Cytometry in the short-wave infrared

Author:

Lin Ching-Wei1ORCID,Liu Te-I1ORCID,Wang Jhih-Shan2,Nguyen Ai-Phuong1ORCID,Raabe Marco1,Quiroz Carlos3,Lin Chih-Hsin4ORCID

Affiliation:

1. Academia Sinica

2. University of Stuttgart

3. Institute of Atomic and Molecular Sciences, Academia Sinica

4. Taipei Medical University

Abstract

Abstract Cytometry plays a crucial role in characterizing cell properties, but its restricted optical window (400-850 nm) limits the number of stained fluorophores that can be detected simultaneously and hampers the study and utilization of short-wave infrared (SWIR; 900-1,700 nm) fluorophores in cells. Here we introduce two SWIR-based methods to address these limitations: SWIR flow cytometry and SWIR image cytometry. We develop a quantification protocol for deducing cellular fluorophore mass. Both systems achieve a limit of detection of ~0.1 fg cell−1 within a 30-min experimental timeframe, using individualized, high-purity (6,5) single-wall carbon nanotubes as a model fluorophore and macrophage-like RAW264.7 as a model cell line. This high-sensitivity feature reveals that low-dose (6,5) serves as an antioxidant, and cell morphology and oxidative stress dose-dependently correlate with (6,5) uptake. Our SWIR cytometry holds immediate applicability for existing SWIR fluorophores and offers a solution to the issue of spectral overlapping in conventional cytometry.

Publisher

Research Square Platform LLC

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