Modification de macromolécules par insertion radicalaire. Etude de la méthylthiotransférase RimO et de la 4-demethylwyosine synthase TYW1 appartenant toutes deux à la superfamille Radical SAM.

Over the last twenty years, the insertion reactions of atoms or molecular fragments into poorly reactive C-H bonds have been actively investigated but the details of their mechanisms remain largely unknown. Enzymes belonging to the "Radical-SAM" superfamily catalyze the activation of their substrate using a [4Fe-4S] in conjunction with the co-substrate S-adenosylmethionine (SAM). Radical insertion enzymes are a subgroup of this family and contain a second iron-sulfur cluster involved in the activation of the second substrate allowing the insertion reaction by radical coupling to take place. The work presented in this thesis is focusing on two enzymes, the first one, RimO is a methylthiotransferase (MTTase) that catalyzes the insertion of a thiomethyl group on the beta position of D89 residue of the ribosomal protein S12 (β-ms-D89-S12). The second one, TYW1, or 4-demethylwyosine synthase, catalyzes the insertion of the acetyl moiety of pyruvate into a C-H bond of a N-methyl group of a guanine derivative in some eukaryotic and archeal tRNAs. This insertion reaction leads to the formation of a tricyclic ring and through several steps to wybutosine (yW), a hypermodified nucleotide important for the translational fidelity of the cell. In this work we demonstrate that these radical inserting enzymes utilize the two iron-sulfur clusters to cooperate and that they control the different partners of the reaction by original redox mechanisms.Ces vingt dernières années, les réactions d'insertion d'atomes ou de fragments moléculaires dans des liaisons C-H peu réactives ont fait l'objet de nombreuses études sans que les mécanismes de ces réactions aient pu être établis. Les enzymes de la superfamille « Radical-SAM » catalysent l'activation de leur substrat en utilisant un centre [4Fe-4S] et le co-substrat S-adénosylméthionine (SAM). Les enzymes d'insertion radicalaire constituent un sous-groupe de cette famille et contiennent un second centre fer-soufre impliqué, lui, dans l'activation du deuxième substrat rendant ainsi possible la réaction d'insertion par couplage radicalaire. Le travail présenté dans cette thèse concerne deux de ces enzymes, la première, RimO, est une méthylthiotransférase (MTTase) qui catalyse l'insertion d'un groupement thiométhyle en beta du résidu D89 de la protéine ribosomale S12 (β-ms-D89-S12). La seconde TYW1 ou 4-demethylwyosine synthase catalyse l'insertion d'un groupement acétyle dérivé du pyruvate dans une liaison C-H d'un groupement N-CH3 appartenant à une guanine spécifique de certains ARNt eucaryotes. Cette réaction d'insertion est suivie d'une cyclisation conduisant en plusieurs étapes à la wybutosine (yW), une base tricyclique importante pour la fidélité traductionnelle de la cellule. Dans ce travail il a été montré que les deux centres de cette famille d'enzyme coopèrent pour ces réactions et contrôlent l'utilisation des différents acteurs par des mécanismes redox originaux

Modification de macromolécules par insertion radicalaire. Etude de la méthylthiotransférase RimO et de la 4-demethylwyosine synthase TYW1 appartenant toutes deux à la superfamille Radical SAM.

Over the last twenty years, the insertion reactions of atoms or molecular fragments into poorly reactive C-H bonds have been actively investigated but the details of their mechanisms remain largely unknown. Enzymes belonging to the "Radical-SAM" superfamily catalyze the activation of their substrate using a [4Fe-4S] in conjunction with the co-substrate S-adenosylmethionine (SAM). Radical insertion enzymes are a subgroup of this family and contain a second iron-sulfur cluster involved in the activation of the second substrate allowing the insertion reaction by radical coupling to take place. The work presented in this thesis is focusing on two enzymes, the first one, RimO is a methylthiotransferase (MTTase) that catalyzes the insertion of a thiomethyl group on the beta position of D89 residue of the ribosomal protein S12 (β-ms-D89-S12). The second one, TYW1, or 4-demethylwyosine synthase, catalyzes the insertion of the acetyl moiety of pyruvate into a C-H bond of a N-methyl group of a guanine derivative in some eukaryotic and archeal tRNAs. This insertion reaction leads to the formation of a tricyclic ring and through several steps to wybutosine (yW), a hypermodified nucleotide important for the translational fidelity of the cell. In this work we demonstrate that these radical inserting enzymes utilize the two iron-sulfur clusters to cooperate and that they control the different partners of the reaction by original redox mechanisms.Ces vingt dernières années, les réactions d'insertion d'atomes ou de fragments moléculaires dans des liaisons C-H peu réactives ont fait l'objet de nombreuses études sans que les mécanismes de ces réactions aient pu être établis. Les enzymes de la superfamille « Radical-SAM » catalysent l'activation de leur substrat en utilisant un centre [4Fe-4S] et le co-substrat S-adénosylméthionine (SAM). Les enzymes d'insertion radicalaire constituent un sous-groupe de cette famille et contiennent un second centre fer-soufre impliqué, lui, dans l'activation du deuxième substrat rendant ainsi possible la réaction d'insertion par couplage radicalaire. Le travail présenté dans cette thèse concerne deux de ces enzymes, la première, RimO, est une méthylthiotransférase (MTTase) qui catalyse l'insertion d'un groupement thiométhyle en beta du résidu D89 de la protéine ribosomale S12 (β-ms-D89-S12). La seconde TYW1 ou 4-demethylwyosine synthase catalyse l'insertion d'un groupement acétyle dérivé du pyruvate dans une liaison C-H d'un groupement N-CH3 appartenant à une guanine spécifique de certains ARNt eucaryotes. Cette réaction d'insertion est suivie d'une cyclisation conduisant en plusieurs étapes à la wybutosine (yW), une base tricyclique importante pour la fidélité traductionnelle de la cellule. Dans ce travail il a été montré que les deux centres de cette famille d'enzyme coopèrent pour ces réactions et contrôlent l'utilisation des différents acteurs par des mécanismes redox originaux

