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Cellular Barcodes for Efficiently Profiling Single-Cell Secretory Responses by Microengraving

机译:通过微雕刻有效地分析单细胞分泌反应的细胞条形码。

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We present a method that uses fluorescent cellular barcodes to increase the number of unique samples that can be analyzed simultaneously by microengraving, a nanowell array-based technique for quantifying the secretory responses of thousands of single cells in parallel. Using n different fluorescent dyes to generate 2~n unique cellular barcodes, we achieved a 2~n-fold reduction in the number of arrays and quantity of reagents required per sample. The utility of this approach was demonstrated in three applications of interest in clinical and experimental immunology. Using barcoded human peripheral blood mononuclear cells and T cells, we constructed dose-response curves, profiled the secretory behavior of cells treated with mechanistically distinct stimuli, and tracked the secretory behaviors of different lineages of CD4~+ T helper cells. In addition to increasing the number of samples analyzed by generating secretory profiles of single cells from multiple populations in a time- and reagent-efficient manner, we expect that cellular barcoding in combination with microengraving will facilitate unique experimental opportunities for quantitatively analyzing interactions among heterogeneous cells isolated in small groups (~2-5 cells).
机译:我们提出了一种使用荧光细胞条形码增加可通过微雕刻同时分析的独特样品数量的方法,微雕刻是一种基于纳米孔阵列的技术,用于量化并行处理数千个单细胞的分泌反应。使用n种不同的荧光染料生成2〜n个独特的细胞条形码,我们使每个样品所需的阵列数量和所需试剂数量减少了2〜n倍。在临床和实验免疫学中感兴趣的三个应用中证明了该方法的实用性。我们使用条形码的人类外周血单核细胞和T细胞,绘制了剂量-反应曲线,描绘了机械性不同刺激处理的细胞的分泌行为,并跟踪了CD4〜+ T辅助细胞不同谱系的分泌行为。除了通过以时间和试剂有效的方式从多个群体生成单细胞的分泌谱来增加分析样品的数量外,我们还期望细胞条形码与微雕刻技术的结合将为定量分析异质细胞之间相互作用提供独特的实验机会分成小群(约2-5个细胞)。

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