Analysis of the results of etiology and drug resistance in different surgical specimens of tuberculous empyema by two techniques

doi:10.3969/j.issn.1000-6621.2021.01.011

Abstract

Abstract:

Objective BACTEC MGIT 960 (MGIT 960) and fluorescence PCR melting curve method (PCR melting curve method) were used to detect the etiology and drug resistance of different surgical specimens of tuberculous empyema, and comparative study was conducted. Methods From January 2019 to June 2020, 150 patients with tuberculous empyema were enrolled (MTB MGIT 960 was positive and MPB64 monoclonal antibody was MTB strain of thoracic puncture before surgery, or histopathological examination showed typical tuberculous granulomatous inflammation with caseous necrosis). MGIT 960 liquid culture, phenotypic drug sensitivity test (drug sensitivity test) and PCR melting curve method were used to detect nucleic acid and drug resistance genes of different surgical specimens (150 lesions and 150 pus). Positive rate of etiological diagnosis between two kinds of techniques in different surgical specimens, and drug resistance results of 40 pathogenic positive cases (copies) detected by two kinds of techniques at the same time were comparatively analyzed. Results In 300 surgical specimens (pus and tissue), the overall positive rate of MTB detection by PCR fusion curve method (44.0%, 132/300) was significantly higher than that of MGIT 960 (18.0%, 54/300) (χ²=47.405, P=0.000). The positive rate of PCR melting curve nucleic acid detection in tissue samples (50.0% (75/150)) was significantly higher than that in pus samples (38.0%, (57/150)) (χ ²=4.383, P=0.048); while the positive rate of MGIT 960 in tissue samples (12.7% (19/150)) was significantly lower than that in pus samples (23.3% (35/150)) (χ ²=5.781, P=0.024). Further analysis of the positive rate of MGIT 960, fluorescent PCR and two combined techniques in etiological diagnosis of 150 patients was made (if one of the methods is positive, the patient woulde be judged pathogenic positive). The results showed that the positive rate of the former (30.7% (46/150)) was significantly lower than those of the latter two (66.7% (100/150) and 70.7% (106/150), respectively) (χ ²=38.908, 48.009; both P=0.000), no significant difference was found between the latter two (χ ²=0.558, P=0.455). The results of drug resistance of 40 pathogenic positive cases (copies) detected by two methods at the same time showed that the detection rates of isoniazid, rifampicin, ethambutol, streptomycin and levofloxacin by MGIT 960 and PCR melting curve method were 20.0% (8/40) and 17.5% (7/40), 17.5% (7/40) and 15.0% (6/40), 17.5% (7/40) and 17.5% (7/40), 17.5% (7/40) and 22.5% (9/40), 5.0% (2/40) and 7.5% (3/40), respectively, and the differences were not significant (χ ²=0.082, 0.092, 0.000, 0.313, 0.213, all P>0.05). Conclusion In tuberculous empyema patients, the overall positive rate of MTB detected by PCR melting curve method was significantly higher than that of MGIT 960 culture, and the positive rate of tissue samples was higher than that of pus samples; the detection rate of drug resistance was similar to that of MGIT 960 phenotype drug sensitivity test, which could quickly detect the etiology and drug resistance.

Key words: Empyema,tuberculous, Specimen Handling, Polymerase chain reaction, Molecular diagnostic techniques, Tuberculosis,multi-drug resistant, Microbial sensitivity tests, Comparative study

LI Qian, WANG Lin-bao, LUO Pei-jia, WEI Lin, LIU Yu-gang, REN Lei-peng, DING Chao. Analysis of the results of etiology and drug resistance in different surgical specimens of tuberculous empyema by two techniques[J]. Chinese Journal of Antituberculosis, 2021, 43(1): 52-57. doi: 10.3969/j.issn.1000-6621.2021.01.011

Figures/Tables 3

References 23

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手术标本	PCR熔解曲线法检测Ct值 [份数(构成比,%)]			χ²值	P值	MGIT 960培养		χ²值	P值
	PCR熔解曲线法检测Ct值 [份数(构成比,%)]					阳性[份数 (构成比,%)]	阴性[份数 (构成比,%)]
	<30	30~	≥40			阳性[份数 (构成比,%)]	阴性[份数 (构成比,%)]
脓液(150份)	57(38.0)	16(10.7)	77(51.3)	4.383	0.048	35(23.3)	115(76.7)	5.781	0.024
组织(150份)	75(50.0)	12(8.0)	63(42.0)			19(12.7)	131(87.3)

检测结果	MGIT 960培养	PCR熔解曲线法	联合检测	χ²值^a	P值	χ²值^b	P值	χ²值^c	P值
病原学阳性	46(30.7)	100(66.7)	106(70.7)	38.908	0.000	48.009	0.000	0.558	0.455
病原学阴性	104(69.3)	50(33.3)	44(29.3)

检测技术	异烟肼	利福平	乙胺丁醇	链霉素	左氧氟沙星
MGIT 960表型药敏试验(40份)	8(20.0)	7(17.5)	7(17.5)	7(17.5)	2(5.0)
PCR熔解曲线法耐药基因检测(40份)	7(17.5)	6(15.0)	7(17.5)	9(22.5)	3(7.5)
χ²值	0.082	0.092	0.000	0.313	0.213
P值	0.775	0.762	1.000	0.576	0.644