Schematic drawing of alternatively-spliced GFP reporter gene.

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Schematic drawing of alternatively-spliced GFP reporter gene. Schematic drawing of alternatively-spliced GFP reporter gene. Top: The T-DNA original construct introduced into Arabidopsis contained a GFP reporter gene under the transcriptional control of a minimal promoter (TATA) and upstream viral (EPRV) enhancer element. However, analysis of the wild-type T line revealed that neither the minimal promoter nor the downstream ATG initiation codon (gray letters) is used. Bottom: The T line analysis indicated that transcription of GFP pre-mRNA initiates at an upstream promoter (black bar and arrow) to generate three alternative splice variants that comprise part of the enhancer region (Kanno et al. 2008). These variants include a long unspliced transcript, a middle-length transcript arising from splicing of a canonical GT-AG intron, and a short transcript resulting from splicing a U2-type intron with non-canonical AT-AC splice sites, which are generally considered inefficient splice sites (Crotti et al. 2007). Because the unspliced and GU-AG transcripts contain a number of premature termination codons (blue asterisks), only the AU-AC transcript can be translated into GFP protein. The actual coding sequence of GFP protein (green bars) contains a unique 27 amino acid extension (short stippled green bars) relative to standard GFP (Fu et al. 2015; Kanno et al. 2016). Arrowheads designate a short tandem repeat upstream of the promoter. The black AUG denotes the major translation initiation codon. The distance between the 3′ splice sites for the GT-AG and AT-AC introns is only 3 nt; the non-canonical AC is on the outside (Kanno et al. 2016, 2017a,b). Tatsuo Kanno et al. G3 2018;8:1367-1377 ©2018 by Genetics Society of America