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Identification of nucleotide sequences for the specific and rapid detection of Yersinia pestis
Authors:Radnedge L  Gamez-Chin S  McCready P M  Worsham P L  Andersen G L
Institution:Biology and Biotechnology Research Program, Lawrence Livermore National Laboratory, Livermore, California 94551, USA.
Abstract:Suppression subtractive hybridization, a cost-effective approach for targeting unique DNA, was used to identify a 41.7-kb Yersinia pestis-specific region. One primer pair designed from this region amplified PCR products from natural isolates of Y. pestis and produced no false positives for near neighbors, an important criterion for unambiguous bacterial identification.
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