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2. The Deinococcus radiodurans DR1245 Protein, a DdrB Partner Homologous to YbjN Proteins and Reminiscent of Type III Secretion System Chaperones

Author

Norais, C, Servant, P, Bouthier-de-la-Tour, C, Coureux, PD, Ithurbide, S, Vannier, F, Guerin, PP, Dulberger, CL, Satyshur, KA, Keck, JL, Armengaud, J, Cox, MM, Sommer, S, Norais, C, Servant, P, Bouthier-de-la-Tour, C, Coureux, PD, Ithurbide, S, Vannier, F, Guerin, PP, Dulberger, CL, Satyshur, KA, Keck, JL, Armengaud, J, Cox, MM, and Sommer, S

Abstract

The bacterium Deinococcus radiodurans exhibits an extreme resistance to ionizing radiation. A small subset of Deinococcus genus-specific genes were shown to be up-regulated upon exposure to ionizing radiation and to play a role in genome reconstitution. These genes include an SSB-like protein called DdrB. Here, we identified a novel protein encoded by the dr1245 gene as an interacting partner of DdrB. A strain devoid of the DR1245 protein is impaired in growth, exhibiting a generation time approximately threefold that of the wild type strain while radioresistance is not affected. We determined the three-dimensional structure of DR1245, revealing a relationship with type III secretion system chaperones and YbjN family proteins. Thus, DR1245 may display some chaperone activity towards DdrB and possibly other substrates. © 2013 Norais et al.

Published
2013

3. Crystal Structure of DR_1245 from Deinococcus radiodurans

Author

Norais, C., primary, Servant, P., additional, Bouthier-de-la-Tour, C., additional, Coureux, P.D., additional, Ithurbide, S., additional, Vannier, F., additional, Guerin, P., additional, Dulberger, C.L., additional, Satyshur, K.A., additional, Keck, J.L., additional, Armengaud, J., additional, Cox, M.M., additional, and Sommer, S., additional

Published
2013
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8. Structural and functional characterization of DdrC, a novel DNA damage-induced nucleoid associated protein involved in DNA compaction.

Author

Banneville AS, Bouthier de la Tour C, De Bonis S, Hognon C, Colletier JP, Teulon JM, Le Roy A, Pellequer JL, Monari A, Dehez F, Confalonieri F, Servant P, and Timmins J

Subjects
Bacterial Proteins metabolism, DNA Damage, DNA Repair, DNA, Circular metabolism, Bacterial Proteins chemistry, Deinococcus genetics, Deinococcus metabolism
Abstract

Deinococcus radiodurans is a spherical bacterium well-known for its outstanding resistance to DNA-damaging agents. Exposure to such agents leads to drastic changes in the transcriptome of D. radiodurans. In particular, four Deinococcus-specific genes, known as DNA Damage Response genes, are strongly up-regulated and have been shown to contribute to the resistance phenotype of D. radiodurans. One of these, DdrC, is expressed shortly after exposure to γ-radiation and is rapidly recruited to the nucleoid. In vitro, DdrC has been shown to compact circular DNA, circularize linear DNA, anneal complementary DNA strands and protect DNA from nucleases. To shed light on the possible functions of DdrC in D. radiodurans, we determined the crystal structure of the domain-swapped DdrC dimer at a resolution of 2.5 Å and further characterized its DNA binding and compaction properties. Notably, we show that DdrC bears two asymmetric DNA binding sites located on either side of the dimer and can modulate the topology and level of compaction of circular DNA. These findings suggest that DdrC may be a DNA damage-induced nucleoid-associated protein that enhances nucleoid compaction to limit the dispersion of the fragmented genome and facilitate DNA repair after exposure to severe DNA damaging conditions., (© The Author(s) 2022. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published
2022
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9. Characterization of the Radiation Desiccation Response Regulon of the Radioresistant Bacterium Deinococcus radiodurans by Integrative Genomic Analyses.

Author

Eugénie N, Zivanovic Y, Lelandais G, Coste G, Bouthier de la Tour C, Bentchikou E, Servant P, and Confalonieri F

Subjects
Bacterial Proteins metabolism, DNA Damage genetics, Deinococcus genetics, Genomics, Regulon physiology, Deinococcus metabolism, Gene Expression Regulation, Bacterial physiology, Regulon genetics, Transcription Factors metabolism
Abstract

Numerous genes are overexpressed in the radioresistant bacterium Deinococcus radiodurans after exposure to radiation or prolonged desiccation. It was shown that the DdrO and IrrE proteins play a major role in regulating the expression of approximately twenty genes. The transcriptional repressor DdrO blocks the expression of these genes under normal growth conditions. After exposure to genotoxic agents, the IrrE metalloprotease cleaves DdrO and relieves gene repression. At present, many questions remain, such as the number of genes regulated by DdrO. Here, we present the first ChIP-seq analysis performed at the genome level in Deinococcus species coupled with RNA-seq, which was achieved in the presence or not of DdrO. We also resequenced our laboratory stock strain of D. radiodurans R1 ATCC 13939 to obtain an accurate reference for read alignments and gene expression quantifications. We highlighted genes that are directly under the control of this transcriptional repressor and showed that the DdrO regulon in D. radiodurans includes numerous other genes than those previously described, including DNA and RNA metabolism proteins. These results thus pave the way to better understand the radioresistance pathways encoded by this bacterium and to compare the stress-induced responses mediated by this pair of proteins in diverse bacteria.

