Abstract:Studies have shown that fibroblast growth factor (Fgf ) signalling is necessary for appendage regeneration, but its exact function and the ligands involved during regeneration have not yet been elucidated. Here, we performed comprehensive expression analyses and identified fgf20a and fgf3/10a as major Fgf ligands in the wound epidermis and blastema, respectively. To reveal the target cells and processes of Fgf signalling, we performed a transplantation experiment of mesenchymal cells that express the dominantn… Show more
“…Compared with WT larvae, the clo larvae showed marked upregulation of regeneration-induced genes such as junba , junbb , matrix metallopeptidase 9 ( mmp9 ), fibronectin 1b ( fn1b ), and fgf20a (Yoshinari et al, 2009; Shibata et al, 2016) (Figure 1A and Supplementary file 1). In addition to these genes, expression of a group of genes including il1b and tumor necrosis factor-b ( tnfb ), which are involved in the inflammatory response, was also upregulated in the clo mutant during fin fold regeneration.…”
Section: Resultsmentioning
confidence: 99%
“…The Dex-treated larvae displayed apparent retardation of regeneration at 3 dpa (Figure 7A and B) and a statistically significant reduction in cell proliferation in the distal fin fold region (Figure 7C and D). Notably, the expression of regeneration-induced genes such as junba (Yoshinari et al, 2009) and fgf20a (Whitehead et al, 2005; Shibata et al, 2016) was downregulated in the Dex-treated larvae (Figure 7E). These data suggest that inflammation is required for activation of regeneration-induced gene expression which is a prerequisite for normal regeneration.10.7554/eLife.22716.016Figure 7.Il1b-mediated inflammation is required for normal regeneration.( A ) Fin fold regeneration in WT larvae treated with Dex.…”
Section: Resultsmentioning
confidence: 99%
“…BrdU-positive cells were significantly reduced following Dex treatment. ( E ) Detection of junba expression using ISH and fgf20a expression using the HGn21A enhancer-trap line (Shibata et al, 2016) in DMSO- or Dex-treated larvae. The expression of junba and fgf20a was also significantly downregulated following Dex treatment.…”
Cellular responses to injury are crucial for complete tissue regeneration, but their underlying processes remain incompletely elucidated. We have previously reported that myeloid-defective zebrafish mutants display apoptosis of regenerative cells during fin fold regeneration. Here, we found that the apoptosis phenotype is induced by prolonged expression of interleukin 1 beta (il1b). Myeloid cells are considered to be the principal source of Il1b, but we show that epithelial cells express il1b in response to tissue injury and initiate the inflammatory response, and that its resolution by macrophages is necessary for survival of regenerative cells. We further show that Il1b plays an essential role in normal fin fold regeneration by regulating expression of regeneration-induced genes. Our study reveals that proper levels of Il1b signaling and tissue inflammation, which are tuned by macrophages, play a crucial role in tissue regeneration.DOI:
http://dx.doi.org/10.7554/eLife.22716.001
“…Compared with WT larvae, the clo larvae showed marked upregulation of regeneration-induced genes such as junba , junbb , matrix metallopeptidase 9 ( mmp9 ), fibronectin 1b ( fn1b ), and fgf20a (Yoshinari et al, 2009; Shibata et al, 2016) (Figure 1A and Supplementary file 1). In addition to these genes, expression of a group of genes including il1b and tumor necrosis factor-b ( tnfb ), which are involved in the inflammatory response, was also upregulated in the clo mutant during fin fold regeneration.…”
Section: Resultsmentioning
confidence: 99%
“…The Dex-treated larvae displayed apparent retardation of regeneration at 3 dpa (Figure 7A and B) and a statistically significant reduction in cell proliferation in the distal fin fold region (Figure 7C and D). Notably, the expression of regeneration-induced genes such as junba (Yoshinari et al, 2009) and fgf20a (Whitehead et al, 2005; Shibata et al, 2016) was downregulated in the Dex-treated larvae (Figure 7E). These data suggest that inflammation is required for activation of regeneration-induced gene expression which is a prerequisite for normal regeneration.10.7554/eLife.22716.016Figure 7.Il1b-mediated inflammation is required for normal regeneration.( A ) Fin fold regeneration in WT larvae treated with Dex.…”
Section: Resultsmentioning
confidence: 99%
“…BrdU-positive cells were significantly reduced following Dex treatment. ( E ) Detection of junba expression using ISH and fgf20a expression using the HGn21A enhancer-trap line (Shibata et al, 2016) in DMSO- or Dex-treated larvae. The expression of junba and fgf20a was also significantly downregulated following Dex treatment.…”
