Petruccioli Elisa, Chiacchio Teresa, Pepponi Ilaria, Vanini Valentina, Urso Rocco, Cuzzi Gilda, Barcellini Lucia, Palmieri Fabrizio, Cirillo Daniela M, Ippolito Giuseppe, Goletti Delia
Translational Research Unit, Department of Epidemiology and Preclinical Research, National Institute for Infectious Diseases L Spallanzani (INMI), Rome, Italy.
Emerging Bacterial Pathogens Unit, Division of Immunology and Infectious Diseases IRCCS, San Raffaele Scientific Institute, Milan, Italy.
Int J Mycobacteriol. 2016 Dec;5 Suppl 1:S25-S26. doi: 10.1016/j.ijmyco.2016.09.063. Epub 2016 Nov 11.
OBJECTIVE/BACKGROUND: QuantiFERON-TB Gold In-Tube (QFT-GIT, Qiagen, Hilden, Germany) is an interferon-γ (IFN-γ) release assay designed to detect latent tuberculosis infection (LTBI). Although QFT-GIT has several advantages (mainly that it is not affected by the Bacille Calmette-Guérin vaccination), it has a poor sensitivity in immune-compromised individuals as it involves an immune response-based detection. Recently, QuantiFERON-TB Gold Plus (QFT-Plus) assay has been proposed as a new generation of QFT-GIT. QFT-Plus includes two tubes, TB1 and TB2 with Mycobacterium tuberculosis antigens to elicit a specific immune response. TB1 contains peptides derived from the antigens 6kDa early secretory antigenic target (ESAT-6) and 10kDa culture filtrate protein (CFP-10) (TB-7.7, present in QFT-GIT, has been removed), and it is designed to induce a specific CD4 T-cell response. TB2 contains newly designed peptides stimulating IFN-γ production by both CD4 and CD8 T cells. The additional peptides for eliciting CD8 T-cell responses have been included to increase the sensitivity of the test for LTBI detection. The aim of the study was to evaluate specific CD4 and CD8 T-cell responses to the M. tuberculosis antigens contained within the QFT-Plus test by flow cytometry in individuals with active TB and LTBI.
We enrolled 23 individuals with active TB and 30 individuals with LTBI. QFT-Plus assay and intracellular staining were performed. One million of peripheral blood mononuclear cells in 1ml of complete medium (RPMI 1640) were dispensed in QFT-Plus tubes. Following 16-24h stimulation, antigen-specific T cells were characterized by flow cytometry evaluating CD4, CD8, CD3 markers, and IFN-γ production. For statistical analysis, nonparametric tests were performed.
We found that CD4 T-cell responses were induced by both TB1 and TB2. Differently, the CD8 T-cell response was mainly induced by TB2 and was significantly higher than that induced by TB1 (p=0.01). The frequency of Mtb specific T-cells observed in individuals with active TB was significantly higher than in those with LTBI (p=0.04). Finally, TB2-specific CD8 T-cell responses in individuals with active TB were associated with high radiological severity of lung lesions and microbiological diagnosis (based on M. tuberculosis isolation in sputum culture).
This is the first characterization of CD4 and CD8 T-cell responses to QFT-Plus TB1 and TB2 tubes in individuals with active TB and LTBI enrolled in a low TB-endemic country such as Italy. We demonstrated that the increased sensitivity is a consequence of the ability of TB2 to induce a CD8 T-cell response which is mainly associated with active TB. This assay has the potential to be very useful in conditions of immune depression due to CD4 T-cell impairments.
目的/背景:全血γ干扰素释放试验(QFT-GIT,德国希尔德市凯杰公司产品)是一种用于检测潜伏性结核感染(LTBI)的γ干扰素(IFN-γ)释放检测方法。尽管QFT-GIT有诸多优点(主要是不受卡介苗接种的影响),但由于其基于免疫反应进行检测,在免疫功能低下个体中的敏感性较差。最近,全血γ干扰素释放试验升级版(QFT-Plus)被提出作为新一代的QFT-GIT。QFT-Plus包括两支试管,TB1和TB2,其中含有结核分枝杆菌抗原以引发特异性免疫反应。TB1含有源自6 kDa早期分泌性抗原靶标(ESAT-6)和10 kDa培养滤液蛋白(CFP-10)的肽段(QFT-GIT中含有的TB-7.7已被去除),旨在诱导特异性CD4 T细胞反应。TB2含有新设计的肽段,可刺激CD4和CD8 T细胞产生IFN-γ。包含用于引发CD8 T细胞反应的额外肽段是为了提高LTBI检测试验的敏感性。本研究的目的是通过流式细胞术评估活动性结核病患者和LTBI患者对QFT-Plus检测中所含结核分枝杆菌抗原的特异性CD4和CD8 T细胞反应。
我们招募了23例活动性结核病患者和30例LTBI患者。进行了QFT-Plus检测和细胞内染色。将100万个外周血单个核细胞加入1ml完全培养基(RPMI 1640)中,分装到QFT-Plus试管中。在16 - 24小时刺激后,通过流式细胞术评估CD4、CD8、CD3标志物和IFN-γ产生情况,以鉴定抗原特异性T细胞。进行统计分析时采用非参数检验。
我们发现TB1和TB2均可诱导CD4 T细胞反应。不同的是,CD8 T细胞反应主要由TB2诱导且显著高于TB1诱导的反应(p = 0.01)。活动性结核病患者中观察到的结核分枝杆菌特异性T细胞频率显著高于LTBI患者(p = 0.04)。最后,活动性结核病患者中TB2特异性CD8 T细胞反应与肺部病变的高放射学严重程度和微生物学诊断(基于痰培养中结核分枝杆菌的分离)相关。
这是在意大利这样一个结核病低流行国家招募的活动性结核病患者和LTBI患者中,首次对QFT-Plus的TB1和TB2试管的CD4和CD8 T细胞反应进行的特征描述。我们证明,敏感性的提高是由于TB2诱导CD8 T细胞反应的能力,而这种反应主要与活动性结核病相关。该检测方法在因CD4 T细胞受损导致免疫抑制的情况下可能非常有用。