Published
2021
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10. Natural Transformation in Deinococcus radiodurans : A Genetic Analysis Reveals the Major Roles of DprA, DdrB, RecA, RecF, and RecO Proteins.

Author

Ithurbide S, Coste G, Lisboa J, Eugénie N, Bentchikou E, Bouthier de la Tour C, Liger D, Confalonieri F, Sommer S, Quevillon-Cheruel S, and Servant P

Abstract

Horizontal gene transfer is a major driver of bacterial evolution and adaptation to environmental stresses, occurring notably via transformation of naturally competent organisms. The Deinococcus radiodurans bacterium, characterized by its extreme radioresistance, is also naturally competent. Here, we investigated the role of D. radiodurans players involved in different steps of natural transformation. First, we identified the factors (PilQ, PilD, type IV pilins, PilB, PilT, ComEC-ComEA, and ComF) involved in DNA uptake and DNA translocation across the external and cytoplasmic membranes and showed that the DNA-uptake machinery is similar to that described in the Gram negative bacterium Vibrio cholerae . Then, we studied the involvement of recombination and DNA repair proteins, RecA, RecF, RecO, DprA, and DdrB into the DNA processing steps of D. radiodurans transformation by plasmid and genomic DNA. The transformation frequency of the cells devoid of DprA, a highly conserved protein among competent species, strongly decreased but was not completely abolished whereas it was completely abolished in Δ dprA Δ recF , Δ dprA Δ recO , and Δ dprA Δ ddrB double mutants. We propose that RecF and RecO, belonging to the recombination mediator complex, and DdrB, a specific deinococcal DNA binding protein, can replace a function played by DprA, or alternatively, act at a different step of recombination with DprA. We also demonstrated that a Δ dprA mutant is as resistant as wild type to various doses of γ-irradiation, suggesting that DprA, and potentially transformation, do not play a major role in D. radiodurans radioresistance., (Copyright © 2020 Ithurbide, Coste, Lisboa, Eugénie, Bentchikou, Bouthier de la Tour, Liger, Confalonieri, Sommer, Quevillon-Cheruel and Servant.)

Published
2020
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11. In vivo and in vitro characterization of DdrC, a DNA damage response protein in Deinococcus radiodurans bacterium.

Author

Bouthier de la Tour C, Mathieu M, Meyer L, Dupaigne P, Passot F, Servant P, Sommer S, Le Cam E, and Confalonieri F

Subjects
Bacterial Proteins chemistry, DNA Repair, DNA, Single-Stranded genetics, DNA, Single-Stranded metabolism, Deinococcus radiation effects, Dose-Response Relationship, Radiation, Gamma Rays adverse effects, Gene Deletion, Plasmids genetics, Protein Multimerization, Protein Structure, Quaternary, Ultraviolet Rays adverse effects, Bacterial Proteins metabolism, DNA Damage, Deinococcus genetics, Deinococcus metabolism
Abstract

The bacterium Deinococcus radiodurans possesses a set of Deinococcus-specific genes highly induced after DNA damage. Among them, ddrC (dr0003) was recently re-annotated, found to be in the inverse orientation and called A2G07_00380. Here, we report the first in vivo and in vitro characterization of the corrected DdrC protein to better understand its function in irradiated cells. In vivo, the ΔddrC null mutant is sensitive to high doses of UV radiation and the ddrC deletion significantly increases UV-sensitivity of ΔuvrA or ΔuvsE mutant strains. We show that the expression of the DdrC protein is induced after γ-irradiation and is under the control of the regulators, DdrO and IrrE. DdrC is rapidly recruited into the nucleoid of the irradiated cells. In vitro, we show that DdrC is able to bind single- and double-stranded DNA with a preference for the single-stranded DNA but without sequence or shape specificity and protects DNA from various nuclease attacks. DdrC also condenses DNA and promotes circularization of linear DNA. Finally, we show that the purified protein exhibits a DNA strand annealing activity. Altogether, our results suggest that DdrC is a new DNA binding protein with pleiotropic activities. It might maintain the damaged DNA fragments end to end, thus limiting their dispersion and extensive degradation after exposure to ionizing radiation. DdrC might also be an accessory protein that participates in a single strand annealing pathway whose importance in DNA repair becomes apparent when DNA is heavily damaged.

Published
2017
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12. PprA Protein Is Involved in Chromosome Segregation via Its Physical and Functional Interaction with DNA Gyrase in Irradiated Deinococcus radiodurans Bacteria.

