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An integrated flow cytometry-based platform for isolation and molecular characterization of circulating tumor single cells and clusters

机译:基于流式细胞术的分离和分子表征循环肿瘤单细胞和簇的集成流式细胞术平台

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Comprehensive molecular analysis of rare circulating tumor cells (CTCs) and cell clusters is often hampered by low throughput and purity, as well as cell loss. To address this, we developed a fully integrated platform for flow cytometry-based isolation of CTCs and clusters from blood that can be combined with whole transcriptome analysis or targeted RNA transcript quantification. Downstream molecular signature can be linked to cell phenotype through index sorting. This newly developed platform utilizes in-line magnetic particle-based leukocyte depletion, and acoustic cell focusing and washing to achieve 98% reduction of blood cells and non-cellular debris, along with 1.5 log-fold enrichment of spiked tumor cells. We could also detect 1 spiked-in tumor cell in 1 million WBCs in 4/7 replicates. Importantly, the use of a large 200μm nozzle and low sheath pressure (3.5?psi) minimized shear forces, thereby maintaining cell viability and integrity while allowing for simultaneous recovery of single cells and clusters from blood. As proof of principle, we isolated and transcriptionally characterized 63 single CTCs from a genetically engineered pancreatic cancer mouse model (n?=?12 mice) and, using index sorting, were able to identify distinct epithelial and mesenchymal sub-populations based on linked single cell protein and gene expression.
机译:罕见的循环肿瘤细胞(CTC)和细胞簇的综合分子分析通常是通过低通量和纯度而阻碍的,以及细胞损失。为了解决这一点,我们开发了一种完全集成的平台,用于流式细胞术的基于流式细胞术和来自血液的簇的分离,可以与整个转录组分析或靶向RNA转录物定量相结合。下游分子签名可以通过指数分选与细胞表型连接。该新开发的平台利用在线磁性粒子的白细胞消耗,以及吸音和洗涤以实现血细胞和非细胞碎片的减少> 1.5倍瘤细胞的富集浓缩的98%。我们还可以在4/7重复的100万WBC中检测1次肿瘤细胞。重要的是,使用大的200μm喷嘴和低鞘压(3.5?psi)最小化剪切力,从而保持细胞活力和完整性,同时允许同时恢复单个细胞和来自血液的簇。作为原理的证据,我们分离和转录从遗传工程胰腺癌小鼠模型(N?= 12只小鼠)的63个单CTC,并且使用指数分选,能够基于链接的单一识别不同的上皮和间充质亚群细胞蛋白和基因表达。

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