Rattani Salima, Farooqi Joveria, Jabeen Ghazala, Chandio Saeeda, Kash Qaiser, Khan Aijaz, Jabeen Kauser
Department of Pathology & Laboratory Medicine, The Aga Khan University, Stadium Road, Karachi, 74800, Pakistan.
BMC Pulm Med. 2020 Oct 29;20(1):284. doi: 10.1186/s12890-020-01311-7.
Diagnosis of lower respiratory tract infections (LRTI) depends on the presence of clinical, radiological and microbiological findings. Endotracheal suction aspirate (ETSA) is the commonest respiratory sample sent for culture from intubated patients. Very few studies have compared quantitative and semi-quantitative processing of ETSA cultures for LRTI diagnosis. We determined the diagnostic accuracy of quantitative and semi-quantitative ETSA culture for LRTI diagnosis, agreement between the quantitative and semi quantitative culture techniques and the yield of respiratory pathogens with both methods.
This was a cross-sectional study conducted at the Aga Khan University clinical laboratory, Karachi, Pakistan. One hundred and seventy-eight ETSA samples sent for routine bacteriological cultures were processed quantitatively as part of regular specimen processing method and semi-quantitatively. Sensitivity, specificity, positive predictive value (PPV), negative predictive value (NPV) and diagnostic accuracy was calculated for both methods using clinical diagnosis of pneumonia as reference standard. Agreement between the quantitative and semi quantitative methods was assessed via the kappa statistic test. Pathogen yield between the two methods was compared using Pearson's chi-square test.
The quantitative and semi-quantitative methods yielded pathogens in 81 (45.5%) and 85 (47.8%) cases respectively. There was complete concordance of both techniques in 155 (87.1%) ETSA samples. No growth was observed in 45 (25.3%) ETSA specimens with quantitative culture and 37 (20.8%) cases by semi-quantitative culture. The diagnostic accuracy of both techniques were comparable; 64.6% for quantitative and 64.0% for semi-quantitative culture. The kappa agreement was found to be 0.84 (95% CI, 0.77-0.91) representing almost perfect agreement between the two methods. Although semi-quantitative cultures yielded more pathogens (47.8%) as compared to quantitative ETSA cultures (45.5%), the difference was only 2.3%. However, this difference achieved statistical (chi-square p-value < 0.001) favoring semi-quantitative culture methods over quantitative culture techniques for processing ETSA.
In conclusion, there is a strong agreement between the performances of both methods of processing ETSA cultures in terms of accuracy of LRTI diagnosis. Semi-quantitative cultures of ETSA yielded more pathogens as compared to quantitative cultures. Although both techniques were comparable, we recommend processing of ETSA using semi-quantitative technique due to its ease and reduced processing time.
下呼吸道感染(LRTI)的诊断取决于临床、影像学和微生物学检查结果。气管内吸引物(ETSA)是插管患者送检培养的最常见呼吸道样本。很少有研究比较ETSA培养物的定量和半定量处理用于LRTI诊断的情况。我们确定了ETSA培养物的定量和半定量方法用于LRTI诊断的诊断准确性、定量和半定量培养技术之间的一致性以及两种方法呼吸道病原体的检出率。
这是一项在巴基斯坦卡拉奇阿迦汗大学临床实验室进行的横断面研究。178份送检常规细菌培养的ETSA样本作为常规标本处理方法的一部分进行了定量处理和半定量处理。以肺炎的临床诊断为参考标准,计算两种方法的敏感性、特异性、阳性预测值(PPV)、阴性预测值(NPV)和诊断准确性。通过kappa统计检验评估定量和半定量方法之间的一致性。使用Pearson卡方检验比较两种方法之间的病原体检出率。
定量和半定量方法分别在81例(45.5%)和85例(47.8%)病例中检出病原体。155份(87.1%)ETSA样本中两种技术完全一致。定量培养时45份(25.3%)ETSA标本未生长,半定量培养时37份(20.8%)病例未生长。两种技术的诊断准确性相当;定量培养为64.6%,半定量培养为64.0%。kappa一致性为0.84(95%CI,0.77 - 0.91),表明两种方法之间几乎完全一致。尽管半定量培养比定量ETSA培养检出更多病原体(47.8%对45.5%),但差异仅为2.3%。然而,这种差异具有统计学意义(卡方p值<0.001),在处理ETSA方面,半定量培养方法优于定量培养技术。
总之,在LRTI诊断准确性方面,ETSA培养物的两种处理方法的性能之间有很强的一致性。与定量培养相比,ETSA的半定量培养检出更多病原体。虽然两种技术相当,但由于其简便性和减少的处理时间,我们建议使用半定量技术处理ETSA。
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