首页> 外文期刊>Journal of Clinical Microbiology >Identification of Mycobacterium tuberculosis and M. avium complex directly from smear-positive sputum specimens and BACTEC 12B cultures by high-performance liquid chromatography with fluorescence detection and computer-driven pattern recognition models.
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Identification of Mycobacterium tuberculosis and M. avium complex directly from smear-positive sputum specimens and BACTEC 12B cultures by high-performance liquid chromatography with fluorescence detection and computer-driven pattern recognition models.

机译:通过高效液相色谱,荧光检测和计算机驱动模式识别模型,直接从涂片阳性痰标本和BACTEC 12B培养物中鉴定结核分枝杆菌和鸟分枝杆菌。

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A high-performance liquid chromatography method that utilized fluorescence detection (HPLC-FL) of mycolic acid 6,7-dimethoxycoumarin esters was developed to identify Mycobacterium tuberculosis (MTB) and M. avium complex (MAC) directly from fluorochrome stain smear-positive sputum specimens and young BACTEC 12B cultures. HPLC-FL chromatograms from a training set that included 202 smear-positive clinical sputum specimens and 343 mycobacterial cultures were used to construct a calibrated peak-naming table and computer-based pattern recognition models for MTB and MAC. Pattern recognition model performance was measured with an evaluation set of samples that included 251 smear-positive clinical sputum specimens and 167 BACTEC 12B cultures. Evaluation sputum specimens were culture positive for MTB (n = 132) and MAC (n = 48). With evaluation sputa, the MTB and MAC models were 56.8 and 33.3% sensitive, respectively. Evaluation set BACTEC 12B cultures were culture positive for MTB (n = 97) and MAC (n = 53). The sensitivities of the MTB and MAC models for identification of BACTEC 12B cultures were 99.0 and 94.3%, respectively. The specificity of both models was 100% for both types of evaluation samples. The average times from BACTEC 12B inoculation to cell harvest were 10.2 and 7.4 days for MTB and MAC, respectively. HPLC-FL can identify MTB and MAC in 1 day from many smear-positive sputa. Rapid and sensitive identification of MTB and MAC from young BACTEC 12B cultures was achieved.
机译:建立了一种高效液相色谱方法,该方法利用了霉菌酸6,7-二甲氧基香豆素酯的荧光检测(HPLC-FL),可直接从荧光染料涂片阳性痰中鉴定结核分枝杆菌(MTB)和鸟分枝杆菌复合体(MAC)。标本和年轻的BACTEC 12B培养物。来自包括202个涂片阳性临床痰标本和343个分枝杆菌培养物的训练集的HPLC-FL色谱图用于构建MTB和MAC的校准峰命名表和基于计算机的模式识别模型。模式评估模型的性能是通过评估样本集来衡量的,其中包括251个涂片阳性临床痰标本和167个BACTEC 12B培养物。评估痰标本的MTB(n = 132)和MAC(n = 48)培养阳性。通过评估,MTB和MAC模型的敏感性分别为56.8和33.3%。评估集BACTEC 12B培养物的MTB(n = 97)和MAC(n = 53)培养阳性。 MTB和MAC模型对BACTEC 12B培养物鉴定的敏感性分别为99.0%和94.3%。两种类型的评估样品的两种模型的特异性均为100%。从BACTEC 12B接种到细胞收获的平均时间,MTB和MAC分别为10.2天和7.4天。 HPLC-FL可以在1天之内从许多涂片阳性痰中鉴定出MTB和MAC。从年轻的BACTEC 12B培养物中快速,灵敏地鉴定MTB和MAC。

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