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Crystallographic and Mutational Studies of Mycobacterium tuberculosis recA Mini-inteins Suggest a Pivotal Role for a Highly Conserved Aspartate Residue

  • Patrick Van Roey
  • , Brian Pereira
  • , Zhong Li
  • , Kaori Hiraga
  • , Marlene Belfort
  • , Victoria Derbyshire

Research output: Contribution to journalArticlepeer-review

79 Scopus citations

Abstract

The 440 amino acid Mtu recA intein consists of independent protein-splicing and endonuclease domains. Previously, removal of the central endonuclease domain of the intein, and selection for function, generated a 168 residue mini-intein, ΔI-SM, that had splicing activity similar to that of the full-length, wild-type protein. A D422G mutation (ΔI-CM) increased C-terminal cleavage activity. Using the ΔI-SM mini-intein structure (presented here) as a guide, we previously generated a highly active 139 residue mini-intein, ΔΔIhh-SM, by replacing 36 amino acid residues in the residual endonuclease loop with a seven-residue β-turn from the autoprocessing domain of Hedgehog protein. The three-dimensional structures of ΔI-SM, ΔΔIhh-SM, and two variants, ΔΔIhh-CM and ΔΔIhh, have been determined to evaluate the effects of the minimization on intein integrity and to investigate the structural and functional consequences of the D422G mutation. These structural studies show that Asp422 is capable of interacting with both the N and C termini. These interactions are lacking in the CM variant, but are replaced by contacts with water molecules. Accordingly, additional mutagenesis of residue 422, combined with mutations that isolate N-terminal and C-terminal cleavage, showed that the side-chain of Asp422 plays a role in both N and C-terminal cleavage, thereby suggesting that this highly conserved residue regulates the balance between the two reactions.

Original languageEnglish
Pages (from-to)162-173
Number of pages12
JournalJournal of Molecular Biology
Volume367
Issue number1
DOIs
StatePublished - Mar 16 2007

Keywords

  • crystal structure
  • intein minimization
  • mutational analyses
  • protein splicing

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