Author

Devigne A, Guérin P, Lisboa J, Quevillon-Cheruel S, Armengaud J, Sommer S, Bouthier de la Tour C, and Servant P

Abstract

PprA, a radiation-induced Deinococcus-specific protein, was previously shown to be required for cell survival and accurate chromosome segregation after exposure to ionizing radiation. Here, we used an in vivo approach to determine, by shotgun proteomics, putative PprA partners coimmunoprecipitating with PprA when cells were exposed to gamma rays. Among them, we found the two subunits of DNA gyrase and, thus, chose to focus our work on characterizing the activities of the deinococcal DNA gyrase in the presence or absence of PprA. Loss of PprA rendered cells hypersensitive to novobiocin, an inhibitor of the B subunit of DNA gyrase. We showed that treatment of bacteria with novobiocin resulted in induction of the radiation desiccation response (RDR) regulon and in defects in chromosome segregation that were aggravated by the absence of PprA. In vitro, the deinococcal DNA gyrase, like other bacterial DNA gyrases, possesses DNA negative supercoiling and decatenation activities. These two activities are inhibited in vitro by novobiocin and nalidixic acid, whereas PprA specifically stimulates the decatenation activity of DNA gyrase. Together, these results suggest that PprA plays a major role in chromosome decatenation via its interaction with the deinococcal DNA gyrase when D. radiodurans cells are recovering from exposure to ionizing radiation. IMPORTANCE D. radiodurans is one of the most radiation-resistant organisms known. This bacterium is able to cope with high levels of DNA lesions generated by exposure to extreme doses of ionizing radiation and to reconstruct a functional genome from hundreds of radiation-induced chromosomal fragments. Here, we identified partners of PprA, a radiation-induced Deinococcus-specific protein, previously shown to be required for radioresistance. Our study leads to three main findings: (i) PprA interacts with DNA gyrase after irradiation, (ii) treatment of cells with novobiocin results in defects in chromosome segregation that are aggravated by the absence of PprA, and (iii) PprA stimulates the decatenation activity of DNA gyrase. Our results extend the knowledge of how D. radiodurans cells survive exposure to extreme doses of gamma irradiation and point out the link between DNA repair, chromosome segregation, and DNA gyrase activities in the radioresistant D. radiodurans bacterium.

Published
2016
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13. The abundant and essential HU proteins in Deinococcus deserti and Deinococcus radiodurans are translated from leaderless mRNA.

Author

Bouthier de la Tour C, Blanchard L, Dulermo R, Ludanyi M, Devigne A, Armengaud J, Sommer S, and de Groot A

Subjects
5' Untranslated Regions, Amino Acid Sequence, Bacterial Proteins chemistry, Bacterial Proteins metabolism, Codon, Initiator genetics, Codon, Initiator metabolism, DNA-Binding Proteins chemistry, DNA-Binding Proteins metabolism, Deinococcus chemistry, Deinococcus metabolism, Molecular Sequence Data, RNA, Messenger metabolism, Sequence Alignment, Bacterial Proteins genetics, DNA-Binding Proteins genetics, Deinococcus genetics, Gene Expression Regulation, Bacterial, Protein Biosynthesis, RNA, Messenger genetics
Abstract

HU proteins have an important architectural role in nucleoid organization in bacteria. Compared with HU of many bacteria, HU proteins from Deinococcus species possess an N-terminal lysine-rich extension similar to the eukaryotic histone H1 C-terminal domain involved in DNA compaction. The single HU gene in Deinococcus radiodurans, encoding DrHU, is required for nucleoid compaction and cell viability. Deinococcus deserti contains three expressed HU genes, encoding DdHU1, DdHU2 and DdHU3. Here, we show that either DdHU1 or DdHU2 is essential in D. deserti. DdHU1 and DdHU2, but not DdHU3, can substitute for DrHU in D. radiodurans, indicating that DdHU3 may have a non-essential function different from DdHU1, DdHU2 and DrHU. Interestingly, the highly abundant DrHU and DdHU1 proteins, and also the less expressed DdHU2, are translated in Deinococcus from leaderless mRNAs, which lack a 5'-untranslated region and, hence, the Shine-Dalgarno sequence. Unexpectedly, cloning the DrHU or DdHU1 gene under control of a strong promoter in an expression plasmid, which results in leadered transcripts, strongly reduced the DrHU and DdHU1 protein level in D. radiodurans compared with that obtained from the natural leaderless gene. We also show that the start codon position for DrHU and DdHU1 should be reannotated, resulting in proteins that are 15 and 4 aa residues shorter than initially reported. The expression level and start codon correction were crucial for functional characterization of HU in Deinococcus.

Published
2015
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14. DdrO is an essential protein that regulates the radiation desiccation response and the apoptotic-like cell death in the radioresistant Deinococcus radiodurans bacterium.

