Low-frequency RNA-Seq exon junction(s) not annotated.
Annotated transcripts do not represent all supported alternative splices within 5' UTR.
Gene model reviewed during 5.46
Gene model reviewed during 6.03
Click to get a list of regulatory features (enhancers, TFBS, etc.) and gene disruptions (point mutations, indels, etc.) within or overlapping Dmel\RpL26 using the Feature Mapper tool.
GBrowse - Visual display of RNA-Seq signalsView Dmel\RpL26 in GBrowse 2
Please Note This section lists cDNAs and ESTs that fall within the genomic extent of the gene model, which may include cDNAs and ESTs of genes within introns, or of overlapping genes. Please see GBrowse for alignment of the cDNAs and ESTs to the gene model.
For each fully sequenced cDNA the DGRC maintains various forms of the cDNA (e.g tagged or untagged) in several different host vectors for subsequent cloning and expression in Drosophila and Drosophila cell lines.
Two observations suggest that RpL26 is haplolethal or haplosterile. First, we know of no deletion that has ever been reported for this region. Second, three attempts to generate a deletion for this region using FLP-mediated recombination between FRT-bearing transposon insertions failed during the work described in Cook et al. (FBrf0219066). By the criteria outlined in Marygold et al. (FBrf0205398), we categorize RpL26 as a "likely Minute" gene.
RNAi screen using dsRNA made from templates generated with primers directed against this gene results in aberrantly short, monopolar spindles when assayed in S2 cells. This phenotype can be observed when the screen is performed with or without Cdc27 dsRNA.
RNAi generated by PCR using primers directed to this gene causes a cell growth and viability phenotype when assayed in Kc167 and S2R+ cells.