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Title: Structural Insight into How Bacteria Prevent Interference between Multiple Divergent Type IV Secretion Systems

Journal Article · · mBio (Online)
 [1];  [2];  [3];  [2];  [4];  [1];  [5];  [1];  [1];  [2];  [5];  [2];  [2];  [1];  [6];
  1. Department of Microbiology and Immunology, University of Maryland School of Medicine, Baltimore, Maryland, USA
  2. Seattle Structural Genomics Center for Infectious Disease, Seattle, Washington, USA; The Center for Infectious Disease Research (formerly Seattle Biomedical Research Institute), Seattle, Washington, USA
  3. Venom Evolution Lab, School of Biological Sciences, University of Queensland, St. Lucia, Queensland, Australia
  4. Seattle Structural Genomics Center for Infectious Disease, Seattle, Washington, USA; Beryllium Discovery Corp., Bainbridge Island, Washington, USA
  5. Department of Biosciences, University of Helsinki, Helsinki, Finland
  6. Department of Biosciences, University of Helsinki, Helsinki, Finland; Institute of Biomedicine, University of Turku, Turku, Finland

ABSTRACT Prokaryotes use type IV secretion systems (T4SSs) to translocate substrates (e.g., nucleoprotein, DNA, and protein) and/or elaborate surface structures (i.e., pili or adhesins). Bacterial genomes may encode multiple T4SSs, e.g., there are three functionally divergent T4SSs in someBartonellaspecies (vir,vbh, andtrw). In a unique case, most rickettsial species encode a T4SS (rvh) enriched with gene duplication. Within single genomes, the evolutionary and functional implications of cross-system interchangeability of analogous T4SS protein components remains poorly understood. To lend insight into cross-system interchangeability, we analyzed the VirB8 family of T4SS channel proteins. Crystal structures of three VirB8 and two TrwGBartonellaproteins revealed highly conserved C-terminal periplasmic domain folds and dimerization interfaces, despite tremendous sequence divergence. This implies remarkable structural constraints for VirB8 components in the assembly of a functional T4SS. VirB8/TrwG heterodimers, determined via bacterial two-hybrid assays and molecular modeling, indicate that differential expression oftrwandvirsystems is the likely barrier to VirB8-TrwG interchangeability. We also determined the crystal structure ofRickettsia typhiRvhB8-II and modeled its coexpressed divergent paralog RvhB8-I. Remarkably, while RvhB8-I dimerizes and is structurally similar to other VirB8 proteins, the RvhB8-II dimer interface deviates substantially from other VirB8 structures, potentially preventing RvhB8-I/RvhB8-II heterodimerization. For thervhT4SS, the evolution of divergent VirB8 paralogs implies a functional diversification that is unknown in other T4SSs. Collectively, our data identify two different constraints (spatiotemporal forBartonellatrwandvirT4SSs and structural forrvhT4SSs) that mediate the functionality of multiple divergent T4SSs within a single bacterium. IMPORTANCEAssembly of multiprotein complexes at the right time and at the right cellular location is a fundamentally important task for any organism. In this respect, bacteria that express multiple analogous type IV secretion systems (T4SSs), each composed of around 12 different components, face an overwhelming complexity. Our work here presents the first structural investigation on factors regulating the maintenance of multiple T4SSs within a single bacterium. The structural data imply that the T4SS-expressing bacteria rely on two strategies to prevent cross-system interchangeability: (i) tight temporal regulation of expression or (ii) rapid diversification of the T4SS components. T4SSs are ideal drug targets provided that no analogous counterparts are known from eukaryotes. Drugs targeting the barriers to cross-system interchangeability (i.e., regulators) could dysregulate the structural and functional independence of discrete systems, potentially creating interference that prevents their efficient coordination throughout bacterial infection.

Research Organization:
Argonne National Lab. (ANL), Argonne, IL (United States). Advanced Photon Source (APS)
Sponsoring Organization:
DHS - DEPARTMENT OF HOMELAND SECURITYNIHNIAID
OSTI ID:
1498342
Journal Information:
mBio (Online), Vol. 6, Issue 6; ISSN 2150-7511
Publisher:
American Society for Microbiology
Country of Publication:
United States
Language:
ENGLISH

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