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Single-cell barcode analysis provides a rapid readout of cellular signaling pathways in clinical specimens

机译:单细胞条形码分析可快速读取临床标本中的细胞信号通路

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Serial tissue sampling has become essential in guiding modern targeted and personalized cancer treatments. An alternative to image guided core biopsies are fine needle aspirates (FNA) that yield cells rather than tissues but are much better tolerated and have lower complication rates. The efficient pathway analysis of such cells in the clinic has been difficult, time consuming and costly. Here we develop an antibody-DNA barcoding approach where harvested cells can be rapidly re-stained through the use of custom designed oligonucleotide-fluorophore conjugates. We show that this approach can be used to interrogate drug-relevant pathways in scant clinical samples. Using the PI3K/PTEN/CDK4/6 pathways in breast cancer as an example, we demonstrate how analysis can be performed in tandem with trial enrollment and can evaluate downstream signaling following therapeutic inhibition. This approach should allow more widespread use of scant single cell material in clinical samples.
机译:连续组织采样已成为指导现代靶向和个性化癌症治疗的关键。图像引导核心活检的替代方法是细针穿刺术(FNA),可产生细胞而不是组织,但耐受性好得多,并发症发生率较低。在临床中对此类细胞进行有效的途径分析是困难,费时且昂贵的。在这里,我们开发了一种抗体-DNA条形码方法,其中可以通过使用定制设计的寡核苷酸-荧光团结合物快速重现收获的细胞。我们表明,该方法可用于询问临床样品较少的药物相关途径。以乳腺癌中的PI3K / PTEN / CDK4 / 6途径为例,我们演示了如何与试验入组同时进行分析,并可以评估治疗抑制后的下游信号传导。这种方法应允许在临床样品中更广泛地使用稀少的单细胞材料。

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