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鉴定和表征一种用于检测临床样本中诺如病毒的肽亲和试剂。

Identification and characterization of a peptide affinity reagent for detection of noroviruses in clinical samples.

机构信息

Departments of Pharmacology, aylor College of Medicine, Houston, Texas, USA.

出版信息

J Clin Microbiol. 2013 Jun;51(6):1803-8. doi: 10.1128/JCM.00295-13. Epub 2013 Apr 3.

Abstract

Norovirus (NoV) is the most common agent of nonbacterial epidemic gastroenteritis and is estimated to cause 21 million cases of the disease in the United States annually. The antigen enzyme-linked immunosorbent assays (ELISAs) currently available for NoV diagnosis detect only certain strains and are approved for use in the United States only in epidemics where NoV is suspected. There is a clear need for simpler, more rapid, and more reliable diagnostic tools for the detection of NoV. In this study, phage display technology was used to screen a library of phage displaying random 12-mer peptides for those that bind to Norwalk virus virus-like particles (NV VLPs). Three phage clones displaying unique peptides were identified, and both the peptide-displaying phages and the peptides were confirmed to bind specifically to NV VLPs. The peptide displayed on phage clone NV-N-R5-1 was determined to bind to the protruding domain of the VP1 capsid protein. This phage also bound to NV VLPs seeded into NoV-negative stool with a limit of detection of 1.56 ng NV VLP. This value was comparable to monoclonal antibody (MAb) 3912, which is currently used in commercially available assays. Furthermore, the NV-N-R5-1 phage exhibited high specificity by detecting NV only in previously characterized NV-positive stool samples in contrast to no detection in NV-negative stool samples. These data demonstrate that the further development of NV-N-R5-1 phage as a diagnostic reagent is possible and might offer several distinct advantages over antibodies, such as decreases in the time and cost of production and ease of isolating phage against other epidemic strains currently circulating as well as those that are emerging.

摘要

诺如病毒(NoV)是最常见的非细菌性流行肠胃炎病原体,据估计,每年在美国导致 2100 万例该病。目前用于 NoV 诊断的抗原酶联免疫吸附测定(ELISA)仅检测某些特定株,并且仅在美国怀疑存在 NoV 流行时才被批准使用。显然需要更简单、更快速和更可靠的诊断工具来检测 NoV。在这项研究中,噬菌体展示技术被用于筛选噬菌体展示随机 12 肽文库,以寻找与诺如病毒样颗粒(NV VLPs)结合的肽。鉴定出三个显示独特肽的噬菌体克隆,并且噬菌体展示肽和肽都被证实特异性结合 NV VLPs。噬菌体克隆 NV-N-R5-1 上展示的肽被确定与 VP1 衣壳蛋白的突出结构域结合。这种噬菌体还与 NV VLPs 结合,NV VLPs 被播种到 NoV 阴性粪便中,检测限为 1.56ng NV VLP。这一值与目前用于商业检测的单克隆抗体(MAb)3912 相当。此外,与 NV 阴性粪便样本中无检测结果相比,NV-N-R5-1 噬菌体仅在先前表征的 NV 阳性粪便样本中检测到 NV,显示出高特异性。这些数据表明,进一步开发 NV-N-R5-1 噬菌体作为诊断试剂是可能的,并且可能比抗体具有几个明显的优势,例如降低生产时间和成本,以及更容易分离针对当前流行的其他流行株以及新兴株的噬菌体。

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