首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Evaluation of commercially available acridinium ester-labeled chemiluminescent DNA probes for culture identification of Blastomyces dermatitidis, Coccidioides immitis, Cryptococcus neoformans, and Histoplasma capsulatum.
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Evaluation of commercially available acridinium ester-labeled chemiluminescent DNA probes for culture identification of Blastomyces dermatitidis, Coccidioides immitis, Cryptococcus neoformans, and Histoplasma capsulatum.

机译:评估市售的cri啶鎓酯标记的化学发光DNA探针,用于培养鉴定皮肤芽孢杆菌,球虫球菌,新隐球菌和荚膜组织胞浆菌。

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摘要

Four commercially available acridinium ester-labeled DNA probes directed against rRNA were evaluated for their ability to identify Blastomyces dermatitidis, Coccidioides immitis, Histoplasma capsulatum, and Cryptococcus neoformans in culture. rRNA was extracted by sonication of 1- to 2-mm2 portions of cultures of fungi in two chaotropic reagents with glass beads. Following a heat inactivation step, the extracts were hybridized in solution with probes specific for each pathogen. The acridinium ester reporter moiety of nonhybridized probe was selectively hydrolyzed, and chemiluminescence of specific DNA:RNA hybrids was quantitated in relative light units with a luminometer. A positive identification required a relative light unit value of > or = 50,000. Sensitivity and specificity of the probes were determined by probing cultures of the respective pathogenic fungi (target) and nontarget fungi. Both mycelial and yeast forms of the dimorphic fungi (B. dermatitidis and H. capsulatum) were tested. For B. dermatitidis, sensitivity and specificity were 87.8 and 100%, respectively (74 target and 219 nontarget fungi tested). For C. immitis, sensitivity and specificity were 99.2 and 100%, respectively (122 target and 164 nontarget fungi tested). For H. capsulatum, sensitivity and specificity were 100 and 100%, respectively (86 target and 154 nontarget fungi tested). For C. neoformans, sensitivity and specificity were 97 and 100%, respectively (100 target and 230 nontarget fungi tested). For B. dermatitidis, C. immitis, and C. neoformans, repeat testing increased the respective sensitivities to 97.3, 100, and 100%. The high sensitivities and specificities of the probes, the relatively short time (less than 1 h) required to perform the assay, and the availability of standardized reagent kits make the acridinium ester-labeled DNA probes well suited to laboratories in need of a rapid method to identify these fungal pathogens. Further, use of the probes to identify pathogenic fungi as soon as colonies appear on primary recovery media significantly shortens the time to reporting.
机译:对四种针对rRNA的市售cri啶酯标记的DNA探针进行了评估,以鉴定其在培养中鉴定皮肤芽孢杆菌,球菌球菌,荚膜组织胞浆菌和新隐球菌的能力。通过在两种离液试剂中用玻璃珠对1至2 mm2的真菌培养物进行超声处理来提取rRNA。在热灭活步骤之后,将提取物在溶液中与每种病原体的特异性探针杂交。选择性水解未杂交探针的a啶酯报告分子,并使用发光计以相对光单位对特定DNA:RNA杂种的化学发光进行定量。阳性鉴定需要相对光单位值大于或等于50,000。探针的敏感性和特异性是通过探查各自的病原真菌(靶标)和非靶标真菌的培养物来确定的。测试了双态真菌(B. dermatitidis和H.荚膜菌)的菌丝体和酵母形式。对于皮肤病双歧杆菌,敏感性和特异性分别为87.8和100%(测试了74种靶标真菌和219种非靶标真菌)。对于秀丽隐杆线虫,敏感性和特异性分别为99.2和100%(测试了122种靶标真菌和164种非靶标真菌)。对于荚膜葡萄球菌,敏感性和特异性分别为100%和100%(测试了86种靶标真菌和154种非靶标真菌)。对于新孢梭菌,敏感性和特异性分别为97%和100%(测试了100种靶标真菌和230种非靶标真菌)。对于皮炎芽孢杆菌,C。immitis和C. neoformans,重复测试将各自的敏感性提高到97.3%,100%和100%。探针的高灵敏度和特异性,进行测定所需的时间相对较短(不到1小时)以及标准化试剂盒的可用性,使得a啶酯标记的DNA探针非常适合需要快速方法的实验室识别这些真菌病原体。此外,一旦菌落出现在主要恢复培养基上,立即使用探针鉴定病原真菌会大大缩短报告时间。

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