4E1P
Crystal structure of the dimerization domain of Lsr2 from Mycobacterium tuberculosis in the P 1 21 1 space group
Summary for 4E1P
| Entry DOI | 10.2210/pdb4e1p/pdb |
| Related | 4E1R |
| Descriptor | Protein lsr2 (2 entities in total) |
| Functional Keywords | anti-parallel beta sheet, dimer, dna binding protein |
| Biological source | Mycobacterium tuberculosis |
| Cellular location | Cytoplasm, nucleoid: P65648 |
| Total number of polymer chains | 2 |
| Total formula weight | 13078.65 |
| Authors | Summers, E.L.,Meindl, K.,Uson, I.,Arcus, V.L. (deposition date: 2012-03-06, release date: 2012-06-20, Last modification date: 2024-02-28) |
| Primary citation | Summers, E.L.,Meindl, K.,Uson, I.,Mitra, A.K.,Radjainia, M.,Colangeli, R.,Alland, D.,Arcus, V.L. The structure of the oligomerization domain of Lsr2 from Mycobacterium tuberculosis reveals a mechanism for chromosome organization and protection. Plos One, 7:e38542-e38542, 2012 Cited by PubMed Abstract: Lsr2 is a small DNA-binding protein present in mycobacteria and related actinobacteria that regulates gene expression and influences the organization of bacterial chromatin. Lsr2 is a dimer that binds to AT-rich regions of chromosomal DNA and physically protects DNA from damage by reactive oxygen intermediates (ROI). A recent structure of the C-terminal DNA-binding domain of Lsr2 provides a rationale for its interaction with the minor groove of DNA, its preference for AT-rich tracts, and its similarity to other bacterial nucleoid-associated DNA-binding domains. In contrast, the details of Lsr2 dimerization (and oligomerization) via its N-terminal domain, and the mechanism of Lsr2-mediated chromosomal cross-linking and protection is unknown. We have solved the structure of the N-terminal domain of Lsr2 (N-Lsr2) at 1.73 Å resolution using crystallographic ab initio approaches. The structure shows an intimate dimer of two ß-ß-a motifs with no close homologues in the structural databases. The organization of individual N-Lsr2 dimers in the crystal also reveals a mechanism for oligomerization. Proteolytic removal of three N-terminal residues from Lsr2 results in the formation of an anti-parallel β-sheet between neighboring molecules and the formation of linear chains of N-Lsr2. Oligomerization can be artificially induced using low concentrations of trypsin and the arrangement of N-Lsr2 into long chains is observed in both monoclinic and hexagonal crystallographic space groups. In solution, oligomerization of N-Lsr2 is also observed following treatment with trypsin. A change in chromosomal topology after the addition of trypsin to full-length Lsr2-DNA complexes and protection of DNA towards DNAse digestion can be observed using electron microscopy and electrophoresis. These results suggest a mechanism for oligomerization of Lsr2 via protease-activation leading to chromosome compaction and protection, and concomitant down-regulation of large numbers of genes. This mechanism is likely to be relevant under conditions of stress where cellular proteases are known to be upregulated. PubMed: 22719899DOI: 10.1371/journal.pone.0038542 PDB entries with the same primary citation |
| Experimental method | X-RAY DIFFRACTION (1.728 Å) |
Structure validation
Download full validation report