Cellular responses to injury are crucial for complete tissue regeneration, but their underlying processes remain incompletely elucidated. We have previously reported that myeloid-defective zebrafish mutants display apoptosis of regenerative cells during fin fold regeneration. Here, we found that the apoptosis phenotype is induced by prolonged expression of interleukin 1 beta (il1b). Myeloid cells are considered to be the principal source of Il1b, but we show that epithelial cells express il1b in response to tissue injury and initiate the inflammatory response, and that its resolution by macrophages is necessary for survival of regenerative cells. We further show that Il1b plays an essential role in normal fin fold regeneration by regulating expression of regeneration-induced genes. Our study reveals that proper levels of Il1b signaling and tissue inflammation, which are tuned by macrophages, play a crucial role in tissue regeneration.DOI:
http://dx.doi.org/10.7554/eLife.22716.001
“…7). Since the body of a zebrafish larva is transparent through all developmental stages, such transgenic fish have been used to visualize the vascular system [108], the central and peripheral nervous systems [109, 110], the regenerating processes of the sensory system and fin [111, 112], the cellular process of muscle wound repair [113], and proteolytic cleavage of the extracellular domain of a membrane protein (Neuregulin) in the motor neurons [114], among others. Also, the transgenic fish were applied to image the activity of specific neuronal populations or endothelial cells by targeted expression of a calcium indicator GCaMP [115, 116].…”
Section: Transposons and Functional Genomicsmentioning
confidence: 99%
“…( D ) Lateral line glial cells in gSAGFF202A at 5 dpf [111]. ( E ) Caudal trunk (and the wound epidermis) in HGn21A embryo at 1 dpf [112]. ( F ) Fgf7b-positive muscle cells in gSAIzGFFD164A at 1 dpf [113].…”
Genetic tools and mutagenesis strategies based on transposable elements are currently under development with a vision to link primary DNA sequence information to gene functions in vertebrate models. By virtue of their inherent capacity to insert into DNA, transposons can be developed into powerful tools for chromosomal manipulations. Transposon-based forward mutagenesis screens have numerous advantages including high throughput, easy identification of mutated alleles and providing insight into genetic networks and pathways based on phenotypes. For example, the Sleeping Beauty transposon has become highly instrumental to induce tumors in experimental animals in a tissue-specific manner with the aim of uncovering the genetic basis of diverse cancers. Here, we describe a battery of mutagenic cassettes that can be applied in conjunction with transposon vectors to mutagenize genes, and highlight versatile experimental strategies for the generation of engineered chromosomes for loss-of-function as well as gain-of-function mutagenesis for functional gene annotation in vertebrate models, including zebrafish, mice and rats.
Background: Matrix metalloproteinases 13 (MMP13) is a potent endopeptidase that regulate cell growth, migration, and extracellular matrix remodeling. However, its role in fin regeneration remains unclear. Results: mmp13a expression is strongly upregulated during blastema formation and persists in the distal blastema. mmp13a knockdown via morpholino electroporation impairs regenerative outgrowth by decreasing cell proliferation, which correlates with a downregulation of fgf10a and sall4 expression in the blastema.Laminin distribution in the basement membrane is also affected in mmp13a MOinjected rays. Another impact of mmp13a knockdown is observed in the skeletal elements of the fin rays. Expression of two main components of actinotrichia, Collagen II and Actinodin 1 is highly reduced in mmp13a MO-injected rays leading to highly disorganized actinotrichia pattern. Inhibition of mmp13a strongly affects bone formation as shown by a reduction of Zns5 and sp7 expression and of bone matrix mineralization in rays. These defects are accompanied by a significant increase in apoptosis in mmp13a MO-injected fin regenerates. Conclusion: Defects of expression of this multifunctional proteinase drastically affects osteoblast differentiation, bone and actinotrichia formation as well as Laminin distribution in the basement membrane of the fin regenerate, suggesting the important role of Mmp13 during the regenerative process.
K E Y W O R D Sactinotrichia, blastema, fin regeneration, mmp13a, morpholino knockdown, osteoblast differentiation
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