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Cell-Mediated Immune Response to Tuberculosis Antigens: Comparison of Skin Testing and Measurement of In Vitro Gamma Interferon Production in Whole-Blood Culture

机译:细胞介导的对肺结核抗原的免疫反应:皮肤测试和全血培养中体外γ干扰素生产的比较

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摘要

Although delayed-type hypersensitivity skin testing with tuberculin purified protein derivative (PPD) is the standard for tuberculosis screening, its variability suggests the need for a more sensitive, noninvasive test. An in vitro whole-blood assay has been proposed as an alternative. Using health care worker volunteers, we confirmed the correlation between PPD skin test (PPD-ST) results (positive, induration of >15 mm) and a standardized gamma interferon (IFN-γ) assay, QuantiFERON-TB (Q-IFN), manufactured by CSL Biosciences in Australia, and we evaluated Mycobacterium tuberculosis culture subfractions as potential substitutes for PPD. Twenty healthy volunteers with positive PPD-ST results and 20 PPD-ST-negative controls were enrolled. Whole blood was cultured with human PPD antigens (HuPPD), Mycobacterium avium complex (MAC) PPD, phytohemagglutinin (PHA), and four M. tuberculosis culture subfractions: low-molecular-weight culture, filtrate, culture filtrate without lipoarabinomannan, soluble cell wall proteins, and cytosolic proteins, all developed from M. tuberculosis strain H37RV. Secretion of IFN-γ (expressed as international units per milliliter) was measured by an enzyme immunoassay. The PPD or subculture fraction response as a percentage of the PHA response was used to determine positivity. Sixteen of 20 PPD-ST-positive individuals were classified as M. tuberculosis positive by Q-IFN, and 1 was classified as MAC positive. Sixteen of 20 PPD-ST-negative individuals were M. tuberculosis negative by Q-IFN, 2 were MAC positive, and 2 were M. tuberculosis positive. The tuberculosis culture subfractions stimulated IFN-γ production in PPD-ST-positive volunteers, and significant differences could be seen between the two PPD-ST groups with all subfractions except soluble cell wall protein; however, the response was variable and no better than the Q-IFN PPD. The agreement between the Q-IFN test and the PPD-ST was good (Cohen's kappa = 0.73). The Q-IFN assay can be a useful tool in further studies of immune responses to M. tuberculosis antigens.
机译:尽管结核菌素纯化蛋白衍生物(PPD)的迟发型超敏性皮肤测试是结核病筛查的标准,但其可变性表明需要进行更敏感的,非侵入性的测试。已经提出了体外全血测定法作为替代方案。我们使用医护人员自愿者,证实了PPD皮肤测试(PPD-ST)结果(阳性,硬结> 15毫米)与标准伽玛干扰素(IFN-γ)测定,QuantiFERON-TB(Q-IFN),由澳大利亚的CSL Biosciences生产,我们评估了结核分枝杆菌培养亚组分作为PPD的潜在替代品。招募了20名PPD-ST结果阳性和20名PPD-ST阴性对照的健康志愿者。用人PPD抗原(HuPPD),鸟分枝杆菌复合物(MAC)PPD,植物血凝素(PHA)和四个结核分枝杆菌培养亚种培养全血:低分子量培养物,滤液,无脂阿拉伯糖甘露聚糖的培养物滤液,可溶性细胞壁蛋白和胞浆蛋白均来自结核分枝杆菌菌株H37RV。通过酶免疫测定法测量IFN-γ的分泌(以国际单位每毫升表示)。 PPD或继代培养分数反应占PHA反应的百分比用于确定阳性。 Q-IFN将20个PPD-ST阳性个体中的16个分类为结核分枝杆菌阳性,将1个分类为MAC阳性。 20例PPD-ST阴性患者中有16例通过Q-IFN阴性,结核分枝杆菌,MAC阳性2例,结核分枝杆菌阳性2例。结核培养亚组刺激PPD-ST阳性志愿者中的IFN-γ产生,两个PPD-ST组之间除了可溶细胞壁蛋白外,所有亚组均存在显着差异。然而,反应是可变的,并不比Q-IFN PPD好。 Q-IFN测试与PPD-ST之间的一致性很好(Cohenκ= 0.73)。 Q-IFN测定法可能是进一步研究针对结核分枝杆菌抗原的免疫反应的有用工具。

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