Author

Devigne A, Ithurbide S, Bouthier de la Tour C, Passot F, Mathieu M, Sommer S, and Servant P

Subjects
Amino Acid Sequence, Bacterial Proteins metabolism, Bacterial Proteins radiation effects, DNA Damage radiation effects, DNA Repair, Dehydration, Deinococcus growth & development, Deinococcus ultrastructure, Genomics, Ketoglutarate Dehydrogenase Complex genetics, Mutagenesis, Open Reading Frames, Promoter Regions, Genetic, Protein Structure, Tertiary, Deinococcus genetics, Deinococcus radiation effects, Gene Expression Regulation, Bacterial, Regulon
Abstract

Deinococcus radiodurans is known for its extreme radioresistance. Comparative genomics identified a radiation-desiccation response (RDR) regulon comprising genes that are highly induced after DNA damage and containing a conserved motif (RDRM) upstream of their coding region. We demonstrated that the RDRM sequence is involved in cis-regulation of the RDR gene ddrB in vivo. Using a transposon mutagenesis approach, we showed that, in addition to ddrO encoding a predicted RDR repressor and irrE encoding a positive regulator recently shown to cleave DdrO in Deinococcus deserti, two genes encoding α-keto-glutarate dehydrogenase subunits are involved in ddrB regulation. In wild-type cells, the DdrO cell concentration decreased transiently in an IrrE-dependent manner at early times after irradiation. Using a conditional gene inactivation system, we showed that DdrO depletion enhanced expression of three RDR proteins, consistent with the hypothesis that DdrO acts as a repressor of the RDR regulon. DdrO-depleted cells loose viability and showed morphological changes evocative of an apoptotic-like response, including membrane blebbing, defects in cell division and DNA fragmentation. We propose that DNA repair and apoptotic-like death might be two responses mediated by the same regulators, IrrE and DdrO, but differently activated depending on the persistence of IrrE-dependent DdrO cleavage., (© 2015 John Wiley & Sons Ltd.)

Published
2015
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15. The PprA protein is required for accurate cell division of γ-irradiated Deinococcus radiodurans bacteria.

Author

Devigne A, Mersaoui S, Bouthier-de-la-Tour C, Sommer S, and Servant P

Subjects
Bacterial Proteins metabolism, DNA Breaks, Double-Stranded, DNA Repair, DNA Replication, Deinococcus cytology, Deinococcus radiation effects, Gene Deletion, Phenotype, Radiation Tolerance genetics, Rec A Recombinases genetics, Rec A Recombinases metabolism, Bacterial Proteins genetics, Cell Division genetics, Deinococcus genetics, Gamma Rays
Abstract

Deinococcus radiodurans, one of the most radioresistant organisms known to date is able to reconstruct an intact genome from hundreds of DNA fragments. Here, we investigate the in vivo role of PprA, a radiation-induced Deinococcus specific protein. We report that DNA double strand break repair in cells devoid of PprA and exposed to 3800Gy γ-irradiation takes place efficiently with a delay of only 1h as compared to the wild type, whereas massive DNA synthesis begins 90min after irradiation as in the wild type, a phenotype insufficient to explain the severe radiosensitivity of the ΔpprA mutant. We show that the slow kinetics of reassembly of DNA fragments in a ΔpprA ΔrecA double mutant was the same as that observed in a ΔrecA single mutant demonstrating that PprA does not play a major role in DNA repair through RecA-independent pathways. Using a tagged PprA protein and immunofluorescence microscopy, we show that PprA is recruited onto the nucleoid after γ-irradiation before DNA double strand break repair completion, and then is found as a thread across the septum in dividing cells. Moreover, whereas untreated cells devoid of PprA displayed a wild type morphology, they showed a characteristic cell division abnormality after irradiation not found in other radiosensitive mutants committed to die, as DNA is present equally in the two daughter cells but not separated at the division septum. We propose that PprA may play a crucial role in the control of DNA segregation and/or cell division after DNA double strand break repair., (Copyright © 2013 Elsevier B.V. All rights reserved.)

Published
2013
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16. The Deinococcus radiodurans DR1245 protein, a DdrB partner homologous to YbjN proteins and reminiscent of type III secretion system chaperones.

Author

Norais C, Servant P, Bouthier-de-la-Tour C, Coureux PD, Ithurbide S, Vannier F, Guerin PP, Dulberger CL, Satyshur KA, Keck JL, Armengaud J, Cox MM, and Sommer S

Subjects
Amino Acid Sequence, Bacterial Proteins chemistry, Base Sequence, Deinococcus genetics, Deinococcus growth & development, Deinococcus radiation effects, Models, Molecular, Molecular Chaperones chemistry, Molecular Sequence Data, Mutation, Protein Binding, Protein Conformation, Radiation Tolerance genetics, Sequence Alignment, Bacterial Proteins metabolism, Bacterial Secretion Systems, Deinococcus metabolism, Molecular Chaperones metabolism
Abstract

The bacterium Deinococcus radiodurans exhibits an extreme resistance to ionizing radiation. A small subset of Deinococcus genus-specific genes were shown to be up-regulated upon exposure to ionizing radiation and to play a role in genome reconstitution. These genes include an SSB-like protein called DdrB. Here, we identified a novel protein encoded by the dr1245 gene as an interacting partner of DdrB. A strain devoid of the DR1245 protein is impaired in growth, exhibiting a generation time approximately threefold that of the wild type strain while radioresistance is not affected. We determined the three-dimensional structure of DR1245, revealing a relationship with type III secretion system chaperones and YbjN family proteins. Thus, DR1245 may display some chaperone activity towards DdrB and possibly other substrates.

