首页> 外文期刊>Journal of Medical Microbiology: An Official Journal of the Pathological Society of Great Britain and Ireland >Development of a 4-valent genotyping assay for direct identification of the most frequent Pseudomonas aeruginosa serotypes from respiratory specimens of pneumonia patients
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Development of a 4-valent genotyping assay for direct identification of the most frequent Pseudomonas aeruginosa serotypes from respiratory specimens of pneumonia patients

机译:一种4 Venten基因分型测定,用于直接鉴定肺炎患者呼吸标本中最常见的假目表毒素血清型血清型

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Pseudomonas aeruginosa is a common cause of nosocomial infections and is associated with high rates of mortality. In order to facilitate rapid and sensitive identification of the most prevalent serotypes of P. aeruginosa, we have developed a 4-valent real-time PCR-based assay using oligonucleotides specific for open-reading frames constituting the O-antigen-specific lipopolysaccharide loci of P. aeruginosa. The assay simultaneously detects and differentiates between each of the four serotypes IATS-O1, -O6, -O11 and serogroup 2 (IATS-O2, -O5, and -O16) with high sensitivity and specificity in a single-tube reaction. No cross-reactivity was observed with other serotypes of P. aeruginosa or other microbial species, and reproducibility was demonstrated regardless of template, i.e. purified DNA, bacterial culture and clinical specimens (broncho-alveolar lavage). The limit of detection of the assay was approximately 100 copies per reaction for IATS-O1, -O2 and -O11, and 50 copies per reaction for IATS-O6. Comparison of the assay specificity with a commercially available slide agglutination kit showed consistent results; however, the number of non-typable isolates was reduced by 15 % using the genotyping assay. Use of the 4-valent genotyping assay in the context of a clinical trial resulted in identification of pneumonia patients positive for the IATS-O11 serotype, and hence eligible for therapy with panobacumab (an investigational monoclonal antibody against the O-polysaccharide of serotype IATS-O11).
机译:假单胞菌铜绿假单胞菌是医院感染的常见原因,与高死亡率相关。为了便于快速敏感的P.铜绿假单胞菌的血清型鉴定最普遍的血清型,我们已经使用寡核苷酸开发了一种基于4价实时PCR的测定,所述寡核苷酸特异于构成O-抗原特异性脂多糖基因座的开放读数框架P. eruginosa。该测定同时检测和分化四种血清型IATS-O1,-O6,-O11和血清群2(IATS-O2,-O5和-O16),在单管反应中具有高灵敏度和特异性。除铜绿假单胞菌或其他微生物物种的其他血清型没有观察到交叉反应性,无论模板,即纯化的DNA,细菌培养和临床标本(支气管 - 肺泡灌洗)都证明了再现性。测定的检测极限为IATS-O1,-O2和-O11的每反应约100份,每次反应IATS-O6的50份。与市售的载玻片凝集试剂盒的测定特异性的比较显示结果一致;然而,使用基因分型测定法减少了15%的非类型分离株的数量。在临床试验的背景下使用4 Venten基因分型测定导致患有IATS-O11血清型阳性的肺炎患者的鉴定,因此有资格获得Panobacumab的治疗(一种针对血清型IAt的O-多糖的调查单克隆抗体 - o11)。

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