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Rapid Antibiotic Combination Testing for Carbapenem-Resistant Gram-Negative Bacteria within Six Hours Using ATP Bioluminescence

机译:使用ATP生物发光在六小时内快速抗生素组合测试在六小时内耐药抗革兰阴性细菌

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To guide the timely selection of antibiotic combinations against carbapenem-resistant Gram-negative bacteria (CR-GNB), an in vitro test with a short turnaround time is essential. We developed an in vitro ATP bioluminescence assay to determine effective antibiotic combinations against CR-GNB within 6 h. We tested 42 clinical CR-GNB strains (14 Acinetobacter baumannii, 14 Pseudomonas aeruginosa, and 14 Klebsiella pneumoniae strains) against 74 single antibiotics and two-antibiotic combinations. Bacteria (approximately 5 log(10) CFU/ml) were incubated with an antibiotic(s) at 35 degrees C; ATP bioluminescence was measured at 6 h and 24 h; and the measurements were compared to viable counts at 24 h. Receiver operating characteristic (ROC) curves were used to determine the optimal luminescence thresholds (T-RLU) for distinguishing between inhibitory and noninhibitory combinations. The areas under the 6-h and 24-h ROC curves were compared using the DeLong method. Prospective validation of the established thresholds was conducted using 18 additional CR-GNB. The predictive accuracy of T-RLU for the 6-h ATP bioluminescence assay was 77.5% when all species were analyzed collectively. Predictive accuracies ranged from 73.7% to 82.7% when each species was analyzed individually. Upon comparison of the areas under the 6-h and 24-h ROC curves, the 6-h assay performed significantly better than the 24-h assay (P 0.01). Predictive accuracy remained high upon prospective validation of the 6-h ATP assay (predictive accuracy, 79.8%; 95% confidence interval [CI], 77.6 to 81.9%), confirming the external validity of the assay. Our findings indicate that our 6-h ATP bioluminescence assay can provide guidance for prospective selection of antibiotic combinations against CR-GNB in a timely manner and may be useful in the management of CR-GNB infections.
机译:为了指导及时选择抗菌组合对抗CarbapeNem抗性革兰氏阴性细菌(Cr-GNB),在短暂的周转时间内的体外测试是必不可少的。我们开发了体外ATP生物发光测定,以确定在6小时内对CR-GNB的有效抗生素组合。我们测试了42种临床CR-GNB菌株(14例肺杆菌,14例铜绿假单胞菌,14个Klebsiella肺炎菌株),针对74个抗生素和两种抗生素组合。将细菌(约5个log(10)cfu / ml)在35℃下与抗生素孵育;在6小时和24小时测量ATP生物发光;将测量值与24小时的可行计数进行比较。接收器操作特征(ROC)曲线用于确定用于区分抑制和非抑制组合的最佳发光阈值(T-RLU)。使用Delong方法进行比较6-H和24-H ROC曲线的区域。使用18个额外CR-GNB进行既定阈值的预期验证。当集体分析所有物种时,6-H ATP生物发光测定的T-RLU的预测精度为77.5%。单独分析每种物种时,预测精度为73.7%至82.7%。在比较6-H和24-H ROC曲线下的区域时,6-H测定显着优于24-H测定(P <0.01)。在6-H ATP测定的前瞻性验证(预测精度,79.8%; 95%置信区间[CI],77.6至81.9%),确认测定的外部有效性,预测精度保持高。我们的研究结果表明,我们的6-H ATP生物发光测定可以在及时选择对CR-GNB的抗生素组合的预期选择的指导,并且可用于治疗Cr-GNB感染。

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