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Cited 16 time in webofscience Cited 18 time in scopus
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A new single-step quantitative pathogen detection system: Template-tagging followed by multiplex asymmetric PCR using common primers and CE-SSCP SCIE SCOPUS

Title
A new single-step quantitative pathogen detection system: Template-tagging followed by multiplex asymmetric PCR using common primers and CE-SSCP
Authors
Shin, GWCho, YSHwang, HSOh, MHNam, HGPark, JHJung, GY
Date Issued
2009-08
Publisher
WILEY-V C H VERLAG GMBH
Abstract
Rapid diagnosis of bacterial infection is important for patient management and appropriate therapy during the early phase of bacteria-induced disease. Among the existing techniques for identifying microbial, CE-SSCP combined with 16S ribosomal RNA gene-specific PCR has the benefits of excellent sensitivity, resolution, and reproducibility. However, even though CE-SSCP can separate PCR products with high-resolution, multiplex detection and quantification are complicated by primer-dimer formation and non-specific amplification. Here, we describe a novel technique for multiplex detection and quantification of pathogens by template-tagging followed by multiplex asymmetric PCR and subsequent CE-SSCP. More specifically, we reverse transcribed 16S ribosomal RNAs from seven septicemia-inducing pathogens, tagged the templates with common end sequences, and amplified them using common primers. The resulting amplicons could be successfully separated by CE-SSCP and quantified by comparison to an internal standard. This method yielded results that illustrate the potential of this system for diagnosing infectious disease.
Keywords
CE-SSCP; Common primer; Diagnosis; Pathogen; Template-tagging; RIBOSOMAL-RNA GENE; REAL-TIME PCR; DNA MICROARRAY; MICROBIAL COMMUNITY; BACTERIAL PATHOGENS; IDENTIFICATION; ASSAY; AMPLIFICATION; DIAGNOSTICS; SAMPLES
URI
https://oasis.postech.ac.kr/handle/2014.oak/26271
DOI
10.1002/ELPS.200900074
ISSN
0173-0835
Article Type
Article
Citation
ELECTROPHORESIS, vol. 30, no. 15, page. 2728 - 2736, 2009-08
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