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多重评估 SARS-CoV-2 抗体可提高检测敏感性,并与中和抗体相关。

Multiplex assessment of SARS-CoV-2 antibodies improves assay sensitivity and correlation with neutralizing antibodies.

机构信息

University of Pittsburgh Medical Center, Department of Pathology, Pittsburgh, PA, USA.

University of Pittsburgh, School of Medicine, Department of Pediatrics and Center for Vaccine Research, Pittsburgh, PA, USA.

出版信息

Clin Biochem. 2021 Nov;97:54-61. doi: 10.1016/j.clinbiochem.2021.08.006. Epub 2021 Aug 26.

Abstract

OBJECTIVES

Detection of antibodies to multiple SARS-CoV-2 antigens in a single assay could increase diagnostic accuracy, differentiate vaccination from natural disease, and aid in retrospective exposure determination. Correlation of binding antibody assessment in clinical assays with neutralizing antibodies is needed to better understand the humoral response to SARS-CoV-2 infection and establish of correlates of protection.

METHODS

A cohort of 752 samples was used to assess specificity, sensitivity, and comparison to 6 other Conformitè Europëenne serologic assays for the BioRad SARS-CoV-2 IgG multiplex assay which measures receptor binding domain IgG (RBD), spike-S1 IgG (S1), spike-S2 IgG (S2), and nucleocapsid IgG (N). A subset of serial specimens from 14 patients was also tested for neutralizing antibodies (n = 61).

RESULTS

Specificity for RBD and S1 IgG was 99.4% (n = 170) and 100% for S2 and N IgG (n = 170) in a cohort selected for probable interference. Overall assay concordance with other assays was >93% for IgG and total antibody assays and reached 100% sensitivity for clinical concordance at >14 days as a multiplex assay. RBD and S1 binding antibody positivity demonstrated 79-95% agreement with the presence of neutralizing antibodies.

CONCLUSIONS

The BioRad SARS-CoV-2 IgG assay is comparable to existing assays, and achieved 100% sensitivity when all markers were included. The ability to measure antibodies against spike and nucleocapsid proteins simultaneously may be advantageous for complex clinical presentations, epidemiologic research, and in decisions regarding infection prevention strategies. Additional independent validations are needed to further determine binding antibody and neutralizing antibody correlations.

摘要

目的

在单次检测中检测针对多种 SARS-CoV-2 抗原的抗体,可提高诊断准确性,区分疫苗接种和自然感染,有助于追溯暴露情况。为了更好地了解针对 SARS-CoV-2 感染的体液免疫反应并建立保护相关性,需要将临床检测中的结合抗体评估与中和抗体相关联。

方法

使用了一个包含 752 个样本的队列,评估了 BioRad SARS-CoV-2 IgG 多重检测试剂盒(该试剂盒可检测受体结合域 IgG(RBD)、刺突蛋白-S1 IgG(S1)、刺突蛋白-S2 IgG(S2)和核衣壳蛋白 IgG(N))的特异性、敏感性,并与其他 6 种欧洲合格认证的血清学检测方法进行了比较。还对来自 14 名患者的部分连续标本(n=61)进行了中和抗体检测。

结果

在一个针对可能存在干扰的队列中,RBD 和 S1 IgG 的特异性分别为 99.4%(n=170)和 100%(n=170),而 S2 和 N IgG 的特异性均为 100%(n=170)。该检测试剂盒与其他 IgG 和总抗体检测方法的总体一致性>93%,作为一种多重检测方法,在 14 天以上的临床一致性中达到 100%的敏感性。RBD 和 S1 结合抗体阳性与中和抗体的存在有 79-95%的一致性。

结论

BioRad SARS-CoV-2 IgG 检测试剂盒与现有的检测试剂盒相当,当包含所有标志物时,其敏感性达到 100%。同时检测针对刺突蛋白和核衣壳蛋白的抗体的能力可能对复杂的临床表现、流行病学研究以及针对感染预防策略的决策具有优势。需要进行更多的独立验证,以进一步确定结合抗体和中和抗体的相关性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e1e9/8387133/f75ee0c9b7ed/gr1_lrg.jpg

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