Published
2013
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17. A comparative proteomic approach to better define Deinococcus nucleoid specificities.

Author

Toueille M, Mirabella B, Guérin P, Bouthier de la Tour C, Boisnard S, Nguyen HH, Blanchard L, Servant P, de Groot A, Sommer S, and Armengaud J

Subjects
Bacterial Proteins isolation & purification, DNA Gyrase metabolism, DNA-Binding Proteins chemistry, DNA-Binding Proteins isolation & purification, Deinococcus radiation effects, Organelles chemistry, Proteomics, Bacterial Proteins chemistry, Deinococcus genetics, Organelles metabolism
Abstract

Compared to radiation-sensitive bacteria, the nucleoids of radiation-resistant Deinococcus species show a higher degree of compaction. Such a condensed nucleoid may contribute to the extreme radiation resistance of Deinococcus by limiting dispersion of radiation-induced DNA fragments. Architectural proteins may play a role in this high degree of nucleoid compaction, but comparative genomics revealed only a limited number of Deinococcus homologs of known nucleoid-associated proteins (NAPs) from other species such as Escherichia coli. A comparative proteomic approach was used to identify potentially novel proteins from isolated nucleoids of Deinococcus radiodurans and Deinococcus deserti. Proteins in nucleoid enriched fractions were identified and semi-quantified by shotgun proteomics. Based on normalized spectral counts, the histone-like DNA-binding protein HU appeared to be the most abundant among candidate NAPs from both micro-organisms. By immunofluorescence microscopy, D. radiodurans HU and both DNA gyrase subunits were shown to be distributed throughout the nucleoid structure and absent from the cytoplasm. Taken together, our results suggest that D. radiodurans and D. deserti bacteria contain a very low diversity of NAPs, with HU and DNA gyrase being the main proteins involved in the organization of the Deinococcus nucleoids., (Copyright © 2012 Elsevier B.V. All rights reserved.)

Published
2012
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18. The deinococcal DdrB protein is involved in an early step of DNA double strand break repair and in plasmid transformation through its single-strand annealing activity.

Author

Bouthier de la Tour C, Boisnard S, Norais C, Toueille M, Bentchikou E, Vannier F, Cox MM, Sommer S, and Servant P

Subjects
Active Transport, Cell Nucleus radiation effects, Bacterial Proteins chemistry, Bacterial Proteins genetics, Cell Nucleus metabolism, Cell Nucleus radiation effects, DNA Fragmentation radiation effects, DNA Repair radiation effects, DNA, Bacterial biosynthesis, DNA, Bacterial genetics, DNA, Bacterial metabolism, DNA, Single-Stranded biosynthesis, DNA, Single-Stranded genetics, Deinococcus genetics, Deinococcus radiation effects, Mutation, Protein Structure, Tertiary, Radiation Tolerance genetics, Time Factors, Bacterial Proteins metabolism, DNA Breaks, Double-Stranded radiation effects, DNA Repair genetics, DNA, Single-Stranded metabolism, Deinococcus metabolism, Plasmids genetics, Transformation, Bacterial radiation effects
Abstract

The Deinococcus radiodurans bacterium exhibits an extreme resistance to ionizing radiation. Here, we investigated the in vivo role of DdrB, a radiation-induced Deinococcus specific protein that was previously shown to exhibit some in vitro properties akin to those of SSB protein from Escherichia coli but also to promote annealing of single stranded DNA. First we report that the deletion of the C-terminal motif of the DdrB protein, which is similar to the SSB C-terminal motif involved in recruitment to DNA of repair proteins, did neither affect cell radioresistance nor DNA binding properties of purified DdrB protein. We show that, in spite of their different quaternary structure, DdrB and SSB occlude the same amount of ssDNA in vitro. We also show that DdrB is recruited early and transiently after irradiation into the nucleoid to form discrete foci. Absence of DdrB increased the lag phase of the extended synthesis-dependent strand annealing (ESDSA) process, affecting neither the rate of DNA synthesis nor the efficiency of fragment reassembly, as indicated by monitoring DNA synthesis and genome reconstitution in cells exposed to a sub-lethal ionizing radiation dose. Moreover, cells devoid of DdrB were affected in the establishment of plasmid DNA during natural transformation, a process that requires pairing of internalized plasmid single stranded DNA fragments, whereas they were proficient in transformation by a chromosomal DNA marker that integrates into the host chromosome through homologous recombination. Our data are consistent with a model in which DdrB participates in an early step of DNA double strand break repair in cells exposed to very high radiation doses. DdrB might facilitate the accurate assembly of the myriad of small fragments generated by extreme radiation exposure through a single strand annealing (SSA) process to generate suitable substrates for subsequent ESDSA-promoted genome reconstitution., (2011 Elsevier B.V. All rights reserved.)

