Assessing cell viability with dynamic optical coherence microscopy

Author:

Liu Chao J.1ORCID,Smith Jason T.1ORCID,Wang Yuanbo1,Ouellette Jonathan N.1,Rogers Jeremy D.2ORCID,Oliner Jonathan D.1,Szulczewski Michael1,Wait Eric1,Brown William3,Wax Adam3ORCID,Eliceiri Kevin W.4ORCID,Rafter John1

Affiliation:

1. Elephas Biosciences Corporation

2. University of Wisconsin Madison

3. Lumedica Inc.

4. Center for Quantitative Cell Imaging

Abstract

Assessing cell viability is important in many fields of research. Current optical methods to assess cell viability typically involve fluorescent dyes, which are often less reliable and have poor permeability in primary tissues. Dynamic optical coherence microscopy (dOCM) is an emerging tool that provides label-free contrast reflecting changes in cellular metabolism. In this work, we compare the live contrast obtained from dOCM to viability dyes, and for the first time to our knowledge, demonstrate that dOCM can distinguish live cells from dead cells in murine syngeneic tumors. We further demonstrate a strong correlation between dOCM live contrast and optical redox ratio by metabolic imaging in primary mouse liver tissue. The dOCM technique opens a new avenue to apply label-free imaging to assess the effects of immuno-oncology agents, targeted therapies, chemotherapy, and cell therapies using live tumor tissues.

Publisher

Optica Publishing Group

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