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A Second Leaky Splice-Site Mutation in the Spastin Gene

2001; Elsevier BV; Volume: 69; Issue: 6 Linguagem: Inglês

10.1086/324593

1537-6605

Ingrid K. Svenson, Allison E. Ashley‐Koch, Margaret A. Pericak‐Vance, Douglas A. Marchuk,

Neurogenetic and Muscular Disorders Research

To the Editor: Mutations in the gene encoding spastin, an ATPase of unknown function, cause the most common form of autosomal dominant hereditary spastic paraplegia (SPG4 [MIM 182601]; Hazan et al. Hazan et al., 1999Hazan J Fonknechten N Mavel D Paternotte C Samson D Artiguenave F Davoine C-S Cruaud D Dürr A Wincker P Brottier P Cattolico L Barbe V Burgunder J-M Prud’homme J-F Brice A Fontaine B Heilig R Weissenbach J Spastin, a new AAA protein, is altered in the most frequent form of autosomal dominant spastic paraplegia.Nat Genet. 1999; 23: 296-303Crossref PubMed Scopus (503) Google Scholar), a neurodegenerative disorder characterized by progressive spasticity of the lower limbs. Recently, we described 11 mutations in this gene, 7 of which cause missplicing of the spastin transcript (Svenson et al. Svenson et al., 2001Svenson IK Ashley-Koch AE Gaskell PC Riney TJ Cumming WJK Kingston HM Hogan EL Boustany R-MN Vance JM Nance MA Pericak-Vance MA Marchuk DA Identification and expression analysis of spastin gene mutations in hereditary spastic paraplegia.Am J Hum Genet. 2001; 68: 1077-1085Abstract Full Text Full Text PDF PubMed Scopus (107) Google Scholar). Because of the presence of a rare spastin gene–coding region polymorphism in the proband of one family with an IVS9+4a→g mutation in the spastin gene, we were able to determine that this mutation is only partially penetrant—that is, both normally and aberrantly spliced (skipped exon 9) transcripts are produced from the mutant allele. This “leakiness” of the mutation was not recapitulated in in vitro splicing experiments with minigene constructs containing only exon 9 and flanking intronic sequence. However, when we included additional sequence (exons 8–12, with flanking intronic sequence), the leakiness of the mutation was recapitulated. These findings demonstrate the importance of genomic-sequence context in the determination of splice-site selection and the extent of missplicing caused by this mutation. Because of the absence of any other spastin gene–coding region polymorphisms, we were unable to test several other splice-site mutations for leakiness by reverse-transcriptase (RT)–PCR analysis of patient-derived RNA. None of these other mutations appeared leaky in our in vitro splicing experiments with minigene constructs, even in the larger genomic-sequence context that included flanking exons. We have since found that at least one of these other splice-site mutations is, in fact, leaky in a much larger genomic-sequence context—that is, in the complete human chromosome 2 that harbors the mutation. This mutation, an IVS11+2t insertion, causes skipping of exon 11, as determined by RT-PCR analysis of patient-derived RNA (see the report by Svenson et al. [Svenson et al., 2001Svenson IK Ashley-Koch AE Gaskell PC Riney TJ Cumming WJK Kingston HM Hogan EL Boustany R-MN Vance JM Nance MA Pericak-Vance MA Marchuk DA Identification and expression analysis of spastin gene mutations in hereditary spastic paraplegia.Am J Hum Genet. 2001; 68: 1077-1085Abstract Full Text Full Text PDF PubMed Scopus (107) Google Scholar], for pedigree information and experimental data). In our in vitro splicing experiments with a minigene construct that carries this mutation as well as the complete sequence of both flanking introns and exons on each side of the skipped exon, we detected only aberrantly spliced (skipped exon 11) transcript (fig. 1A). To determine whether the presence of additional genomic-sequence context would affect the change in splice-site selection caused by this mutation, we performed RT-PCR analysis of RNA extracted from mouse-human hybrid cell lines containing either the wild-type or the mutant chromosome 2 of a patient with SPG who is heterozygous for this mutation. As shown in figure 1B, we detected both normally and aberrantly spliced transcripts in the RNA extracted from the hybrid cell line containing the mutant—but not the wild-type—chromosome 2. We confirmed through sequencing that the transcripts were derived from the human and not the mouse spastin gene. We were unable to test the other splice-site mutations for leakiness by this method, because of the lack of availability of appropriate patient-derived cell lines. These findings provide further evidence of the dependence of splice-site selection on genomic-sequence context. The exon-definition model of splice-site selection proposes that an exon is defined by the binding of splicing factors to the 3′ and 5′ splice sites of the same exon (Berget Berget, 1995Berget SM Exon recognition in vertebrate splicing.J Biol Chem. 1995; 270: 2411-2414PubMed Scopus (816) Google Scholar). Pairing of U1 small nuclear RNA (snRNA) to the 5′ splice junction includes at least six nucleotides beyond the invariant gt. The IVS11+2t insertion mutation would shift the base pairing by one nucleotide, resulting in a net loss of four base pairs relative to the pairing with the wild-type sequence. Despite this drastic alteration in U1 snRNA:hnRNA (i.e., heterogeneous nuclear RNA) pairing, this mutation, in its full genomic-sequence context, is only partially penetrant. Given these observations, we suggest that, in the case of splicing mutations outside the invariant gt–ag splice-site sequences, splice-site selection might also depend on the definition of exons and the strength of intron-exon junction sequences not directly adjacent to the mutant splice junction. In addition, splice-site selection might be influenced, in part, by intronic sequences distant from the intron-exon junctions. Although the function and normal range of expression level of spastin are still unknown, our findings reported here provide additional support for the hypothesis that the function of spastin is highly concentration dependent. Our finding that normally spliced transcript is produced from at least two different mutant alleles is consistent with the threshold of spastin required for transition from normal function to disease state lying within a narrower interval than the 50% decrease predicted by a disease model of haploinsufficiency. Thus, as we have speculated elsewhere (Svenson et al. Svenson et al., 2001Svenson IK Ashley-Koch AE Gaskell PC Riney TJ Cumming WJK Kingston HM Hogan EL Boustany R-MN Vance JM Nance MA Pericak-Vance MA Marchuk DA Identification and expression analysis of spastin gene mutations in hereditary spastic paraplegia.Am J Hum Genet. 2001; 68: 1077-1085Abstract Full Text Full Text PDF PubMed Scopus (107) Google Scholar), even slight variation in spastin expression level might have dramatic phenotypic consequences, accounting, at least in part, for the wide variability in age at onset, symptom severity, and rate of symptom progression reported to occur in SPG caused by spastin gene mutations. We thank the patients and their families for their participation. This work was supported, in part, by National Institutes of Health program project grant 2P01-NS26630-11A1.