Identifying lipid particle sub-types in live Caenorhabditis elegans with two-photon fluorescence lifetime imaging

Wei-Wen Chen; Wenyu Tang; Emily K Hamerton; Penelope X Kuo; George A Lemieux; Kaveh Ashrafi; Marcus T Cicerone

doi:10.3389/fchem.2023.1161775

Identifying lipid particle sub-types in live Caenorhabditis elegans with two-photon fluorescence lifetime imaging

Front Chem. 2023 Apr 13:11:1161775. doi: 10.3389/fchem.2023.1161775. eCollection 2023.

Authors

Wei-Wen Chen¹, Wenyu Tang¹, Emily K Hamerton¹, Penelope X Kuo², George A Lemieux³, Kaveh Ashrafi³, Marcus T Cicerone¹

Affiliations

¹ School of Chemistry and Biochemistry, Georgia Institute of Technology, Atlanta, GA, United States.
² School of Environmental and Biological Sciences, Rutgers University, New Brunswick, NJ, United States.
³ School of Medicine, University of California, San Francisco, CA, United States.

Abstract

Fat metabolism is an important modifier of aging and longevity in Caenorhabditis elegans. Given the anatomy and hermaphroditic nature of C. elegans, a major challenge is to distinguish fats that serve the energetic needs of the parent from those that are allocated to the progeny. Broadband coherent anti-Stokes Raman scattering (BCARS) microscopy has revealed that the composition and dynamics of lipid particles are heterogeneous both within and between different tissues of this organism. Using BCARS, we have previously succeeded in distinguishing lipid-rich particles that serve as energetic reservoirs of the parent from those that are destined for the progeny. While BCARS microscopy produces high-resolution images with very high information content, it is not yet a widely available platform. Here we report a new approach combining the lipophilic vital dye Nile Red and two-photon fluorescence lifetime imaging microscopy (2p-FLIM) for the in vivo discrimination of lipid particle sub-types. While it is widely accepted that Nile Red staining yields unreliable results for detecting lipid structures in live C. elegans due to strong interference of autofluorescence and non-specific staining signals, our results show that simple FLIM phasor analysis can effectively separate those signals and is capable of differentiating the non-polar lipid-dominant (lipid-storage), polar lipid-dominant (yolk lipoprotein) particles, and the intermediates that have been observed using BCARS microscopy. An advantage of this approach is that images can be acquired using common, commercially available 2p-FLIM systems within about 10% of the time required to generate a BCARS image. Our work provides a novel, broadly accessible approach for analyzing lipid-containing structures in a complex, live whole organism context.

Keywords: C. elegans; aging; coherent Raman imaging; fluorescence lifetime imaging microscopy (FLIM); in vivo imaging; lipid metabolism; two-photon excitation fluorescence (TPEF) imaging; yolk lipoprotein.

Grants and funding

P30 DK098722/DK/NIDDK NIH HHS/United States