Figure 3
- ID
- ZDB-FIG-210927-41
- Publication
- Wilson et al., 2021 - Imaging cytoplasmic lipid droplets in vivo with fluorescent perilipin 2 and perilipin 3 knock-in zebrafish
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(A) Lateral views of the anterior intestine in unfed larvae and in larvae at different time-points following the start of feeding with a high-fat meal for 1 hr. Fish were heterozygous for both Fus(plin3-RFP) and Fus(EGFP-plin2). Images are representative of three independent experiments (15–25 fish per experiment); data presented are from one experiment. Scale = 50 µm. (B) Higher magnification micrographs of lipid droplets highlight the transition from Plin3-RFP to EGFP-Plin2 on the surface of lipid droplets over time after a high-fat meal. Scale = 10 µm. (C) Manders’ colocalization coefficients for a subset of images was quantified following Costes method for automatic thresholding. Mean ± SD, n = 4 fish per time-point.
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Stage: | Day 6 |
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Stage: | Day 6 |