Enhanced sensitivity and scalability with a Chip-Tip workflow enables deep single-cell proteomics.

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Tác giả: Nicolai Bache, Dorte B Bekker-Jensen, Karl-Henrik Grinnemo, Ulises H Guzman, David Hartlmayr, Ole B Hørning, Haoran Huang, Min Huang, Fabiana Izaguirre, Hiren J Joshi, Maico Y Lechner, Xiangjun Li, Zhen Liu, Jesper V Olsen, Teeradon Phlairaharn, Sergey Rodin, Pierre Sabatier, Anjali Seth, Leander van der Hoeven, Zilu Ye

Ngôn ngữ: eng

Ký hiệu phân loại: 598.635 *Bonasa

Thông tin xuất bản: United States : Nature methods , 2025

Mô tả vật lý:

Bộ sưu tập: NCBI

ID: 701108

 Single-cell proteomics (SCP) promises to revolutionize biomedicine by providing an unparalleled view of the proteome in individual cells. Here, we present a high-sensitivity SCP workflow named Chip-Tip, identifying >
 5,000 proteins in individual HeLa cells. It also facilitated direct detection of post-translational modifications in single cells, making the need for specific post-translational modification-enrichment unnecessary. Our study demonstrates the feasibility of processing up to 120 label-free SCP samples per day. An optimized tissue dissociation buffer enabled effective single-cell disaggregation of drug-treated cancer cell spheroids, refining overall SCP analysis. Analyzing nondirected human-induced pluripotent stem cell differentiation, we consistently quantified stem cell markers OCT4 and SOX2 in human-induced pluripotent stem cells and lineage markers such as GATA4 (endoderm), HAND1 (mesoderm) and MAP2 (ectoderm) in different embryoid body cells. Our workflow sets a benchmark in SCP for sensitivity and throughput, with broad applications in basic biology and biomedicine for identification of cell type-specific markers and therapeutic targets.
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