2005
DOI: 10.1007/s10038-005-0261-9
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Frequent occurrence of protein isoforms with or without a single amino acid residue by subtle alternative splicing: the case of Gln in DRPLA affects subcellular localization of the products

Abstract: Protein isoforms with or without a single amino acid residue make a subtle difference. It has been documented on a few genes that alternative splicing generated such isoforms; however, the fact has attracted little attention. We became aware of a subtle sequence difference in DRPLA, a polyglutamine disease gene for dentatorubral pallidoluysian atrophy. Some reported cDNA sequences lacked 3 nucleotides (nt) (CAG), which were positioned apart from the expandable and polymorphic CAG repeats and also coded for glu… Show more

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Cited by 69 publications
(90 citation statements)
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References 39 publications
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“…The N terminus fragment of AR99Q, was amplified by PCR using primers BglII-AR-Fw and SalI-AR-396Rv (AAAAAAGT-CGACGACGCAACCTCTCTCGGGGT), cleaved by BglII and SalI, and subcloned into the BglII-SalI sites of the pEGFP-C1. EGFP-DRPLA construct encoding atrophin-1 with Gln-71 was described previously (39) and was kindly provided by Dr. Masao Yamada. To prepare pcDNA3.1-tNhtt-60Q-EGFP for transient transfection, tNhtt-polyQ-EGFP fragment was cut from pINDtNhtt-polyQ-EGFP (40) with HindIII-XbaI digestion, and the resulting fragment was inserted into pcDNA3.1-v5/His plasmid.…”
Section: Methodsmentioning
confidence: 99%
“…The N terminus fragment of AR99Q, was amplified by PCR using primers BglII-AR-Fw and SalI-AR-396Rv (AAAAAAGT-CGACGACGCAACCTCTCTCGGGGT), cleaved by BglII and SalI, and subcloned into the BglII-SalI sites of the pEGFP-C1. EGFP-DRPLA construct encoding atrophin-1 with Gln-71 was described previously (39) and was kindly provided by Dr. Masao Yamada. To prepare pcDNA3.1-tNhtt-60Q-EGFP for transient transfection, tNhtt-polyQ-EGFP fragment was cut from pINDtNhtt-polyQ-EGFP (40) with HindIII-XbaI digestion, and the resulting fragment was inserted into pcDNA3.1-v5/His plasmid.…”
Section: Methodsmentioning
confidence: 99%
“…Apart from experimental investigations (Condorelli et al 1994;Vogan et al 1996; Burgar et al 2002;Tadokoro et al 2005), another approach to address this question is to estimate the fraction of tandem sites under purifying selection. Here, we show that the sequence conservation level differs between tandem motifs due to constraints on the splice site consensus and possibly on splicing enhancer motifs as well as on the coding sequence.…”
Section: Discussionmentioning
confidence: 99%
“…Although tissue-or cell-line-specific splicing has been observed at tandem acceptors (Koenig Merediz et al 2000;Hiller et al 2004;Xu et al 2004;Tadokoro et al 2005) and tandem donors (Hu et al 1999;Yan et al 2000), stochastic selection of either of the two splice sites likely explains alternative splicing at most tandems (Chern et al 2006). Stochastic splice events are expected to yield similar splice variant ratios in different tissues, and this was observed in many cases (Vogan et al 1996;Hammes et al 2001;Burgar et al 2002;Tadokoro et al 2005;Hiller et al 2006b).…”
Section: Discussionmentioning
confidence: 99%
“…Many of these sites are 3 nucleotides apart and result in inclusion or exclusion of a single codon. There is debate about the nature of splicing regulation at these sites 5,6 with some arguing that the splicing motif differences are so subtle that selection is stochastic 7 , while others infer regulation based on tissue specificity 8 .…”
Section: Introductionmentioning
confidence: 99%
“…Tandem splice site selection has been analyzed semi-quantitatively using modified capillary electrophoresis 7 , and high-resolution gel electrophoresis 8 . RNA-Seq (RNA sequencing) reads can be used to quantify the splicing ratios at each splice site.…”
Section: Introductionmentioning
confidence: 99%