Exploring functional protein covariation across single cells using nPOP

Andrew Leduc; R Gray Huffman; Joshua Cantlon; Saad Khan; Nikolai Slavov

doi:10.1186/s13059-022-02817-5

Exploring functional protein covariation across single cells using nPOP

Genome Biol. 2022 Dec 16;23(1):261. doi: 10.1186/s13059-022-02817-5.

Authors

Andrew Leduc¹, R Gray Huffman², Joshua Cantlon³, Saad Khan², Nikolai Slavov⁴

Affiliations

¹ Departments of Bioengineering, Biology, Chemistry and Chemical Biology, Single Cell Proteomics Center, and Barnett Institute, Northeastern University, Boston, MA, 02115, USA. leduc.an@northeastern.edu.
² Departments of Bioengineering, Biology, Chemistry and Chemical Biology, Single Cell Proteomics Center, and Barnett Institute, Northeastern University, Boston, MA, 02115, USA.
³ Scienion AG, Phoenix, AZ, 85042, USA.
⁴ Departments of Bioengineering, Biology, Chemistry and Chemical Biology, Single Cell Proteomics Center, and Barnett Institute, Northeastern University, Boston, MA, 02115, USA. nslavov@alum.mit.edu.

Abstract

Background: Many biological processes, such as cell division cycle and drug resistance, are reflected in protein covariation across single cells. This covariation can be quantified and interpreted by single-cell mass spectrometry with sufficiently high throughput and accuracy.

Results: Here, we describe nPOP, a method that enables simultaneous sample preparation of thousands of single cells, including lysing, digesting, and labeling individual cells in volumes of 8-20 nl. nPOP uses piezo acoustic dispensing to isolate individual cells in 300 pl volumes and performs all subsequent sample preparation steps in small droplets on a fluorocarbon-coated glass slide. Protein covariation analysis identifies cell cycle dynamics that are similar and dynamics that differ between cell types, even within subpopulations of melanoma cells delineated by markers for drug resistance priming. Melanoma cells expressing these markers accumulate in the G1 phase of the cell cycle, display distinct protein covariation across the cell cycle, accumulate glycogen, and have lower abundance of glycolytic enzymes. The non-primed melanoma cells exhibit gradients of protein abundance, suggesting transition states. Within this subpopulation, proteins functioning in oxidative phosphorylation covary with each other and inversely with proteins functioning in glycolysis. This protein covariation suggests divergent reliance on energy sources and its association with other biological functions. These results are validated by different mass spectrometry methods.

Conclusions: nPOP enables flexible, automated, and highly parallelized sample preparation for single-cell proteomics. This allows for quantifying protein covariation across thousands of single cells and revealing functionally concerted biological differences between closely related cell states. Support for nPOP is available at https://scp.slavovlab.net/nPOP .

Keywords: Cell division cycle; Drug resistance; Protein covariation; Sample preparation; Single cell; Single-cell proteomics.

Publication types

Research Support, N.I.H., Extramural
Research Support, Non-U.S. Gov't

MeSH terms

Humans
Mass Spectrometry
Melanoma*
Proteins*
Proteomics

Substances

Proteins

Abstract

Publication types

MeSH terms

Substances

Grants and funding