Recognition and processing of the origin of transfer DNA by conjugative relaxase TrwC

Guasch, Alı́cia; Lucas, María; Moncalián, Gabriel; Cabezas, Matilde; Pérez-Luque, R.; Gomis‐Rüth, F. Xavier; Cruz, Fernando de la; Coll, Miquel

doi:10.1038/nsb1017

Cited by 131 publications

(218 citation statements)

References 43 publications

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“…The crystal structures of the relaxase domains of TrwC (R388) and TraI (F) have been determined (Datta et al, 2003;Guasch et al, 2003). They reveal a conserved compact molecular scaVold possessing features that explain the high aYnity and speciWcity for their respective DNA substrates.…”

Section: Conjugative Relaxases: Dna Carrier Proteins Secreted By the mentioning

confidence: 99%

“…The structure consists of a Wve-strand antiparallel -sheet core ('palm' domain), which is Xanked by several -helices. The structure of TrwC in complex with a 25-mer oligonucleotide corresponding to the sequence of the transfer strand just upstream of the nic site furthermore provides details of the interactions between the relaxase and its ssDNA substrate (Guasch et al, 2003). This structure corresponds to the situation most probably encountered after cleavage at the nic site.…”

Section: Conjugative Relaxases: Dna Carrier Proteins Secreted By the mentioning

confidence: 99%

“…Possible roles for the metal cation consist in polarizing the scissile phosphate of the ssDNA substrate for facilitating the nucleophilic attack by the catalytic tyrosine hydroxyl group, and of stabilizing the ensuing transition state. An aspartate residue in TrwC has been proposed as a candidate general base that could activate the catalytic tyrosine by proton abstraction (Guasch et al, 2003). TraI and TrwC each contain a second tyrosine residue which is thought to catalyze the second DNA strand transfer reaction that recircularizes the plasmid after one round of transfer (Grandoso et al, 2000;Pansegrau and Lanka, 1996b).…”

Section: Conjugative Relaxases: Dna Carrier Proteins Secreted By the mentioning

confidence: 99%

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The mating pair formation system of conjugative plasmids—A versatile secretion machinery for transfer of proteins and DNA

Schröder

Lanka

2005

Plasmid

188

146

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The mating pair formation (Mpf) system functions as a secretion machinery for intercellular DNA transfer during bacterial conjugation. The components of the Mpf system, comprising a minimal set of 10 conserved proteins, form a membrane-spanning protein complex and a surface-exposed sex pilus, which both serve to establish intimate physical contacts with a recipient bacterium. To function as a DNA secretion apparatus the Mpf complex additionally requires the coupling protein (CP). The CP interacts with the DNA substrate and couples it to the secretion pore formed by the Mpf system. Mpf/CP conjugation systems belong to the family of type IV secretion systems (T4SS), which also includes DNA-uptake and -release systems, as well as eVector protein translocation systems of bacterial pathogens such as Agrobacterium tumefaciens (VirB/VirD4) and Helicobacter pylori (Cag). The increased eVorts to unravel the molecular mechanisms of type IV secretion have largely advanced our current understanding of the Mpf/CP system of bacterial conjugation systems. It has become apparent that proteins coupled to DNA rather than DNA itself are the actively transported substrates during bacterial conjugation. We here present a uniWed and updated view of the functioning and the molecular architecture of the Mpf/CP machinery. 

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Section: Conjugative Relaxases: Dna Carrier Proteins Secreted By the mentioning

confidence: 99%

Section: Conjugative Relaxases: Dna Carrier Proteins Secreted By the mentioning

confidence: 99%

Section: Conjugative Relaxases: Dna Carrier Proteins Secreted By the mentioning

confidence: 99%

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The mating pair formation system of conjugative plasmids—A versatile secretion machinery for transfer of proteins and DNA

Schröder

Lanka

2005

Plasmid

188

146

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“…[5][6][7][8] Finally, the T4CP functions together with a trans-envelope secretion channel composed of the mating pair formation (Mpf) proteins to deliver the DNA transfer intermediate to the cell exterior. 9 The processing and recruitment reactions are biochemically well characterized for several conjugation systems, and recent structurefunction studies have been aided by available crystal structures for the TrwC 10,11 and TraI 12,13 relaxases of plasmids R388 and F, respectively, and TrwB T4CP 14 of plasmid R388. Until recently, however, there has been very little understanding of the secretion channel architecture or mechanism of action.…”

Section: Introductionmentioning

confidence: 99%

Agrobacterium tumefaciens VirB6 Domains Direct the Ordered Export of a DNA Substrate Through a Type IV Secretion System

Jakubowski

Krishnamoorthy

Cascales

et al. 2004

Journal of Molecular Biology

108

128

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The Agrobacterium tumefaciens VirB/D4 type IV secretion system (T4SS) translocates DNA and protein substrates across the bacterial cell envelope. Six presumptive channel subunits of this T4SS (VirD4, VirB11, VirB6, VirB8, VirB2, and VirB9) form close contacts with the VirD2-Tstrand transfer intermediate during export, as shown recently by a novel transfer DNA immunoprecipitation (TrIP) assay. Here, we characterize the contribution of the hydrophobic channel component VirB6 to substrate translocation. Results of reporter protein fusion and cysteine accessibility studies support a model for VirB6 as a polytopic membrane protein with a periplasmic N terminus, five transmembrane segments, and a cytoplasmic C terminus. TrIP studies aimed at characterizing the effects of VirB6 insertion and deletion mutations on substrate translocation identified several VirB6 functional domains: (i) a central region composed of a large periplasmic loop (P2) (residues 84 to 165) mediates the interaction of VirB6 with the exiting Tstrand; (ii) a multi-membrane-spanning region carboxyl-terminal to loop P2 (residues 165 to 245) is required for substrate transfer from VirB6 to the bitopic membrane subunit VirB8; and (iii) the two terminal regions (residues 1 to 64 and 245 to 290) are required for substrate transfer to the periplasmic and outer membrane-associated VirB2 and VirB9 subunits. Our findings support a model whereby the periplasmic loop P2 comprises a portion of the secretion channel and distinct domains of VirB6 participate in channel subunit interactions required for substrate passage to the cell exterior.

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“…A similar mechanism has been proposed for the integration of a bacterial virus, bacteriophage CTXȠ, into the Vibrio cholerae genome 9 . Moreover, related models would also explain other systems involved in horizontal gene transfer, including plasmid and viral replication (REP proteins), conjugal plasmid transfer from cell to cell (relaxases) and certain transposase enzymes [10][11][12][13][14] .…”

Section: Michael Chandlermentioning

confidence: 99%

Hepatitis C virus biology

2003

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Recognition and processing of the origin of transfer DNA by conjugative relaxase TrwC

Cited by 131 publications

References 43 publications

The mating pair formation system of conjugative plasmids—A versatile secretion machinery for transfer of proteins and DNA

The mating pair formation system of conjugative plasmids—A versatile secretion machinery for transfer of proteins and DNA

Agrobacterium tumefaciens VirB6 Domains Direct the Ordered Export of a DNA Substrate Through a Type IV Secretion System

Hepatitis C virus biology

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