FIGURE

Fig. 7

ID
ZDB-FIG-220415-11
Publication
Wen et al., 2021 - Fxr signaling and microbial metabolism of bile salts in the zebrafish intestine
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Fig. 7

Fxr regulates differentiation and functions of anterior absorptive enterocytes in zebrafish.(A) FACS analysis comparing the relative abundance of anterior enterocytes in 7-dpf fxr+/+ and fxr−/− larvae expressing the Tg(-4.5fabp2:DsRed) and TgBAC(cldn15la-GFP) transgenes. The relative abundance was calculated by dividing the cell counts of DsRed+GFP+ double-positive cells by the cell counts of GFP+ single-positive cells (mean ± SEM). Statistical significance was calculated by unpaired t test. Representative data from two independent experiments are shown. (B) Comparisons between the genes that were differentially expressed in fxr−/− cells relative to fxr+/+ cells in cluster 4 and the mouse genes enriched in jejunal enterocytes/intestinal stem cells (ISCs) (49). Left: Venn diagram showing the number of overlapped genes between the two gene sets, of which the differentially expressed genes in fxr−/− cells were further classified based on the changes in their expression (up- or down-regulated) upon fxr mutation. Middle: Distributions of enterocyte- and ISC-enriched genes from the enterocyte/ISC dataset used in the current comparison. Right: Distribution of overlapped genes resulting from the comparison. (C) Top 3 HOMER-identified motifs enriched within accessible chromatin regions near genes that were down-regulated in the fxr−/− cells relative to fxr+/+ cells in cluster 4. The position weight matrices (PWMs) of the enriched nucleotide sequences are shown. The TF family that most closely matches the motif is indicated above the PWM.

Expression Data

Expression Detail
Antibody Labeling
Phenotype Data

Phenotype Detail
Acknowledgments
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