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Preparation and Characterization of Two Immunogens and Production of Polyclonal Antibody with High Affinity and Specificity for Darunavir

机译:两种免疫原的制备与表征具有高亲和力的多克隆抗体和Darunavir的特异性

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摘要

Darunavir (DRV) is a potent antiviral drug used for treatment of infections with human immunodeficiency virus (HIV). Effective and safe treatment with DRV requires its therapeutic drug monitoring (TDM) in patient’s plasma during therapy. To support TDM of DRV, a specific antibody with high affinity is required in order to develop a sensitive immunoassay for the accurate determination of DRV in plasma. In this study, two new and different immunogens were prepared and characterized. These immunogens were the DRV conjugates with keyhole limpet hemocyanin (KLH) protein. The first immunogen (DRV-KLH) was prepared by zero-length direct linking of DRV via its aromatic amino group with the tyrosine amino acid residues of KLH by diazotization/coupling reaction. The second immunogen (G-DRV-KLH) was prepared by conjugation of the N-glutaryl derivative of DRV (G-DRV) with KLH. The 5-carbon atoms-spacing G-DRV hapten was synthesized by reaction of DRV via its aromatic amino group with glutaric anhydride. The reaction was monitored by HPLC and the chemical structure of G-DRV was confirmed by mass, 1H-NMR, and 13C-NMR spectroscopic techniques. The hapten (G-DRV) was linked to the KLH protein by water-soluble 1-ethyl-3-(3-dimethylaminopropyl) carbodiimide (EDC) coupling procedure. The pertinence of the coupling reactions of haptens to protein was confirmed, and the immunogens were characterized by ultraviolet (UV) spectrophotometry. Both DRV-KLH and G-DRV-KLH were used for the immunization of animals and the animal’s antiserum that showed the highest affinity was selected. The collected antiserum (polyclonal antibody) had very high affinity to DRV (IC50 value = 0.2 ng mL−1; defining IC50 as the DRV concentration that can inhibit antibody binding by 50% of its maximum binding) and high specificity to DRV among other drugs used in the combination therapy with DRV. Cumulative results from direct and competitive enzyme-linked immunosorbent assay (ELISA) using this polyclonal antibody proved that the immunogens were highly antigenic and elicited a specific polyclonal antibody. The produced polyclonal antibody is valuable for the development of highly sensitive and selective immunoassays for TDM of DRV.
机译:Darunavir(DRV)是一种有效的抗病毒药物,用于治疗人类免疫缺陷病毒(HIV)的感染。在治疗期间,患有DRV的有效和安全治疗需要其治疗药物监测(TDM)患者的血浆。为了支持DRV的TDM,需要具有高亲和力的特异性抗体,以便开发敏感的免疫测定以准确测定血浆中的DRV。在这项研究中,制备了两种新的和不同的免疫原和表征。这些免疫原是与匙孔颗粒血糖(KLH)蛋白质的DRV缀合物。通过通过其芳族氨基通过重氮化/偶联反应通过其芳族氨基通过其芳族氨基与酪氨酸氨基酸残基的Zyrosine氨基酸残基进行第一免疫原性(DRV-KLH)。通过将DRV(G-DRV)的N-戊芳基衍生物与KLH的缀合来制备第二种免疫原性(G-DRV-KLH)。通过用戊二酸酐的芳族氨基反应,通过DRV反应合成5-碳原子间距G-DRV Hapten。通过HPLC监测反应,并通过质量,1H-NMR和13C-NMR光谱技术证实G-DRV的化学结构。通过水溶性1-乙基-3-(3-二甲基氨基丙基)碳二亚胺(EDC)偶联方法,HAPTEN(G-DRV)与KLH蛋白质连接。确认了Haptens对蛋白质的偶联反应的问题,通过紫外(UV)分光光度法表征了免疫原。 DRV-KLH和G-DRV-KLH都用于免疫动物,并且选择显示最高亲和力的动物的抗血清。收集的抗血清(多克隆抗体)对DRV具有非常高的亲和力(IC50值= 0.2ng -1;定义IC50作为DRV浓度,可以抑制其最大结合50%的50%的抗体,并且在其他药物中的DRV具有高特异性用于DRV的组合疗法。使用该多克隆抗体的直接和竞争性酶联免疫吸附测定(ELISA)的累积结果证明了免疫原是高抗原并引发特定的多克隆抗体。所产生的多克隆抗体对于用于DDM的TDM的高敏感和选择性免疫测定是有价值的。

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