结核病人体内的 PPE59 抗体以及与其他快速生物标记物一起检测时用于诊断的可能性。

Ana Carla de Paulo Mulinari,Isabela Gama Sardella,Vania Maria C da Silva,Alberto Matteelli,Anna Cristina C Carvalho,Maria Helena Féres Saad
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Additional studies are needed to better evaluate this protein in immune response to tuberculosis.\r\n\r\nOBJECTIVES\r\nTo evaluate the response of antibodies to PPE59 in TB individuals, its combination with IgG response to other, previously tested mycobacterial antigens (Ag) and with sputum smear microbiology (SM) results.\r\n\r\nMETHODS\r\nWe have cloned and expressed the rv3429 gene that encodes PPE59, then IgG, IgM, and IgA against PPE59 antigens measured by enzyme-linked immunosorbent assay (ELISA) in 212 sera samples obtained from the following subject cohorts: TB residents from Italy (79) and in Brazil (52); and an all-Brazilian cohort of 55 patients with other respiratory disorders; 10 patients infected with non-tuberculous mycobacteria, and 16 asymptomatic subjects. 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摘要

背景PPE59在卡介苗(BCG)菌株中并不存在,但似乎能诱导结核病(TB)患者产生体液免疫反应。目的评估肺结核患者对 PPE59 的抗体反应、其与其他先前检测过的分枝杆菌抗原(Ag)的 IgG 反应以及与痰涂片微生物学(SM)结果的结合情况。我们克隆并表达了编码 PPE59 的 rv3429 基因,然后通过酶联免疫吸附试验 (ELISA) 测定了从以下受试者群体中获得的 212 份血清样本中针对 PPE59 抗原的 IgG、IgM 和 IgA:这些血清样本分别来自意大利(79 人)和巴西(52 人)的肺结核居民、55 名患有其他呼吸系统疾病的巴西患者、10 名非结核分枝杆菌感染者和 16 名无症状者。根据之前的一项研究(17)结果,对巴西受试者的血清样本进行了针对分枝杆菌抗原 ESAT-6、16kDa、MT10.3、MPT-64 和 38kDa 的 ELISA IgG 检测,并结合 PPE59 和 SM 检测结果进行了分析。结合 PPE59 IgA/16kDa IgG 结果可将灵敏度提高到 71%,结合 SM 结果时灵敏度更高(86.5%,p = 0.001),特异性为 88.9%。IgA 阳性与肺结核可能性高的肺图像改变有关(p < 0.05)。然而,结合 PPE59 IgA/16kDa IgG/SM 结果所获得的灵敏度较高,这在以前是闻所未闻的,尽管还不完善,但表明这可能是低资源地区快速检测结核病的另一种潜在工具。
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PPE59 antibodies in tuberculous patients and potential use for diagnosis when assayed with other rapid biomarkers.
BACKGROUND PPE 59, which is absent from bacillus Calmette Guérin (BCG) strains, seems to induce a humoral immune response in patients with tuberculosis (TB). Additional studies are needed to better evaluate this protein in immune response to tuberculosis. OBJECTIVES To evaluate the response of antibodies to PPE59 in TB individuals, its combination with IgG response to other, previously tested mycobacterial antigens (Ag) and with sputum smear microbiology (SM) results. METHODS We have cloned and expressed the rv3429 gene that encodes PPE59, then IgG, IgM, and IgA against PPE59 antigens measured by enzyme-linked immunosorbent assay (ELISA) in 212 sera samples obtained from the following subject cohorts: TB residents from Italy (79) and in Brazil (52); and an all-Brazilian cohort of 55 patients with other respiratory disorders; 10 patients infected with non-tuberculous mycobacteria, and 16 asymptomatic subjects. Drawing on results from a previous study(17) of serum samples from Brazilian subjects tested for IgG by ELISA against mycobacterial antigens ESAT-6, 16kDa, MT10.3, MPT-64 and 38kDa, the results were analysed in combination with those of the PPE59 and SM tests. FINDINGS Keeping the specificity rate at 97%, the overall PPE59 IgA sensitivity was 42.7%, while IgG and IgM showed lower performance (p < 0.0001). Combining PPE59 IgA/16kDa IgG results increased sensitivity to 71%, and even higher rates when the results were combined with SM results (86.5%, p = 0.001), at 88.9% specificity. Positive IgA was associated with pulmonary image alterations of high TB probability (p < 0.05). MAIN CONCLUSIONS Tests with TB patients found a moderate frequency of positivity for PPE59 IgA. However, the higher level of sensitivity attained in combination with PPE59 IgA/16kDa IgG/SM results unheard of before, although imperfect, suggests that this may be a potential additional tool for rapid detection of TB in low-resource areas.
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