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免疫靶向纳米晶体的工程抗体SpyCatcher 偶联。

Immunotargeting of Nanocrystals by SpyCatcher Conjugation of Engineered Antibodies.

机构信息

Department of Pharmaceutical Chemistry, University of California San Francisco, San Francisco, California 94143, United States.

出版信息

ACS Nano. 2021 Nov 23;15(11):18374-18384. doi: 10.1021/acsnano.1c07856. Epub 2021 Oct 25.

Abstract

Inorganic nanocrystals such as quantum dots (QDs) and upconverting nanoparticles (UCNPs) are uniquely suited for quantitative live-cell imaging and are typically functionalized with ligands to study specific receptors or cellular targets. Antibodies (Ab) are among the most useful targeting reagents owing to their high affinities and specificities, but common nanocrystal labeling methods may orient Ab incorrectly, be reversible or denaturing, or lead to Ab-NP complexes too large for some applications. Here, we show that SpyCatcher proteins, which bind and spontaneously form covalent isopeptide bonds with cognate SpyTag peptides, can conjugate engineered Ab to nanoparticle surfaces with control over stability, orientation, and stoichiometry. Compact SpyCatcher-functionalized QDs and UCNPs may be labeled with short-chain variable fragment Ab (scFv) engineered to bind urokinase-type plasminogen activator receptors (uPAR) that are overexpressed in many human cancers. Confocal imaging of anti-uPAR scFv-QD conjugates shows the antibody mediates specific binding and internalization by breast cancer cells expressing uPAR. Time-lapse imaging of photostable scFv-UCNP conjugates shows that Ab binding causes uPAR internalization with a ∼20 min half-life on the cell surface, and uPAR is internalized to endolysosomal compartments distinct from general membrane stains and without significant recycling to the cell surface. The controlled and stable conjugation of engineered Ab to NPs enables targeting of diverse receptors for live-cell study of their distribution, trafficking, and physiology.

摘要

无机纳米晶体,如量子点 (QD) 和上转换纳米颗粒 (UCNP),非常适合定量活细胞成像,通常通过配体功能化来研究特定的受体或细胞靶标。抗体 (Ab) 是最有用的靶向试剂之一,因为它们具有高亲和力和特异性,但常见的纳米晶体标记方法可能会导致 Ab 定向不正确、可逆转或变性,或者导致 Ab-NP 复合物太大而无法用于某些应用。在这里,我们展示了 SpyCatcher 蛋白,它可以与同源的 SpyTag 肽结合并自发形成共价异肽键,可以控制稳定性、定向性和化学计量比,将工程化的 Ab 偶联到纳米颗粒表面。紧凑型 SpyCatcher 功能化的 QD 和 UCNP 可以用短链可变片段 Ab (scFv) 进行标记,该 Ab 设计用于结合在许多人类癌症中过度表达的尿激酶型纤溶酶原激活受体 (uPAR)。抗 uPAR scFv-QD 缀合物的共焦成像显示抗体介导了乳腺癌细胞中 uPAR 的特异性结合和内化。光稳定的 scFv-UCNP 缀合物的延时成像显示,Ab 结合导致 uPAR 内化,在细胞表面的半衰期约为 20 分钟,并且 uPAR 被内化到不同于一般膜染色且没有明显再循环到细胞表面的内溶酶体隔室中。工程化 Ab 与 NPs 的可控和稳定偶联能够靶向各种受体,用于活细胞研究它们的分布、运输和生理学。

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