Published
2011
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19. The Deinococcus radiodurans SMC protein is dispensable for cell viability yet plays a role in DNA folding.

Author

Bouthier de la Tour C, Toueille M, Jolivet E, Nguyen HH, Servant P, Vannier F, and Sommer S

Subjects
Bacterial Proteins genetics, Cell Cycle Proteins genetics, DNA, Bacterial genetics, DNA, Superhelical chemistry, DNA, Superhelical genetics, Deinococcus genetics, Deinococcus growth & development, Deoxyribonucleases genetics, Deoxyribonucleases metabolism, Gene Deletion, Genes, Bacterial, Mutation, Nucleic Acid Conformation, Plasmids chemistry, Plasmids genetics, Bacterial Proteins metabolism, Cell Cycle Proteins metabolism, DNA, Bacterial chemistry, Deinococcus metabolism
Abstract

Deinococcus radiodurans contains a highly condensed nucleoid that remains to be unaltered following the exposure to high doses of gamma-irradiation. Proteins belonging to the structural maintenance of chromosome protein (SMC) family are present in all organisms and were shown to be involved in chromosome condensation, pairing, and/or segregation. Here, we have inactivated the smc gene in the radioresistant bacterium D. radiodurans, and, unexpectedly, found that smc null mutants showed no discernible phenotype except an increased sensitivity to gyrase inhibitors suggesting a role of SMC in DNA folding. A defect in the SMC-like SbcC protein exacerbated the sensitivity to gyrase inhibitors of cells devoid of SMC. We also showed that the D. radiodurans SMC protein forms discrete foci at the periphery of the nucleoid suggesting that SMC could locally condense DNA. The phenotype of smc null mutant leads us to speculate that other, not yet identified, proteins drive the compact organization of the D. radiodurans nucleoid.

Published
2009
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20. A universal type IA topoisomerase fold.

Author

Duguet M, Serre MC, and Bouthier de La Tour C

Subjects
Amino Acid Sequence, Crystallography, X-Ray, Molecular Sequence Data, Phylogeny, Protein Conformation, Sequence Analysis, Protein, DNA Topoisomerases, Type I chemistry, Models, Molecular, Protein Folding, Thermotoga maritima chemistry
Abstract

A class of enzymes, called DNA topoisomerases, is responsible for controlling the topological state of cellular DNA. Among these, type IA topoisomerases form a vast family that is present in all living organisms, including higher eukaryotes, in which they play important roles in genome stability. The known 3D structures of three of these enzymes indicate that they share a common toroidal architecture. We previously showed that the toroidal structure could be split off from the core enzyme of Thermotoga maritima topoisomerase I by limited proteolysis. This structure is produced by the association of two tandemly repeated elementary folds in a head-to-tail orientation. By using a combination of structural and sequence data analysis, we show that the elementary fold of about 150 amino acid residues, referred to as the topofold, is likely to be present in the whole topoisomerase IA family. Within each enzyme, the successive topofolds share two conserved sequence motifs located at the base of the ring, and referred to as the MI and MII motifs. However, the overall sequences of the folds have largely diverged. By contrast, secondary and tertiary structures appear remarkably conserved. We suggest that this twofold repeat has evolved by gene duplication/fusion from an ancestral topofold.

Published
2006
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21. Proteolytic cleavage of the hyperthermophilic topoisomerase I from Thermotoga maritima does not impair its enzymatic properties.

Author

Cossard R, Viard T, Lamour V, Duguet M, and Bouthier de La Tour C

Subjects
Amino Acid Motifs, Bacterial Proteins, Binding Sites, DNA metabolism, DNA Topoisomerases, Type I chemistry, Peptide Fragments chemistry, Protein Conformation, DNA Topoisomerases, Type I metabolism, Endopeptidases metabolism, Thermotoga maritima enzymology
Abstract

Using limited proteolysis, we show that the hyperthermophilic topoisomerase I from Thermotoga maritima exhibits a unique hot spot susceptible to proteolytic attack with a variety of proteases. The remaining of the protein is resistant to further proteolysis, which suggests a compact folding of the thermophilic topoisomerase, when compared to its mesophilic Escherichia coli homologue. We further show that a truncated version of the T. maritima enzyme, lacking the last C-terminal 93 amino acids is more susceptible to proteolysis, which suggests that the C-terminal region of the topoisomerase may be important to maintain the compact folding of the enzyme. The hot spot of cleavage is located around amino acids 326-330 and probably corresponds to an exposed loop of the protein, near the active site tyrosine in charge of DNA cleavage and religation. Location of this protease sensitive region in the vicinity of bound DNA is consistent with the partial protection observed in the presence of different DNA substrates. Unexpectedly, although proteolysis splits the enzyme in two halves, each containing part of the motifs involved in catalysis, trypsin-digested topoisomerase I retains full DNA binding, cleavage, and relaxation activities, full thermostability and also the same hydrodynamic and spectral properties as undigested samples. This supports the idea that the two fragments which are generated by proteolysis remain correctly folded and tightly associated after proteolytic cleavage.

