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LASIC: Light Activated Site-Specific Conjugation of Native IgGs

机译:LASIC:天然IgG的光激活位点特异性缀合

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摘要

Numerous biological applications, from diagnostic assays to immunotherapies, rely on the use of antibody-conjugates. The efficacy of these conjugates can be significantly influenced by the site at which Immunoglobulin G (IgG) is modified. Current methods that provide control over the conjugation site, however, suffer from a number of shortfalls and often require large investments of time and cost. We have developed a novel adapter protein that, when activated by long wavelength UV light, can covalently and site-specifically label the Pc region of nearly any native, full-length IgG, including all human IgG subclasses. Labeling occurs with unprecedented efficiency and speed (>90% after 30 min), with no effect on IgG affinity. The adapter domain can be bacterially expressed and customized to contain a variety of moieties (e.g., biotin, azide, fluorophores), making reliable and efficient conjugation of antibodies widely accessible to researchers at large.
机译:从诊断检测到免疫治疗,许多生物学应用都依赖抗体结合物的使用。这些缀合物的功效会受到免疫球蛋白G(IgG)修饰的位点的显着影响。然而,提供对接合部位的控制的当前方法存在许多缺点,并且常常需要大量的时间和成本投资。我们开发了一种新型衔接蛋白,当被长波长紫外线激活时,它可以共价和位点特异性标记几乎所有天然,全长IgG(包括所有人类IgG亚类)的Pc区。标记以前所未有的效率和速度发生(30分钟后> 90%),而对IgG亲和力没有影响。衔接子结构域可以被细菌表达并被定制为包含各种部分(例如,生物素,叠氮化物,荧光团),从而使抗体的可靠和有效的缀合对于广大研究人员而言是广泛可及的。

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