Mass cytometry uses metal-isotope-tagged antibodies to label targets of interest, which enables simultaneous measurements of ~50 proteins or protein modifications in millions of single cells, but its sensitivity is limited. Here, we present a signal amplification technology, termed Amplification by Cyclic Extension (ACE), implementing thermal-cycling-based DNA in situ concatenation in combination with 3-cyanovinylcarbazole phosphoramidite-based DNA crosslinking to enable signal amplification simultaneously on >30 protein epitopes. We demonstrate the utility of ACE in low-abundance protein quantification with suspension mass cytometry to characterize molecular reprogramming during the epithelial-to-mesenchymal transition as well as the mesenchymal-to-epithelial transition. We show the capability of ACE to quantify the dynamics of signaling network responses in human T lymphocytes. We further present the application of ACE in imaging mass cytometry-based multiparametric tissue imaging to identify tissue compartments and profile spatial aspects related to pathological states in polycystic kidney tissues.
Signal amplification by cyclic extension enables high-sensitivity single-cell mass cytometry.
通过循环延伸进行信号放大,可以实现高灵敏度的单细胞质谱流式细胞术
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作者:Lun Xiao-Kang, Sheng Kuanwei, Yu Xueyang, Lam Ching Yeung, Gowri Gokul, Serrata Matthew, Zhai Yunhao, Su Hanquan, Luan Jingyi, Kim Youngeun, Ingber Donald E, Jackson Hartland W, Yaffe Michael B, Yin Peng
| 期刊: | Nature Biotechnology | 影响因子: | 41.700 |
| 时间: | 2025 | 起止号: | 2025 May;43(5):811-821 |
| doi: | 10.1038/s41587-024-02316-x | 方法学: | FCM |
| 研究方向: | 细胞生物学 | ||
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