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基于液滴的微流控技术进行功能型单细胞杂交瘤筛选。

Functional single-cell hybridoma screening using droplet-based microfluidics.

机构信息

Institut de Science et d'Ingénierie Supramoléculaires, Université de Strasbourg, 8 allée Gaspard Monge, 67083 Strasbourg Cedex, France.

出版信息

Proc Natl Acad Sci U S A. 2012 Jul 17;109(29):11570-5. doi: 10.1073/pnas.1204514109. Epub 2012 Jul 2.

DOI:10.1073/pnas.1204514109
PMID:22753519
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3406880/
Abstract

Monoclonal antibodies can specifically bind or even inhibit drug targets and have hence become the fastest growing class of human therapeutics. Although they can be screened for binding affinities at very high throughput using systems such as phage display, screening for functional properties (e.g., the inhibition of a drug target) is much more challenging. Typically these screens require the generation of immortalized hybridoma cells, as well as clonal expansion in microtiter plates over several weeks, and the number of clones that can be assayed is typically no more than a few thousand. We present here a microfluidic platform allowing the functional screening of up to 300,000 individual hybridoma cell clones within less than a day. This approach should also be applicable to nonimmortalized primary B-cells, as no cell proliferation is required: Individual cells are encapsulated into aqueous microdroplets and assayed directly for the release of antibodies inhibiting a drug target based on fluorescence. We used this system to perform a model screen for antibodies that inhibit angiotensin converting enzyme 1, a target for hypertension and congestive heart failure drugs. When cells expressing these antibodies were spiked into an unrelated hybridoma cell population in a ratio of 1:10,000 we observed a 9,400-fold enrichment after fluorescence activated droplet sorting. A wide variance in antibody expression levels at the single-cell level within a single hybridoma line was observed and high expressors could be successfully sorted and recultivated.

摘要

单克隆抗体可以特异性结合甚至抑制药物靶点,因此已成为增长最快的一类人类治疗药物。尽管可以使用噬菌体展示等系统以非常高的通量筛选结合亲和力,但筛选功能特性(例如,抑制药物靶点)则更具挑战性。通常,这些筛选需要生成永生化杂交瘤细胞,并且在微滴定板中克隆扩增数周,可进行测定的克隆数量通常不超过几千个。我们在这里介绍了一种微流控平台,该平台可在不到一天的时间内对多达 300,000 个单个杂交瘤细胞克隆进行功能筛选。该方法也应该适用于非永生化的原始 B 细胞,因为不需要细胞增殖:将单个细胞包封在水性微滴中,并直接基于荧光测定抑制药物靶点的抗体释放。我们使用该系统进行了模型筛选,以获得抑制血管紧张素转换酶 1(高血压和充血性心力衰竭药物的靶标)的抗体。当将表达这些抗体的细胞以 1:10,000 的比例掺入到无关的杂交瘤细胞群中时,我们在荧光激活的液滴分选后观察到 9,400 倍的富集。在单个杂交瘤系内的单个细胞水平上观察到抗体表达水平的广泛差异,并且可以成功地对高表达者进行分选和再培养。

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Memory B cell antibodies to HIV-1 gp140 cloned from individuals infected with clade A and B viruses.从感染 A 型和 B 型病毒的个体中克隆的 HIV-1 gp140 的记忆 B 细胞抗体。
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