The auxiliary diagnostic value of Mycobacterium tuberculosis-specific cytokines combined with common laboratory indicators in early extrapulmonary tuberculosis

doi:10.19982/j.issn.1000-6621.20250176

Abstract

Abstract:

Objective: To evaluate the auxiliary diagnostic value of detecting Mycobacterium tuberculosis (MTB)-specific cytokines (interferon-γ (IFN-γ) and interleukin-2 (IL-2)) combined with common laboratory indicators in extrapulmonary tuberculosis. Methods: A prospective study was conducted. A total of 158 inpatients with extrapulmonary tuberculosis who were treated at Xi'an Chest Hospital from August 2023 to September 2024 were consecutively included as the extrapulmonary tuberculosis group; 107 inpatients with non-tuberculous extrapulmonary diseases treated at Xi'an Chest Hospital during the same period were selected as the control group. All subjects underwent MTB-specific dual-factor detection, mycobacterium culture, real-time fluorescent quantitative PCR (qRT-PCR), real-time fluorescent RNA isothermal detection (SAT-TB), MTB nucleic acid detection (isothermal amplification DNA), GeneXpert MTB/RIF detection (referred to as “Xpert”), and acid-fast bacilli smear microscopy. Additionally, procalcitonin (PCT), C-reactive protein (CRP), systemic immune-inflammation index (SII), neutrophil/lymphocyte ratio (NLR), and platelet/lymphocyte ratio (PLR) were tested. The auxiliary diagnostic value of MTB-specific dual factors alone and in combination with common laboratory indicators (PCT, CRP, SII, NLR, and PLR) for extrapulmonary tuberculosis was evaluated. Results: With clinical diagnosis as the reference standard, the sensitivity, specificity, positive predictive value, and negative predictive value of MTB-specific dual-factor detection were 78.48% (124/158), 71.96% (77/107), 80.52% (124/154), and 69.37% (77/111), respectively. The sensitivity was higher than that of the other 6 methods. Both the Youden index (0.504) and the consistency test Kappa value (0.501) were higher than those of the other 6 detection methods. In the methodological comparison, the positive detection rate of the serological group (MTB-specific dual factors) was 78.48% (124/158), which was significantly higher than that of the molecular biology group (qRT-PCR, SAT-TB, Xpert, and isothermal amplification DNA) and the bacteriology group (mycobacterium culture and acid-fast bacilli smear microscopy), with positive rates of 39.87% (63/158) and 26.58% (42/158), respectively. The differences were statistically significant (χ²=48.743 and 85.333, both P<0.001). In the comparison of laboratory indicators, the levels of PCT, CRP, SII, and PLR in the extrapulmonary tuberculosis group were 0.00 (0.00, 0.09) pg/ml, 24.08 (3.56, 71.69) mg/L, 976.76 (571.92, 2159.82), and 190.66 (135.02, 267.31), respectively; in the control group, the levels were 0.06 (0.00, 0.18)pg/ml, 10.05 (0.39, 63.44) mg/L, 784.56 (401.14, 1409.55), and 151.54 (108.23, 218.47), respectively. The differences between the two groups were statistically significant (U=-2.592, -2.024, -2.484, and -3.285; P=0.010, 0.043, 0.013, and 0.001, respectively). The results of the receiver operating characteristic curve showed that the area under the curve for the detection of MTB-specific dual factors combined with common laboratory indicators (PCT, CRP, SII, NLR, and PLR) was 0.801 (95%CI: 0.720-0.881). Conclusion: MTB-specific dual-factor detection has good sensitivity in the diagnosis of extrapulmonary tuberculosis, and combining it with common laboratory indicators (PCT, CRP, SII, NLR, and PLR) can improve the diagnostic accuracy of extrapulmonary tuberculosis.

Key words: Mycobacterium tuberculosis, Interferons, Interleukin-2, Diagnosis, differential, Extrapulmonary tuberculosis

CLC Number:

Zhang Xin, Zheng Huiqiang, Liu Yuan, Wu Xia, Wang Haidong, Tan Xiaowen. The auxiliary diagnostic value of Mycobacterium tuberculosis-specific cytokines combined with common laboratory indicators in early extrapulmonary tuberculosis[J]. Chinese Journal of Antituberculosis, 2025, 47(10): 1342-1349. doi: 10.19982/j.issn.1000-6621.20250176

Figures/Tables 5

特征	肺外结核组(158例)	对照组(107例)	统计检验值	P值
性别[例(构成比,%)]			χ²=1.989	0.158
男性	76(48.10)	52(48.60)
女性	82(51.90)	55(51.40)
年龄(岁, $x ˉ$ ±s)	51.39±2.06	49.96±2.38	t=0.412	0.522
合并症[例(患病率,%)]
糖尿病	21(13.29)	12(11.21)	χ²=0.252	0.616
高血压	32(20.25)	30(28.04)	χ²=2.157	0.142
其他免疫系统疾病	1(0.63)	1(0.93)	χ²=0.078	0.781

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组别	T-N(pg/ml)	P-N(pg/ml)	判断条件	判定结果
分组1			IFN-γ和(或)IL-2满足条件	阳性
IFN-γ	≥7	任何值
IL-2	≥20	任何值
分组2			两个因子同时满足条件	阴性
IFN-γ	<7	≥35
IL-2	<20	≥130
分组3			当不满足分组1时,其中一个因子满足条件	不确定
IFN-γ	<7	<35
IL-2	<20	<130

检测方法	肺外结核组(例)	对照组 (例)	敏感度 (%)	特异度 (%)	阳性预测值(%)	阴性预测值(%)	约登指数	Kappa值
MTB特异性双因子检测			78.48	71.96	80.52	69.37	0.504	0.501
阳性	124	30
阴性	34	77
荧光实时定量PCR检测			32.27	95.32	91.07	48.80	0.276	0.239
阳性	51	5
阴性	107	102
结核分枝杆菌RNA恒温扩增实时荧光检测			23.42	96.26	90.24	45.98	0.197	0.167
阳性	37	4
阴性	121	103
抗酸杆菌涂片镜检			5.70	99.07	90.00	41.57	0.048	0.039
阳性	9	1
阴性	149	106
分枝杆菌培养			23.41	94.39	86.05	45.50	0.178	0.152
阳性	37	6
阴性	121	101
GeneXpert MTB/RIF检测			23.41	94.39	86.05	45.50	0.178	0.152
阳性	37	6
阴性	121	101
恒温扩增DNA检测			17.09	96.26	87.10	44.02	0.134	0.112
阳性	27	4
阴性	131	103

指标	肺外结核组(158例)	对照组(107例)	U值	P值
PCT(pg/ml)	0.00(0.00,0.09)	0.06(0.00,0.18)	-2.592	0.010
CRP(mg/L)	24.08(3.56,71.69)	10.05(0.39,63.44)	-2.024	0.043
NLR	3.54(2.22,6.40)	3.60(2.55,5.88)	-0.775	0.438
SII	976.76(571.92,2159.82)	784.56(401.14,1409.55)	-2.484	0.013
PLR	190.66(135.02,267.31)	151.54(108.23,218.47)	-3.285	0.001