Published
2004
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23. Hyperthermophilic topoisomerase I from Thermotoga maritima. A very efficient enzyme that functions independently of zinc binding.

Author

Viard T, Lamour V, Duguet M, and Bouthier de la Tour C

Subjects
Amino Acid Motifs, Amino Acid Sequence, Base Sequence, Cloning, Molecular, Cytosine metabolism, DNA Primers, DNA Topoisomerases, Type I chemistry, DNA Topoisomerases, Type I isolation & purification, DNA, Kinetoplast metabolism, Electrophoresis, Polyacrylamide Gel, Molecular Sequence Data, Mutagenesis, Site-Directed, Protein Binding, Sequence Homology, Amino Acid, Spectrometry, Fluorescence, Substrate Specificity, DNA Topoisomerases, Type I metabolism, Thermotoga maritima enzymology, Zinc metabolism
Abstract

Topoisomerases, by controlling DNA supercoiling state, are key enzymes for adaptation to high temperatures in thermophilic organisms. We focus here on the topoisomerase I from the hyperthermophilic bacterium Thermotoga maritima (optimal growth temperature, 80 degrees C). To determine the properties of the enzyme compared with those of its mesophilic homologs, we overexpressed T. maritima topoisomerase I in Escherichia coli and purified it to near homogeneity. We show that T. maritima topoisomerase I exhibits a very high DNA relaxing activity. Mapping of the cleavage sites on a variety of single-stranded oligonucleotides indicates a strong preference for a cytosine at position -4 of the cleavage, a property shared by E. coli topoisomerase I and archaeal reverse gyrases. As expected, the mutation of the putative active site Tyr 288 to Phe led to a totally inactive protein. To investigate the role of the unique zinc motif (Cys-X-Cys-X(16)-Cys-X-Cys) present in T. maritima topoisomerase I, experiments have been performed with the protein mutated on the tetracysteine motif. Strikingly, the results show that zinc binding is not required for DNA relaxation activity, contrary to the E. coli enzyme. Furthermore, neither thermostability nor cleavage specificity is altered in this mutant. This finding opens the question of the role of the zinc-binding motif in T. maritima topoisomerase I and suggests that this hyperthermophilic topoisomerase possesses a different mechanism from its mesophilic homolog.

Published
2001
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24. Analyzing reverse gyrase activity.

Author

Duguet M, Jaxel C, Déclais AC, Confalonieri F, Marsault J, Bouthier de la Tour C, Nadal M, and Portemer C

Subjects
Adenosine Triphosphatases metabolism, Adenosine Triphosphate metabolism, Archaea enzymology, Bacteria enzymology, Catalysis, DNA Topoisomerases, Type II chemistry, DNA, Circular chemistry, DNA, Superhelical chemistry, DNA, Superhelical metabolism, Electrophoresis, Agar Gel, Nucleic Acid Conformation, Nucleic Acid Denaturation, Polyethylene Glycols pharmacology, Protein Structure, Tertiary, DNA Topoisomerases, Type I, DNA Topoisomerases, Type II analysis, DNA Topoisomerases, Type II metabolism, DNA, Circular metabolism
Published
2001
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26. Reverse gyrase from the hyperthermophilic bacterium Thermotoga maritima: properties and gene structure.

Author

Bouthier de la Tour C, Portemer C, Kaltoum H, and Duguet M

Subjects
Amino Acid Sequence, Base Sequence, Cloning, Molecular, DNA Topoisomerases, Type II genetics, DNA, Bacterial chemistry, DNA, Bacterial genetics, DNA, Superhelical chemistry, DNA, Superhelical genetics, Gram-Negative Anaerobic Straight, Curved, and Helical Rods classification, Molecular Sequence Data, Phylogeny, Sequence Homology, Amino Acid, DNA Topoisomerases, Type I, DNA Topoisomerases, Type II metabolism, Gram-Negative Anaerobic Straight, Curved, and Helical Rods enzymology
Abstract

The hyperthermophilic bacterium Thermotoga maritima MSB8 possesses a reverse gyrase whose enzymatic properties are very similar to those of archaeal reverse gyrases. It catalyzes the positive supercoiling of the DNA in an Mg2+- and ATP-dependent process. Its optimal temperature of activity is around 90 degrees C, and it is highly thermostable. We have cloned and DNA sequenced the corresponding gene (T. maritima topR). This is the first report describing the analysis of a gene encoding a reverse gyrase in bacteria. The T. maritima topR gene codes for a protein of 1,104 amino acids with a deduced molecular weight of 128,259, a value in agreement with that estimated from the denaturing gel electrophoresis of the purified enzyme. Like its archaeal homologs, the T. maritima reverse gyrase exhibits helicase and topoisomerase domains, and its sequence matches very well the consensus sequence for six reverse gyrases now available. Phylogenetic analysis shows that all reverse gyrases, including the T. maritima enzyme, form a very homogeneous group, distinct from the type I 5' topoisomerases of the TopA subfamily, for which we have previously isolated a representative gene in T. maritima (topA). The coexistence of these two distinct genes, coding for a reverse gyrase and an omega-like topoisomerase, respectively, together with the recent description of a gyrase in T. maritima (O. Guipaud, E. Marguet, K. M. Noll, C. Bouthier de la Tour, and P. Forterre, Proc. Natl. Acad. Sci. USA 94:10606-10611, 1977) addresses the question of the control of the supercoiling in this organism.