Control of the Evolution of Iron Peroxide Intermediate in Superoxide Reductase from Desulfoarculus baarsii. Involvement of Lysine 48 in Protonation

International audienceSuperoxide reductase is a nonheme iron metalloenzyme that detoxifies superoxide anion radicals O(2)(•-) in some microorganisms. Its catalytic mechanism was previously proposed to involve a single ferric iron (hydro)peroxo intermediate, which is protonated to form the reaction product H(2)O(2). Here, we show by pulse radiolysis that the mutation of the well-conserved lysine 48 into isoleucine in the SOR from Desulfoarculus baarsii dramatically affects its reaction with O(2)(•-). Although the first reaction intermediate and its decay are not affected by the mutation, H(2)O(2) is no longer the reaction product. In addition, in contrast to the wild-type SOR, the lysine mutant catalyzes a two-electron oxidation of an olefin into epoxide in the presence of H(2)O(2), suggesting the formation of iron-oxo intermediate species in this mutant. In agreement with the recent X-ray structures of the peroxide intermediates trapped in a SOR crystal, these data support the involvement of lysine 48 in the specific protonation of the proximal oxygen of the peroxide intermediate to generate H(2)O(2), thus avoiding formation of iron-oxo species, as is observed in cytochrome P450. In addition, we proposed that the first reaction intermediate observed by pulse radiolysis is a ferrous-iron superoxo species, in agreement with TD-DFT calculations of the absorption spectrum of this intermediate. A new reaction scheme for the catalytical mechanism of SOR with O(2)(•-) is presented in which ferrous iron-superoxo and ferric hydroperoxide species are reaction intermediates, and the lysine 48 plays a key role in the control of the evolution of iron peroxide intermediate to form H(2)O(2)

Modification of macromolecules by radical insertion. Study of the methylthiotransferase RimO and the 4-demethylwyosine synthase TYW1 both belonging to the Radical-SAM superfamily

Ces vingt dernières années, les réactions d'insertion d'atomes ou de fragments moléculaires dans des liaisons C-H peu réactives ont fait l'objet de nombreuses études sans que les mécanismes de ces réactions aient pu être établis. Les enzymes de la superfamille « Radical-SAM » catalysent l'activation de leur substrat en utilisant un centre [4Fe-4S] et le co-substrat S-adénosylméthionine (SAM). Les enzymes d'insertion radicalaire constituent un sous-groupe de cette famille et contiennent un second centre fer-soufre impliqué, lui, dans l'activation du deuxième substrat rendant ainsi possible la réaction d'insertion par couplage radicalaire. Le travail présenté dans cette thèse concerne deux de ces enzymes, la première, RimO, est une méthylthiotransférase (MTTase) qui catalyse l'insertion d'un groupement thiométhyle en beta du résidu D89 de la protéine ribosomale S12 (β-ms-D89-S12). La seconde TYW1 ou 4-demethylwyosine synthase catalyse l'insertion d'un groupement acétyle dérivé du pyruvate dans une liaison C-H d'un groupement N-CH3 appartenant à une guanine spécifique de certains ARNt eucaryotes. Cette réaction d'insertion est suivie d'une cyclisation conduisant en plusieurs étapes à la wybutosine (yW), une base tricyclique importante pour la fidélité traductionnelle de la cellule. Dans ce travail il a été montré que les deux centres de cette famille d'enzyme coopèrent pour ces réactions et contrôlent l'utilisation des différents acteurs par des mécanismes redox originaux.Over the last twenty years, the insertion reactions of atoms or molecular fragments into poorly reactive C-H bonds have been actively investigated but the details of their mechanisms remain largely unknown. Enzymes belonging to the "Radical-SAM" superfamily catalyze the activation of their substrate using a [4Fe-4S] in conjunction with the co-substrate S-adenosylmethionine (SAM). Radical insertion enzymes are a subgroup of this family and contain a second iron-sulfur cluster involved in the activation of the second substrate allowing the insertion reaction by radical coupling to take place. The work presented in this thesis is focusing on two enzymes, the first one, RimO is a methylthiotransferase (MTTase) that catalyzes the insertion of a thiomethyl group on the beta position of D89 residue of the ribosomal protein S12 (β-ms-D89-S12). The second one, TYW1, or 4-demethylwyosine synthase, catalyzes the insertion of the acetyl moiety of pyruvate into a C-H bond of a N-methyl group of a guanine derivative in some eukaryotic and archeal tRNAs. This insertion reaction leads to the formation of a tricyclic ring and through several steps to wybutosine (yW), a hypermodified nucleotide important for the translational fidelity of the cell. In this work we demonstrate that these radical inserting enzymes utilize the two iron-sulfur clusters to cooperate and that they control the different partners of the reaction by original redox mechanisms

