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Intravital 2-photon imaging of leukocyte trafficking in beating heart
Wenjun Li, … , Mark J. Miller, Daniel Kreisel
Wenjun Li, … , Mark J. Miller, Daniel Kreisel
Published June 18, 2012
Citation Information: J Clin Invest. 2012;122(7):2499-2508. https://doi.org/10.1172/JCI62970.
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Technical Advance Cardiology

Intravital 2-photon imaging of leukocyte trafficking in beating heart

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Abstract

Two-photon intravital microscopy has substantially broadened our understanding of tissue- and organ-specific differences in the regulation of inflammatory responses. However, little is known about the dynamic regulation of leukocyte recruitment into inflamed heart tissue, largely due to technical difficulties inherent in imaging moving tissue. Here, we report a method for imaging beating murine hearts using intravital 2-photon microscopy. Using this method, we visualized neutrophil trafficking at baseline and during inflammation. Ischemia reperfusion injury induced by transplantation or transient coronary artery ligation led to recruitment of neutrophils to the heart, their extravasation from coronary veins, and infiltration of the myocardium where they formed large clusters. Grafting hearts containing mutant ICAM-1, a ligand important for neutrophil recruitment, reduced the crawling velocities of neutrophils within vessels, and markedly inhibited their extravasation. Similar impairment was seen with the inhibition of Mac-1, a receptor for ICAM-1. Blockade of LFA-1, another ICAM-1 receptor, prevented neutrophil adherence to endothelium and extravasation in heart grafts. As inflammatory responses in the heart are of great relevance to public health, this imaging approach holds promise for studying cardiac-specific mechanisms of leukocyte recruitment and identifying novel therapeutic targets for treating heart disease.

Authors

Wenjun Li, Ruben G. Nava, Alejandro C. Bribriesco, Bernd H. Zinselmeyer, Jessica H. Spahn, Andrew E. Gelman, Alexander S. Krupnick, Mark J. Miller, Daniel Kreisel

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Figure 1

2P microscopy of neutrophils in explanted heart at steady state and after heterotopic heart transplantation.

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2P microscopy of neutrophils in explanted heart at steady state and afte...
(A) Myocardial tissue with resident neutrophils (green cells, white box) and macrophages (green cells, yellow box). Nontargeted Q-dots were injected intravenously 10 minutes before imaging to label the blood vessels (red). Scale bar: 60 μm. (B and C) Zoomed views from panel A showing (B) an intravascular neutrophil (white arrowhead) and (C) a macrophage (yellow arrowhead). These cells can be distinguished by morphology and fluorescence intensity. Scale bar: 10 μm. (D) Time-lapse images of neutrophils in explanted heart tissue after heterotopic cardiac transplantation into B6 LysM-GFP mice. Images are individual frames from a continuous time-lapse recording (Supplemental Video 1). Relative time is displayed in h:min:s. Lower panels are zoomed views from the boxed regions. Neutrophils were found adhering to the endothelium (yellow arrowhead) or crawling along it. Extravascular neutrophils (white arrowheads) formed dynamic clusters (white arrows) over minutes. Scale bars: 60 μm (upper panels); 20 μm (lower panels). Data are representative of at least 3 independent experiments per group.

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ISSN: 0021-9738 (print), 1558-8238 (online)

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