The zebrafish is an excellent genetic system for the study of vertebrate development and disease. In an effort to provide a rapid and robust tool for zebrafish gene mapping, a panel of radiation hybrids (RH) was produced by fusion of irradiated zebrafish AB9 cells with mouse B78 cells. The overall retention of zebrafish sequences in the 93 RH cell lines that constitute the LN54 panel is 22%. Characterization of the LN54 panel with 849 simple sequence length polymorphism markers, 84 cloned genes and 122 expressed sequence tags allowed the production of an RH map whose total size was 11,501 centiRays. From this value, we estimated the average breakpoint frequency of the LN54 RH panel to correspond to 1 centiRay ؍ 148 kilobase. Placement of a group of 235 unbiased markers on the RH map suggests that the map generated for the LN54 panel, at present, covers 88% of the zebrafish genome. Comparison of marker positions in RH and meiotic maps indicated a 96% concordance. Mapping expressed sequence tags and cloned genes by using the LN54 panel should prove to be a valuable method for the identification of candidate genes for specific mutations in zebrafish.Somatic-cell hybrids and radiation hybrids (RHs) have played a key role in the mapping of human and mouse genes (1-7). Cell hybrids constitute one of the most expedient methods for assigning genes to chromosomes or chromosome segments, because mapping with cell hybrids does not require gene polymorphism. RHs are generated by irradiating cells from a donor species, causing random chromosomal breaks, and fusing these to a cell line from a different species. Donor-cell chromosome fragments are retained to different extents in the ensuing hybrid cells. Typing a panel of RHs with PCR-based sequence-tagged sites creates an RH map in which the frequency of breakpoints between two markers is proportional to the distance between them.The large collection of mutations produced in the zebrafish constitutes a valuable resource for the study of vertebrate developmental mechanisms (8-10). The efficient identification of the genes disrupted by mutation in zebrafish requires dense maps of the genome. Meiotic maps based on rapidamplified polymorphic DNA sequences and microsatellite markers have been produced (11-16). Since localization of cDNAs and expressed sequence tags (ESTs) on meiotic maps requires the identification of polymorphisms, the use of RH mapping is a valuable complementary method suitable for high-throughput cDNA/EST mapping projects to identify candidate genes for available mutants.We have previously shown that stable transfer of zebrafish chromosomes or chromosome segments to a rodent cell line was possible (17). Markers from the simple sequence-length polymorphism (SSLP) meiotic map could be anchored on a panel of zebrafish/mouse somatic-cell hybrids (14). Furthermore, Kwok et al. (18) demonstrated that RH technology could be used for nonmammalian vertebrates. In the present study, we report characterization of LN54, a zebrafish RH panel composed of 93 cell...
Amputation of the zebrafish caudal fin stimulates regeneration of the dermal skeleton and reexpression of sonic hedgehog (shh)-signaling pathway genes. Expression patterns suggest a role for shh signaling in the secretion and patterning of the regenerating dermal bone, but a direct role has not been demonstrated. We established an in vivo method of gene transfection to express ectopically genes in the blastema of regenerating fins. Ectopic expression of shh or bmp2 in the blastema-induced excess bone deposition and altered patterning of the regenerate. The effects of shh ectopic expression could be antagonized by ectopic expression of chordin, an inhibitor of bone morphogenetic protein (bmp) signaling. We disrupted shh signaling in the regenerating fin by exposure to cyclopamine and found a dose-dependent inhibition of fin outgrowth, accumulation of melanocytes in the distal region of each fin ray, loss of actinotrichia, and reduction in cell proliferation in the mesenchyme. Morphological changes were accompanied by an expansion, followed by a reduction, in domains of shh expression and a rapid abolition of ptc1 expression. These results implicate shh and bmp2b signaling in the proliferation and͞or differentiation of specialized bone-secreting cells in the blastema and suggest shh expression may be controlled by regulatory feedback mechanisms that define the region of bone secretion in the outgrowing fin.T he extent of regenerative capacity varies between species and tissue types. Analysis of the regenerative events is not only informative in its own right but may also provide information pertaining to earlier morphogenetic events, because regeneration often recapitulates development. An example of this is the dermal skeleton component of the zebrafish (Danio rerio) caudal fin, which regenerates rapidly after amputation by processes reminiscent of those occurring during larval stages (for review, see ref. 1), including reexpression of developmental genes (2-6).The dermal skeleton of the zebrafish fin comprises mineralized lepidotrichia (fin rays) and more distal collagenous actinotrichia (Fig. 1A). The lepidotrichia are composed of two segmented hemirays that bifurcate periodically along their proximal-distal axis forming sister-ray branches. After amputation, epithelial cells migrate from the stump to cover the wound region (7, 8), beneath which a blastema containing undifferentiated proliferative mesenchymal cells forms (1). Scleroblasts then differentiate within the blastema at the epithelial͞mesenchymal interface and begin to secrete the matrix that will form the new dermal bone.During regeneration, the signaling molecule sonic hedgehog (shh) involved in patterning of many structures (reviewed in ref. 9), its membrane-receptor patched1 (ptc1) (9), and bone morphogenetic protein 2b (bmp2b), a member of the transforming growth factor- family (10), are all initially reexpressed in a single domain at the distal stump of the amputated ray. Expression is found in a subset of cells in the basal layer of the epider...
SummaryThe combination of an E2 ubiquitin-conjugating enzyme with an E3 ubiquitin-ligase is essential for ubiquitin modification of a substrate. Moreover, the pairing dictates both the substrate choice and the modification type. The molecular details of generic E3-E2 interactions are well established. Nevertheless, the determinants of selective, specific E3-E2 recognition are not understood. There are ∼40 E2s and ∼600 E3s giving rise to a possible ∼24,000 E3-E2 pairs. Using the Fanconi Anemia pathway exclusive E3-E2 pair, FANCL-Ube2T, we report the atomic structure of the FANCL RING-Ube2T complex, revealing a specific and extensive network of additional electrostatic and hydrophobic interactions. Furthermore, we show that these specific interactions are required for selection of Ube2T over other E2s by FANCL.
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