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Q 热诊断用重组蛋白分析。

Analysis of recombinant proteins for Q fever diagnostics.

机构信息

Rickettsial Zoonoses Branch, Centers for Disease Control and Prevention, Atlanta, GA, USA.

出版信息

Sci Rep. 2020 Dec 1;10(1):20934. doi: 10.1038/s41598-020-77343-0.

Abstract

Serology is essential for Q fever diagnostics, a disease caused by the bacterial pathogen Coxiella burnetii. The gold standard test is an immunofluorescence assay utilizing whole cell antigens, which are both dangerous and laborious to produce. Complexities of the antigen coupled with the subjective nature of the assay lead to decreased uniformity of test results and underscore the need for improved methodologies. Thirty-three C. burnetii proteins, previously identified as immunoreactive, were screened for reactivity to naturally infected goat serum. Based on reactivity, 10 proteins were analyzed in a secondary screen against human serum from healthy donors. Assay sensitivity and specificity ranged from 21 to 71% and 90 to 100%, respectively. Three promising antigens were identified based on receiver operating characteristic curve analysis (CBU_1718, CBU_0307, and CBU_1398). Five multiplex assays failed to outperform the individual proteins, with sensitivities and specificities ranging from 29 to 57% and 90 to 100%, respectively. Truncating the top antigen, CBU_1718, had no effect on specificity (90%); yet sensitivity decreased dramatically (71% to 21%). Through this study, we have expanded the subset of C. burnetii immunoreactive proteins validated by enzyme-linked immunosorbent assay and demonstrate the effect of novel antigen combinations and protein truncations on assay performance.

摘要

血清学对于 Q 热诊断至关重要,Q 热是由细菌病原体贝氏柯克斯体引起的疾病。金标准测试是一种利用全细胞抗原的免疫荧光分析,这种抗原既危险又难以生产。抗原的复杂性以及检测的主观性导致检测结果的一致性降低,这突显了需要改进方法。已经筛选出 33 种先前被鉴定为免疫反应性的贝氏柯克斯体蛋白,以检测其对自然感染山羊血清的反应性。根据反应性,在第二次筛选中针对来自健康供体的人血清分析了 10 种蛋白质。该测定的灵敏度和特异性分别为 21%至 71%和 90%至 100%。根据受试者工作特征曲线分析(CBU_1718、CBU_0307 和 CBU_1398),确定了三种有前途的抗原。五种多重测定均未优于单个蛋白质,其灵敏度和特异性分别为 29%至 57%和 90%至 100%。截断顶部抗原 CBU_1718 对特异性没有影响(90%);然而,灵敏度显著下降(71%降至 21%)。通过这项研究,我们扩展了酶联免疫吸附测定验证的贝氏柯克斯体免疫反应性蛋白子集,并证明了新型抗原组合和蛋白质截断对检测性能的影响。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/952e/7708433/3980c4b8fa1e/41598_2020_77343_Fig1_HTML.jpg

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