Published
1998
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27. Reverse gyrase gene from Sulfolobus shibatae B12: gene structure, transcription unit and comparative sequence analysis of the two domains.

Author

Jaxel C, Bouthier de la Tour C, Duguet M, and Nadal M

Subjects
Adenosine Triphosphate metabolism, Base Sequence, Cloning, Molecular, Consensus Sequence, DNA metabolism, DNA Topoisomerases, Type II chemistry, Hydrolysis, Molecular Sequence Data, Promoter Regions, Genetic, RNA chemistry, Sequence Alignment, Sequence Analysis, DNA, Zinc Fingers, DNA Topoisomerases, Type I, DNA Topoisomerases, Type II genetics, DNA, Bacterial chemistry, Genes, Bacterial, Sulfolobus genetics
Abstract

We cloned and sequenced a DNA fragment from the thermophilic archaeal strain Sulfolobus shibatae B12 that includes the gene topR encoding the reverse gyrase. The RNA of the reverse gyrase gene was characterized indicating that the topR gene is fully functional in vivo. We showed by primer extension analysis that transcription of topR initiates 28 bp downstream from a consensus A-box promoter. In order to understand how this particular type I DNA topoisomerase introduces positive superturns into the DNA, we compared the amino acid sequence of reverse gyrase from S.shibatae with the two other known reverse gyrases. This comparison indicates a common organization of these proteins: the carboxy-terminal domain is related to the type I-5' topoisomerase family while the amino-terminal domain possesses some motifs of proteins described as RNA or DNA helicases. By using local alignments, we showed that (i) reverse gyrases constitute a new and rather homogenous group within the type I-5' DNA topoisomerase family; (ii) a careful sequence analysis of the amino-terminal domain allows us to relate the presence of some motifs with an ATP binding and hydrolysis reaction coupled to a DNA binding and unwinding activity.

Published
1996
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28. Cloning and sequencing of the gene coding for topoisomerase I from the extremely thermophilic eubacterium, Thermotoga maritima.

Author

Bouthier de la Tour C, Kaltoum H, Portemer C, Confalonieri F, Huber R, and Duguet M

Subjects
Amino Acid Sequence, Base Sequence, Molecular Sequence Data, DNA Topoisomerases, Type I genetics, Genes, Bacterial, Gram-Negative Anaerobic Bacteria genetics
Abstract

A 2767 bp fragment containing a gene coding for a topoisomerase I from the extremely thermophilic eubacterium Thermotoga maritima (Tm TopA) has been cloned and sequenced. The protein is composed of 633 amino acids with a calculated molecular mass of 72,695 Da. It shares significant similarity with the topoisomerases I of mesophilic eubacteria. The highest score is obtained with Bacillus subtilis (44% identity); in particular, T. maritima and B. subtilis possess an insertion of 7-8 amino acids in the vicinity of the active site, that is absent in topoisomerases of other organisms. A specific feature of T. maritima topoisomerase I is its low cysteine content compared to its mesophilic homologs. It contains 5 cysteine residues, of which 4 could constitute a zinc finger motif. Finally, analysis of the regions flanking the gene reveals that Tm TopA is surrounded by two other ORFs, suggesting the occurrence of a polycistronic transcriptional unit.

Published
1995
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29. ATP-independent DNA topoisomerase from Fervidobacterium islandicum.

Author

Bouthier de la Tour C, Portemer C, Forterre P, Huber R, and Duguet M

Subjects
DNA, Superhelical, Enzyme Stability, Magnesium, Temperature, Thermoplasma enzymology, Topoisomerase I Inhibitors, DNA Topoisomerases, Type I isolation & purification
Abstract

Thermotogales are thermophilic eubacteria belonging to a very slowly evolving branch in the eubacterial tree. In this report, we describe the purification and characterization of an ATP-independent DNA topoisomerase from the Thermotogale, Fervidobacterium islandicum. The enzyme, a monomer of about 75 kDa, is a type I DNA topoisomerase sharing many properties with the other bacterial topoisomerases I: it absolutely requires Mg2+ for activity, relaxes negatively but not positively supercoiled DNA and is inhibited by single-stranded M13 DNA and spermidine. A feature of the F. islandicum ATP-independent DNA topoisomerase I is its thermophily. The optimal temperature for the enzymatic activity is 75 degrees C. Studies about thermostability show that the enzyme is more stable when incubated undiluted in the storage buffer. In these conditions, 60% activity was retained after a 30 min preincubation at 75 degrees C.

Published
1993
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