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HPV 型 16 特异性修饰 DNA 适体的开发和特性鉴定,用于提高效力检测。

Development and Characterization of an HPV Type-16 Specific Modified DNA Aptamer for the Improvement of Potency Assays.

机构信息

Department of Vaccine Analytical Development, MRL, Merck & Co., Inc. , West Point, Pennsylvania 19486, United States.

出版信息

Anal Chem. 2017 Mar 21;89(6):3554-3561. doi: 10.1021/acs.analchem.6b04852. Epub 2017 Mar 8.

DOI:10.1021/acs.analchem.6b04852
PMID:28233502
Abstract

Measuring vaccine potency is critical for vaccine release and is often accomplished using antibody-based ELISAs. Antibodies can be associated with significant drawbacks that are often overlooked including lot-to-lot variability, problems with cell-line maintenance, limited stability, high cost, and long discovery lead times. Here, we address many of these issues through the development of an aptamer, known as a slow off-rate modified DNA aptamer (SOMAmer), which targets a vaccine antigen in the human papillomavirus (HPV) vaccine Gardasil. The aptamer, termed HPV-07, was selected to bind the Type 16 virus-like-particle (VLP) formed by the self-assembling capsid protein L1. It is capable of binding with high sensitivity (EC of 0.1 to 0.4 μg/mL depending on assay format) while strongly discriminating against other VLP types. The aptamer competes for binding with the neutralizing antibody H16.V5, indicating at least partial recognition of a neutralizing and clinically relevant epitope. This makes it a useful reagent for measuring both potency and stability. When used in an ELISA format, the aptamer displays both high precision (intermediate precision of 6.3%) and a large linear range spanning from 25% to 200% of a typical formulation. To further exploit the advantages of aptamers, a simplified mix and read assay was also developed. This assay format offers significant time and resource reductions compared to a traditional ELISA. These results show aptamers are suitable reagents for biological potency assays, and we expect that their implementation could improve upon current assay formats.

摘要

测定疫苗效价对于疫苗放行至关重要,通常采用基于抗体的 ELISA 来实现。然而,抗体存在一些显著的缺点,这些缺点往往被忽视,包括批次间差异、细胞系维持问题、稳定性有限、成本高以及发现时间长等。在这里,我们通过开发一种适体(称为慢解离率修饰 DNA 适体,SOMAmer)来解决其中的许多问题,该适体针对人乳头瘤病毒(HPV)疫苗 Gardasil 中的疫苗抗原。该适体称为 HPV-07,被选择来结合由自组装衣壳蛋白 L1 形成的 16 型病毒样颗粒(VLP)。它能够以高灵敏度结合(取决于检测模式,EC 值为 0.1 至 0.4μg/mL),同时强烈区分其他 VLP 类型。该适体与中和抗体 H16.V5 竞争结合,表明至少部分识别中和和临床相关表位。这使其成为测量效价和稳定性的有用试剂。当用于 ELISA 模式时,该适体显示出高精确度(中间精度为 6.3%)和大线性范围,从典型配方的 25%到 200%。为了进一步利用适体的优势,还开发了一种简化的混合和读取检测方法。与传统 ELISA 相比,该检测方法在时间和资源方面具有显著优势。这些结果表明适体是生物效价检测的合适试剂,我们期望它们的应用可以改进当前的检测方法。

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