Wide field-of-view fluorescence imaging for organ-level lineage tracing of rare intestinal stem cell populations

Noelle Daigle; Suzann Duan; Heyu Song; Natzem Lima; Ricky Sontz; Juanita L Merchant; Travis W Sawyer

doi:10.1117/1.JBO.28.9.096004

Wide field-of-view fluorescence imaging for organ-level lineage tracing of rare intestinal stem cell populations

J Biomed Opt. 2023 Sep;28(9):096004. doi: 10.1117/1.JBO.28.9.096004. Epub 2023 Sep 13.

Authors

Noelle Daigle¹, Suzann Duan², Heyu Song², Natzem Lima¹, Ricky Sontz², Juanita L Merchant², Travis W Sawyer^{1

2}

Affiliations

¹ University of Arizona, Wyant College of Optical Sciences, Tucson, Arizona, United States.
² University of Arizona, College of Medicine, Tucson, Arizona, United States.

Abstract

Significance: Lineage tracing using fluorescent reporters is a common tool for monitoring the expression of genes and transcription factors in stem cell populations and their progeny. The zinc-binding protein 89 (ZBP-89/Zfp148 mouse gene) is a transcription factor that plays a role in gastrointestinal (GI) stem cell maintenance and cellular differentiation and has been linked to the progression of colon cancer. While lineage tracing is a useful tool, it is commonly performed with high-magnification microscopy on a small field of view within tissue sections, thereby limiting the ability to resolve reporter expression at the organ level. Furthermore, this technique requires extensive tissue processing, which is time consuming and requires euthanizing the animal. Further knowledge could be elucidated by measuring the expression of fluorescent reporters across entire organs with minimal tissue processing.

Aim: We present the application of wide-field fluorescence imaging for whole-organ lineage tracing of an inducible Zfp148-tdTomato-expressing transgenic mouse line to assess the expression of ZBP-89/Zfp148 in the GI tract.

Approach: We measured tdTomato fluorescence in ex vivo organs at time points between 24 h and 6 months post-induction. Fluctuations in tdTomato expression were validated by fluorescence microscopy of tissue sections.

Results: Quantification of the wide field-of-view images showed a statistically significant increase in fluorescent signal across the GI tract between transgenic mice and littermate controls. The results also showed a gradient of decreasing reporter expression from proximal to distal intestine, suggesting a higher abundance of ZBP-89 expressing stem cells, or higher expression of ZBP-89 within the stem cells, in the proximal intestine.

Conclusions: We demonstrate that wide-field fluorescence imaging is a valuable tool for monitoring whole-organ expression of fluorescent reporters. This technique could potentially be applied in vivo for longitudinal assessment of a single animal, further enhancing our ability to resolve rare stem cell lineages spatially and temporally.

Keywords: ZBP-89; Zfp148; fluorescence imaging; lineage tracing.

Publication types

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

MeSH terms

Animals
Colonic Neoplasms*
Coloring Agents
DNA-Binding Proteins
Intestines* / diagnostic imaging
Mice
Mice, Transgenic
Microscopy, Fluorescence
Optical Imaging
Transcription Factors

Substances

Coloring Agents
Zfp148 protein, mouse
DNA-Binding Proteins
Transcription Factors

Grants and funding

P30 CA023074/CA/NCI NIH HHS/United States