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Literature DB >> 11105751

Deletion of a conserved dinucleotide inhibits the second step of group II intron splicing.

S Mikheeva¹, H L Murray, H Zhou, B M Turczyk, K A Jarrell.

Abstract

Few point mutations have been described that specifically inhibit the second step of group II intron splicing. Furthermore, the effects of such mutations are typically not apparent unless the mutations are studied in the context of a substrate that harbors a very short 5' exon. Truncation of the 5' exon slows the second step of splicing. Once the second step has been slowed, the effects of point mutations can be seen. We report the unexpected observation that the deletion of a conserved GA dinucleotide dramatically inhibits the second step of splicing, even when the mutation is studied in the context of a full-length substrate. In contrast, we find that this mutation does not significantly affect the first step of splicing, unless the mutation is studied in combination with a second point mutation that is known to inhibit the first step. Even in that context, the effect of the GA deletion mutation on the first step is modest. These observations, together with the inferred location of the GA dinucleotide in the three-dimensional structure of the intron, suggest that this dinucleotide plays a particularly important role in the second step of splicing.

Entities: Chemical

Mesh：

Substances：

Year: 2000 PMID： 11105751 PMCID： PMC1370021 DOI： 10.1017/s1355838200000972

Source DB: PubMed Journal: RNA ISSN： 1355-8382 Impact factor: 4.942

17 in total

Review 1. Comparative and functional anatomy of group II catalytic introns--a review.

Authors: F Michel; K Umesono; H Ozeki
Journal: Gene Date: 1989-10-15 Impact factor: 3.688

2. Catalytically critical nucleotide in domain 5 of a group II intron.

Authors: C L Peebles; M Zhang; P S Perlman; J S Franzen
Journal: Proc Natl Acad Sci U S A Date: 1995-05-09 Impact factor: 11.205

3. Stereochemical selectivity of group II intron splicing, reverse splicing, and hydrolysis reactions.

Authors: M Podar; P S Perlman; R A Padgett
Journal: Mol Cell Biol Date: 1995-08 Impact factor: 4.272

4. Base-pairing interactions involving the 5' and 3'-terminal nucleotides of group II self-splicing introns.

Authors: A Jacquier; F Michel
Journal: J Mol Biol Date: 1990-06-05 Impact factor: 5.469

5. An RNA conformational change between the two chemical steps of group II self-splicing.

Authors: G Chanfreau; A Jacquier
Journal: EMBO J Date: 1996-07-01 Impact factor: 11.598

Review 6. Structure and activities of group II introns.

Authors: F Michel; J L Ferat
Journal: Annu Rev Biochem Date: 1995 Impact factor: 23.643

7. Branch-point attack in group II introns is a highly reversible transesterification, providing a potential proofreading mechanism for 5'-splice site selection.

Authors: K Chin; A M Pyle
Journal: RNA Date: 1995-06 Impact factor: 4.942

8. Catalytic site components common to both splicing steps of a group II intron.

Authors: G Chanfreau; A Jacquier
Journal: Science Date: 1994-11-25 Impact factor: 47.728

9. Studies of point mutants define three essential paired nucleotides in the domain 5 substructure of a group II intron.

Authors: S C Boulanger; S M Belcher; U Schmidt; S D Dib-Hajj; T Schmidt; P S Perlman
Journal: Mol Cell Biol Date: 1995-08 Impact factor: 4.272

10. Interaction of intronic boundaries is required for the second splicing step efficiency of a group II intron.

Authors: G Chanfreau; A Jacquier
Journal: EMBO J Date: 1993-12-15 Impact factor: 11.598

11 in total

1. Linking the group II intron catalytic domains: tertiary contacts and structural features of domain 3.

Authors: Olga Fedorova; Anna Marie Pyle
Journal: EMBO J Date: 2005-10-27 Impact factor: 11.598

2. Three essential and conserved regions of the group II intron are proximal to the 5'-splice site.

Authors: Alexandre de Lencastre; Anna Marie Pyle
Journal: RNA Date: 2007-11-26 Impact factor: 4.942

3. The linear form of a group II intron catalyzes efficient autocatalytic reverse splicing, establishing a potential for mobility.

Authors: Michael Roitzsch; Anna Marie Pyle
Journal: RNA Date: 2009-01-23 Impact factor: 4.942

Deletion of a conserved dinucleotide inhibits the second step of group II intron splicing.

Review 1. Comparative and functional anatomy of group II catalytic introns--a review.

2. Catalytically critical nucleotide in domain 5 of a group II intron.

3. Stereochemical selectivity of group II intron splicing, reverse splicing, and hydrolysis reactions.

4. Base-pairing interactions involving the 5' and 3'-terminal nucleotides of group II self-splicing introns.

5. An RNA conformational change between the two chemical steps of group II self-splicing.

Review 6. Structure and activities of group II introns.

7. Branch-point attack in group II introns is a highly reversible transesterification, providing a potential proofreading mechanism for 5'-splice site selection.

8. Catalytic site components common to both splicing steps of a group II intron.

9. Studies of point mutants define three essential paired nucleotides in the domain 5 substructure of a group II intron.

10. Interaction of intronic boundaries is required for the second splicing step efficiency of a group II intron.

1. Linking the group II intron catalytic domains: tertiary contacts and structural features of domain 3.

2. Three essential and conserved regions of the group II intron are proximal to the 5'-splice site.

3. The linear form of a group II intron catalyzes efficient autocatalytic reverse splicing, establishing a potential for mobility.

4. Crystal structure of a self-spliced group II intron.

5. A structural analysis of the group II intron active site and implications for the spliceosome.

6. DNA cleavage and reverse splicing of ribonucleoprotein particles reconstituted in vitro with linear RmInt1 RNA.

7. Structural basis for the second step of group II intron splicing.

8. Visualizing group II intron catalysis through the stages of splicing.

9. Now on display: a gallery of group II intron structures at different stages of catalysis.

10. Evidence for a group II intron-like catalytic triplex in the spliceosome.