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Screening one bead one compound libraries against serum using a flow cytometer: Determination of the minimum antibody concentration required for ligand discovery

机译:使用流式细胞仪筛选一个珠子对血清的一种复合文库:测定配体发现所需的最小抗体浓度

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One bead one compound (OBOC) libraries can be screened against serum samples to identify ligands to antibodies in this mixture. In this protocol, hit beads are identified by staining with a fluorescent labeled secondary antibody. When screens are conducted against two different sets of serum, antibodies, and ligands to them, can be discovered that distinguish the two populations. The application of DNA-encoding technology to OBOC libraries has allowed the use of 10?μm beads for library preparation and screening, which pass through a standard flow cytometer, allowing the fluorescent hit beads to be separated from beads displaying non-ligands easily. An important issue in using this approach for the discovery of antibody biomarkers is its analytical sensitivity. In other words, how abundant must an IgG be to allow it to be pulled out of serum in an unbiased screen using a flow cytometer? We report here a model study in which monoclonal antibodies with known ligands of varying affinities are doped into serum. We find that for antibody ligands typical of what one isolates from an unbiased combinatorial library, the target antibody must be present at 10–50?nM. True antigens, which bind with significantly higher affinity, can detect much less abundant serum antibodies.
机译:可以筛选一个珠子一种化合物(OBOC)文库,用于针对血清样品筛选,以鉴定该混合物中的抗体的配体。在该方案中,通过用荧光标记的二抗染色来鉴定麦芽珠。当屏幕与两组不同的血清,抗体和配体进行时,可以被发现区分两种群体。将DNA编码技术应用于OBOC图书馆,允许使用10?μm珠粒用于库制备和筛选,其通过标准流式细胞仪,允许荧光撞击珠子容易地与显示非配体显示非配体的珠子分离。使用这种方法对发现抗体生物标志物的重要问题是其分析敏感性。换句话说,IGG必须丰富,以便使用流式细胞仪在无偏筛网中释放出血清中的血清?我们在此报告了一种模型研究,其中具有不同亲和力的已知配体的单克隆抗体掺杂到血清中。我们发现,对于典型的抗体配体,典型的一种分离物来自无偏的组合库,靶抗体必须在10-50℃下存在。真正的抗原与显着更高的亲和力结合,可以检测到大量丰富的血清抗体。

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