In vivo recognition of a vertebrate mini-exon as an exon-intron-exon unit.

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Mol Cell Biol. 1993 May; 13(5): 2677-2687

In vivo recognition of a vertebrate mini-exon as an exon-intron-exon unit.

D A Sterner and S M Berget

Verna and Marrs McClean Department of Biochemistry, Baylor College of Medicine, Houston, Texas 77030.

ABSTRACT

Very small vertebrate exons are problematic for RNA splicingbecause of the proximity of their 3' and 5' splice sites. Inthis study, we investigated the recognition of a constitutive7-nucleotide mini-exon from the troponin I gene that residesquite close to the adjacent upstream exon. The mini-exon failedto be included in spliced RNA when placed in a heterologousgene unless accompanied by the upstream exon. The requirementfor the upstream exon disappeared when the mini-exon was internallyexpanded, suggesting that the splice sites bordering the mini-exonare compatible with those of other constitutive vertebrate exonsand that the small size of the exon impaired inclusion. Mutationof the 5' splice site of the natural upstream exon did not resultin either exon skipping or activation of a cryptic 5' splicesite, the normal vertebrate phenotypes for such mutants. Instead,a spliced RNA accumulated that still contained the upstreamintron. In vitro, the mini-exon failed to assemble into spliceosomecomplexes unless either internally expanded or accompanied bythe upstream exon. Thus, impaired usage of the mini-exon invivo was accompanied by impaired recognition in vitro, and recognitionof the mini-exon was facilitated by the presence of the upstreamexon in vivo and in vitro. Cumulatively, the atypical in vivoand in vitro properties of the troponin exons suggest a mechanismfor the recognition of this mini-exon in which initial recognitionof an exon-intron-exon unit is followed by subsequent recognitionof the intron.

Mol Cell Biol. 1993 May; 13(5): 2677-2687

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