def+/- liver suffers from haploinsufficiency of Def.

(A) qPCR analysis of def transcripts in adult wild-type and def+/- liver. The expression of def was normalised against elf1a and is shown as the fold change in expression, with the value from def+/- being set at 1. The values plotted represent the means ± standard errors of the mean. (B) Western blotting analysis of the Def protein. Bhmt: loading control. Densitometry was performed using Photoshop. The value of Def was obtained by normalising against Bhmt expression. The relative value of Def protein in def+/- was set at 1. (C) Representative images of immunostaining of Def (red) in wild-type and def+/- liver 2 days after PH. lv, liver tissue. Scale bar: 100 μm (C).

EXPRESSION / LABELING:
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Stage: Adult

The liver-to-body ratio of the regenerated livers did not differ significantly between the wild-type and def+/- mutant fish after PH.

(A) Liver-to-body ratio of the wild-type sham control and amputated wild-type liver at 3, 7 and 36 days after PH (ne5). (B) Liver-to-body ratios of the sham controls (n≥5) for the wild-type and def+/- mutant fish. (C–F) Comparison of the liver-to-body ratios of the amputated wild-type and def+/- livers 3 days after PH (C), 7 days after PH (D), 14 days after PH (E) and 30 days after PH (F) as indicated (n≥5 in each case). NS: not significant; *: p<0.05. (G) Representative images of haematoxylin-eosin staining of sections across the wild-type or def+/- hepatic parenchyma without performing PH or 9 months after PH. Scale bar: 50 μm.

Def haploinsufficiency results in a failure in the remodelling of the wound epidermis to liver tissue.

(A) Ventral view of the gross morphology of an amputated adult wild-type and def+/-liver 7 days after PH. The dotted white line indicates the amputation site. 1: ventral lobe, 2: left dorsal lobe, 3: right dorsal lobe. (B–D) Representative images of co-immunostaining of PCNA and Bhmt to compare the process of epithelialisation of the amputation site 2 days after PH (B), wound epidermis formation 3 days after PH (C), and wound epidermis remodelling 5.5 days after PH (D) between the wild-type and the def+/- mutant. Nuclei were stained with 4′,6-diamidino-2-phenylindole (DAPI) (blue). In each case or at each time-point, more than 10 sections from at least three wild-type or def+/- mutant fish were examined. bc, blood clot; lv, liver tissue; we, wound epidermis. Scale bar: 5 mm (A) and 75 μm (B–D).

Def haploinsufficiency results in accumulation of ColI at the amputation site after PH.

(A,B) Representative images of immunostaining of keratin 18 (green) (A) and co-immunostaining of ColI (red) and Bhmt (green) (B) at the amputation site in wild-type and def+/- strains 3 days after PH. Nuclei were stained with DAPI (blue). At each time-point, more than 10 sections from at least three wild-type or def+/- mutant fish were examined. lv, liver tissue; we, wound epidermis. Scale bars: 75 μm (A,B) and 100 μm (C).

Def haploinsufficiency results in the formation of a fibrotic scar at the amputation site after PH.

Masson staining of sections across the amputation site 3 (A), 5.5 (B) and 30 (C) days after PH (dPH), respectively. Fibrotic tissue was stained in blue (highlighted with an asterisk), cytoplasm in light red and nuclei in dark brown. Green, dashed lines outline the amputation site. Scale bar: 100 μm.

Constitutive activation of TGFβ signalling promotes ColI deposition at the amputation site in def+/- fish after PH.

(A–D) Representative images of immunostaining of pSmad2 (red) and Bhmt (green) in wound epidermis in wild-type (A), def+/- (B), def+/- treated with SB431542 (C) or def+/-treated with Dex (D) 1.5, 3 and 5 days after PH, respectively. (E,F) Representative images of immunostaining of ColI (red) and Bhmt (green) in the wound epidermis in wild-type and def+/-fish treated or not treated with SB431542 (E) or Dex (F) 5 days after PH, respectively. Nuclei were stained with DAPI (blue). In each case, more than 10 sections from at least three wild-type or def+/- mutant fish were examined. bc, blood clot; lv, liver tissue; we, wound epidermis. Scale bar:75 μm (A–F).

def+/- mutant liver exhibited a prolonged inflammatory reaction at the amputation site after PH.

