science, Tarbiat moallem university,Tehran, Iran | ||
| چکیده | ||
| Bacillary dysentery, or shigellosis, is a disease of humans in which the colonic epithelium is invaded by bacteria and subjected to inflammatory destruction. The aim of this study was to develop a polymerase chain reaction(PCR) test for detection of virulent Shigella spp.. For this purpose, the primers were designed to amplify a 526-bp internal region of the Shigella spp. icsA gene, which encodes IcsA (intracellular spread)/VirG protein, a 116-kDa surface exposed outer membrane protein that mediates actin polymerization to aid bacterial movement inside the cell. The use of PCR to amplify a specific icsA gene fragment serves as a highly specific and sensitive method to detect virulent bacteria of the genus Shigella. Specific DNA band was obtained by using isolated plasmid DNA of Shigella and a bacterial suspension. Amplification of extracted DNA from all other genera of the family Enterobacteriaceae and various other gram-positive bacteria yielded negative results. Therefore this PCR method, can serve as a routine protocol for detecting and identifying virulent Shigella spp. from clinical samples. | ||
| کلیدواژهها | ||
| Shigella spp icsA PCR | ||
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