Wybutosine biosynthesis: Structural and mechanistic overview

International audienceOver the last 10 years, significant progress has been made in understanding the genetics, enzymology and structural components of the wybutosine (yW) biosynthetic pathway. These studies have played a key role in expanding our understanding of yW biosynthesis and have revealed unexpected evolutionary ties, which are presently being unraveled. The enzymes catalyzing the 5 steps of this pathway, from genetically encoded guanosine to wybutosine base, provide an ensemble of amazing reaction mechanisms that are to be discussed in this review article

Unanticipated coordination of tris buffer to the Radical SAM cluster of the RimO methylthiotransferase

International audienceRadical SAM enzymes generally contain a [4Fe-4S](2+/1+) (RS cluster) cluster bound to the protein via the three cysteines of a canonical motif CxxxCxxC. The non-cysteinyl iron is used to coordinate SAM via its amino-carboxylate moiety. The coordination-induced proximity between the cluster acting as an electron donor and the adenosyl-sulfonium bond of SAM allows for the homolytic cleavage of the latter leading to the formation of the reactive 5'-deoxyadenosyl radical used for substrate activation. Most of the structures of Radical SAM enzymes have been obtained in the presence of SAM, and therefore, little is known about the situation when SAM is not present. In this report, we show that RimO, a methylthiotransferase belonging to the radical SAM superfamily, binds a Tris molecule in the absence of SAM leading to specific spectroscopic signatures both in Mössbauer and pulsed EPR spectroscopies. These data provide a cautionary note for researchers who work with coordinative unsaturated iron sulfur clusters

Redox Behavior of the S-Adenosylmethionine (SAM)-Binding Fe-S Cluster in Methylthiotransferase RimO, toward Understanding Dual SAM Activity

International audienceRimO, a radical-S-adenosylmethionine (SAM) enzyme, catalyzes the specific C3 methylthiolation of the D89 residue in the ribosomal S12 protein. Two intact iron–sulfur clusters and two SAM cofactors both are required for catalysis. By using electron paramagnetic resonance, Mössbauer spectroscopies, and site-directed mutagenesis, we show how two SAM molecules sequentially bind to the unique iron site of the radical-SAM cluster for two distinct chemical reactions in RimO. Our data establish that the two SAM molecules bind the radical-SAM cluster to the unique iron site, and spectroscopic evidence obtained under strongly reducing conditions supports a mechanism in which the first molecule of SAM causes the reoxidation of the reduced radical-SAM cluster, impeding reductive cleavage of SAM to occur and allowing SAM to methylate a HS– ligand bound to the additional cluster. Furthermore, by using density functional theory-based methods, we provide a description of the reaction mechanism that predicts the attack of the carbon radical substrate on the methylthio group attached to the additional [4Fe-4S] cluster

Control of the Evolution of Iron Peroxide Intermediate in Superoxide Reductase from Desulfoarculus baarsii. Involvement of Lysine 48 in Protonation

Superoxide reductase is a nonheme iron metalloenzyme that detoxifies superoxide anion radicals O₂^•– in some microorganisms. Its catalytic mechanism was previously proposed to involve a single ferric iron (hydro)­peroxo intermediate, which is protonated to form the reaction product H₂O₂. Here, we show by pulse radiolysis that the mutation of the well-conserved lysine 48 into isoleucine in the SOR from Desulfoarculus baarsii dramatically affects its reaction with O₂^•–. Although the first reaction intermediate and its decay are not affected by the mutation, H₂O₂ is no longer the reaction product. In addition, in contrast to the wild-type SOR, the lysine mutant catalyzes a two-electron oxidation of an olefin into epoxide in the presence of H₂O₂, suggesting the formation of iron-oxo intermediate species in this mutant. In agreement with the recent X-ray structures of the peroxide intermediates trapped in a SOR crystal, these data support the involvement of lysine 48 in the specific protonation of the proximal oxygen of the peroxide intermediate to generate H₂O₂, thus avoiding formation of iron-oxo species, as is observed in cytochrome P450. In addition, we proposed that the first reaction intermediate observed by pulse radiolysis is a ferrous-iron superoxo species, in agreement with TD-DFT calculations of the absorption spectrum of this intermediate. A new reaction scheme for the catalytical mechanism of SOR with O₂^•– is presented in which ferrous iron-superoxo and ferric hydroperoxide species are reaction intermediates, and the lysine 48 plays a key role in the control of the evolution of iron peroxide intermediate to form H₂O₂