(A) qPCR analysis of cytokine genes TNFα, IL-1β, IL-6 and IL-8 in adult wild-type, def+/-, fabp10a:def+/- and def+/- p53M214K/M214K livers prior to the surgical procedure. Gene expression is expressed as the fold change after normalisation against β-actin. The value for each gene in the wild-type was set at 1. The p value represents the statistical differences between def+/- and another corresponding group. *: p<0.05, **: p<0.01, NS: not significant. (B–D) Adult fish of Tg(zlyz:EGFP) in a wild-type and def+/- background were subjected to PH, and collected 6 h after PH (B), 12 h after PH (C) and 36 h after PH (D) for EGFP fluorescence imaging. Images were taken from the region outlined in white in the corresponding bright field picture shown on the left. The region above the dashed magenta lines is the liver tissue adjacent to the amputation site. Black asterisks highlight the EGFP signal yielded possibly from neutrophils in the intestine. A representative image is shown for each time-point. bc, blood clot; in, intestine; lv, liver tissue. Scale bar: 5 mm (bright field) and 2 mm (GFP field).

Def haploinsufficiency caused an altered migration behaviour of leukocytes in def+/- fish that was rescued by treatment with Dex or ectopic expression of Def in hepatocytes.

(A–H) Representative images of co-immunostaining of EGFP (green, label macrophage), dsRed (yellow, label neutrophil) and Bhmt (red) in the wound epidermis in wild-type (A,B), def+/- (C,D), def+/- treated with Dex (E,F) and def+/-Tg(fabp10a:def) progeny (G,H) 12 and 36 h after PH, respectively. All are in the background of Tg(coro1a:eGFP;lyz:dsRED). Nuclei were stained with DAPI (blue). In each case, more than 10 sections from at least three wild-type or def+/- mutant fish were examined. bc, blood clot; lv, liver tissue. Scale bars: 150 μm (A–H).

Formation of the fibrotic scar in def+/- fish after PH was mediated by the activation of the p53-pathway.

(A) Immunostaining of pSmad2 (red) and Bhmt (green) in the wound dermis in def+/-Tg(fabp10:def)+/- progeny 1.5, 3 and 5 days after PH, respectively. (B) Immunostaining of ColI (red) and Bhmt (green) in the wild-type, def+/- and def+/-Tg(fabp10:def)+/- progeny 5 days after PH. (C) Masson staining of the amputation site (indicated by a green dashed line) in the wild-type, def+/- and def+/- Tg(fabp10:def)+/- progeny 14 days after PH. (D,E) Immunostaining of pSmad2 (red) and Bhmt (green) (D) and of ColI (red) and Bhmt (green) (E) in the wound epidermis in the wild-type, def+/- and def+/-p53M214K/M214K 5 days after PH. (F) Masson staining of the amputation site in the wild-type, def+/- and def+/-p53M214K/M214K progeny 14 days after PH. Fibrotic tissue in the def+/- fish is highlighted by a red asterisk. In (A,B,D,E), nuclei were stained with DAPI (blue). In each case, more than 10 sections from at least three wild-type or def+/- mutant fish were examined. Representative images are shown here. bc, blood clot; lv, liver tissue; we, wound epidermis. Scale bars: 150 μm (C,F) and 75 μm (A,B,D,E).

A model to explain how Def haploinsufficiency activates the p53-dependent inflammation-mediated TGFβ signalling and causes fibrotic scar formation in def+/- after PH.

