联合使用Pastorex Staph-Plus与两种新型显色琼脂(MRSA ID和CHROMagar MRSA)中的任意一种来检测耐甲氧西林金黄色葡萄球菌。
Combined use of Pastorex Staph-Plus and either of two new chromogenic agars, MRSA ID and CHROMagar MRSA, for detection of methicillin-resistant Staphylococcus aureus.
作者信息
Compernolle Veerle, Verschraegen Gerda, Claeys Geert
机构信息
Department of Microbiology, Ghent University Hospital, De Pintelaan 185, B-9000 Ghent, Belgium.
出版信息
J Clin Microbiol. 2007 Jan;45(1):154-8. doi: 10.1128/JCM.01115-06. Epub 2006 Nov 8.
We describe the search toward a fast and reliable strategy to detect and confirm the presence of methicillin-resistant Staphylococcus aureus (MRSA) in screening samples. First, we evaluated the sensitivities and specificities of oxacillin resistance screening agar (ORSA) with enrichment (tryptic soy broth [TSB] and ORSA [TSB-ORSA]) and without enrichment (ORSA), MRSA ID (MRSA_ID) plates, and CHROMagar MRSA (C_MRSA) plates, all of which were inoculated with equal volumes of a suspension made by emulsifying screening swabs. Whereas the sensitivities after 48 h were similar for all media tested (77% for MRSA_ID and ORSA; 73% for C_MRSA and ORSA after enrichment [TSB-ORSA]), the specificities of MRSA_ID (98% after 24 h and 94% after 48 h) and C_MRSA (98% after 24 h and 90% after 48 h) were superior to the specificities of ORSAs (92% after 24 h and 83% after 48 h) and TSB-ORSA (86% after 24 h and 81% after 48 h). Subsequently, the performance of the Pastorex Staph-Plus agglutination test with presumptive MRSA isolates taken directly from chromogenic agars (direct_Pastorex agglutination) was compared to that of the Pastorex Staph-Plus agglutination test with isolates from blood agar subcultures (conventional_Pastorex agglutination). When the direct_Pastorex agglutination test on MRSA_ID plates was combined with Gram staining, the direct_Pastorex agglutination test with samples from MRSA_ID plates was as reliable as the conventional_Pastorex agglutination test with samples from blood agar subcultures from MRSA_ID plates. In contrast, the direct_Pastorex agglutination test with samples from C_MRSA plates gave false-negative results. Finally, we calculated the processing times of the four different strategies, namely, (i) enrichment in TSB supplemented with NaCl, subsequent culture on ORSA, and the conventional_Pastorex agglutination test; (ii) direct inoculation of ORSA combined with conventional_Pastorex agglutination test; (iii) direct inoculation of MRSA_ID plates combined with Gram staining and the direct_Pastorex agglutination test; and (iv) direct inoculation of C_MRSA plates combined with Gram staining and the direct_Pastorex agglutination test. We concluded that the use of MRSA_ID in combination with Gram staining and the direct_Pastorex agglutination test is faster and more specific than the other strategies tested.
我们描述了一种用于在筛查样本中检测和确认耐甲氧西林金黄色葡萄球菌(MRSA)存在的快速可靠策略。首先,我们评估了含增菌(胰蛋白胨大豆肉汤[TSB]和ORSA[TSB - ORSA])和不含增菌(ORSA)的苯唑西林耐药性筛查琼脂(ORSA)、MRSA ID(MRSA_ID)平板以及CHROMagar MRSA(C_MRSA)平板的敏感性和特异性,所有这些平板均接种了等量的由筛查拭子乳化制成的悬液。尽管在48小时后所有测试培养基的敏感性相似(MRSA_ID和ORSA为77%;增菌后[TSB - ORSA]的C_MRSA和ORSA为73%),但MRSA_ID(24小时后为98%,48小时后为94%)和C_MRSA(24小时后为98%,48小时后为90%)的特异性优于ORSA(24小时后为92%,48小时后为83%)和TSB - ORSA(24小时后为86%,48小时后为81%)的特异性。随后,将直接从显色琼脂中获取的推测性MRSA分离株进行的Pastorex Staph - Plus凝集试验(直接_Pastorex凝集)与从血琼脂传代培养物中获取的分离株进行的Pastorex Staph - Plus凝集试验(传统_Pastorex凝集)的性能进行了比较。当将MRSA_ID平板上的直接_Pastorex凝集试验与革兰氏染色相结合时,MRSA_ID平板样本的直接_Pastorex凝集试验与MRSA_ID平板血琼脂传代培养物样本的传统_Pastorex凝集试验一样可靠。相比之下,C_MRSA平板样本的直接_Pastorex凝集试验产生了假阴性结果。最后,我们计算了四种不同策略的处理时间,即:(i)在补充有NaCl的TSB中增菌,随后在ORSA上培养,并进行传统_Pastorex凝集试验;(ii)直接接种ORSA并结合传统_Pastorex凝集试验;(iii)直接接种MRSA_ID平板并结合革兰氏染色和直接_Pastorex凝集试验;(iv)直接接种C_MRSA平板并结合革兰氏染色和直接_Pastorex凝集试验。我们得出结论,将MRSA_ID与革兰氏染色和直接_Pastorex凝集试验结合使用比所测试的其他策略更快且更具特异性。
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