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在配对皮升级分室中,对单细胞水平的蛋白质和转录组的表达动态进行解码。

Decoding Expression Dynamics of Protein and Transcriptome at the Single-Cell Level in Paired Picoliter Chambers.

机构信息

Collaborative Innovation Center of Chemistry for Energy Materials, The MOE Key Laboratory of Spectrochemical Analysis and Instrumentation, State Key Laboratory of Physical Chemistry of Solid Surfaces, Department of Chemical Biology, College of Chemistry and Chemical Engineering, Xiamen University, Xiamen, Fujian 361005, China.

Suzhou Dynamic Biosystems Co., Ltd., Suzhou, Jiangsu 215000, China.

出版信息

Anal Chem. 2022 Jun 14;94(23):8164-8173. doi: 10.1021/acs.analchem.1c05312. Epub 2022 Jun 1.

Abstract

Simultaneous analysis of mRNAs and proteins at the single-cell level provides information about the dynamics and correlations of gene and protein expressions in individual cells, enabling a comprehensive study of cellular heterogeneity and expression patterns. Here, we present a platform for about 1000 cellular indexing of mRNAs and membrane proteins, named multi-Paired-seq, with high cell utilization, accurate molecular measurement, and low cost. Based on hydrodynamic differential flow resistance, multi-Paired-seq largely improves cell utilization in the percentage of cells measured in population (>95%). Combined with the pump/valve structure, cell-free antibodies and mRNAs can be removed completely for highly accurate detection ( = 0.96) of protein copies. The picoliter reaction chambers allow high detection sensitivity for both mRNA transcripts and protein copies and low sequencing cost. Using multi-Paired-seq, three clusters of known breast cancer cell types are identified according to multimodal measurements, and the expression correlations between mRNAs and proteins under altered conditions are quantified. Multi-Paired-seq provides multimodal measurements at the single-cell level, which offers a new tool for cell biology, developmental biology, drug discovery, and precision medicine.

摘要

在单细胞水平上同时分析 mRNA 和蛋白质,可以提供关于单个细胞中基因和蛋白质表达的动态和相关性的信息,从而全面研究细胞异质性和表达模式。在这里,我们提出了一种名为多配对测序(multi-Paired-seq)的用于约 1000 个细胞的 mRNA 和膜蛋白的同时分析的平台,该平台具有高细胞利用率、准确的分子测量和低成本的特点。基于流体动力学的差分流动阻力,多配对测序大大提高了群体中被测量细胞的百分比(>95%)的细胞利用率。结合泵/阀结构,细胞游离抗体和 mRNAs 可以被完全去除,从而实现高度准确的蛋白拷贝检测(=0.96)。皮升级反应室允许对 mRNA 转录本和蛋白拷贝进行高检测灵敏度和低测序成本。使用多配对测序,根据多模态测量结果鉴定出三种已知的乳腺癌细胞类型簇,并量化了改变条件下 mRNA 和蛋白质之间的表达相关性。多配对测序在单细胞水平上提供了多模态测量,为细胞生物学、发育生物学、药物发现和精准医学提供了一种新工具。

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