(A) Western blot of HMGB1 in the adult liver from wild-type, def+/-, def+/-Tg(fabp10:def)+/- and def+/-p53M214K/M214K fish. Loading control: Bhmt. (B) Immunostaining of ColI and Bhmt in the wound epidermis in wild-type, def+/- and def+/-fish treated with 100 &mu;M of glycyrrhizic acid ammonium 5 days after PH. lv, liver; we, wound epidermis. (C) In a wild-type liver, Def complexes with Capn3 to mediate p53 degradation in the nucleoli to mitigate the inflammatory response after acute injury. In def+/- fish, the activity of the Def-Capn3 protein degradation pathway is compromised and p53 protein is thus stabilised, which in turn activates the p53 pathway. Constant activation of the p53 pathway up-regulates the expression of the pro-inflammatory factor HMGB1 that up-regulates the expression of cytokines (e.g., TNFα, IL-1β, IL-6 and IL-8) and other signalling pathways that lead to a prolonged inflammatory response in def+/-. The prolonged inflammatory response activates TGFβ signalling and causes the over-production of fibrotic molecules (e.g., collagens, elastin and fibronectin) in the wound epidermis that finally forms a fibrotic scar at the amputation site in def+/-. Fibrotic scar formation in def+/- can be blocked by over-expressing Def specifically in the hepatocytes, by the loss of function of p53, and by treatment with Dex (anti-inflammatory drug), SB431542 (inhibitor of TGFβ signalling) or glycyrrhizic acid ammonium (inhibitor of HMGB1 function).

The def+/- mutant showed defective lobe structure recovery at the amputation site after PH. Lower magnifications of the ventral and lateral views of the gross morphology of the liver 3, 7 and 21 days after PH. The images for 7 days after PH correspond to the closer view of the amputation site shown in Figure 1d. The white, dashed line outlines the amputation site on the ventral tip. The red arrow highlights the ventral lobe in the sham control. VL: ventral lobe; LDL: left dorsal lobe; RDL: right dorsal lobe. Scale bar: 1 cm.

Comparison of the wound healing process between the wild-type and def+/- livers after PH. Frontal plane sections of the liver 12, 24 and 36 h after PH were stained for apoptotic cells (in white, using the TUNEL assay), proliferative cells (in red, by EdU incorporation) together with Bhmt (hepatocyte marker) (in green). DAPI was used to stain the nuclei (blue). All images show the part of the hepatic tissue adjacent to the amputation site. Yellow dashed lines outline the amputation site, while regions defined by red brackets represent the blood clot. (A–D) The blood clot was clearly formed in both the wild-type (A) and def+/- mutant (B) fish 12 h after PH. Cells in the blood clot underwent massive apoptosis 24 h after PH (C,D). (E,F) By 36 h after PH, the blood clot was detached from the liver mass in the wild-type fish (E), whereas it was still connected to the liver mass in the def+/- mutant (F). The inset, enlarged view corresponds to the amputation site (A–F). bc, blood clot; lv, liver tissue. Scale bar: 250 μm (A–F).

Comparison of cell proliferation in the adult liver in the wild-type and def+/- sham controls. Representative images of immunostaining of PCNA (in red) in the Tg(fabp10a:RFP) background, in which hepatocytes are genetically labelled by expressing the red fluorescent protein (in green), showed that proliferating cells were rarely detected along the epithelial edge of an adult liver in either the wild-type or def+/- mutant sham controls. Nuclei were stained with DAPI (blue). lv, liver tissue. Scale bar: 75 μm.

ColI deposition at the amputation site in def+/- is not mediated by the reactive oxygen species signalling pathway. Representative images of co-immunostaining of ColI (red) and Bhmt (green) in the wound epidermis in wild-type, def+/- and def+/- fish treated with diphenyleneiodonium (DPI) or apocynin (APO), two inhibitors of the reactive oxygen species signalling, 5 days after PH. Nuclei were stained with DAPI (blue). lv, liver tissue; we, wound epidermis. Scale bar: 75 μm.

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