Your search keyword '"Dos Santos PC"' showing total 15 results

1. Distribution of Nitrogen-Fixation Genes in Prokaryotes Containing Alternative Nitrogenases.

Author

Addo MA and Dos Santos PC

Subjects

Azotobacter vinelandii enzymology, Nitrogen Fixation genetics, Nitrogenase metabolism, Prokaryotic Cells metabolism

Abstract

Biological nitrogen fixation is an inherent trait exclusive to a select number of prokaryotes. Although molybdenum nitrogenase is the dominant catalyst for dinitrogen reduction, some diazotrophs also contain one or two additional types of nitrogenase that use alternative metal content as the active-site cofactor. The occurrence of alternative nitrogenases has not been well studied due to the discriminatory expression of the molybdenum nitrogenase and lack of comprehensive genomic data. This study reports on the genomic analysis of 87 unique species containing alternative nitrogenase sequences. The distribution of nitrogen-fixing genes within these species from distinct taxonomic groups shows the presence of the minimum gene set required for nitrogen fixation, including catalytic and biosynthetic enzymes of the Mo-dependent system (NifHDKENB) and the varying occurrence of additional Nif-dedicated components. These include NifS and NifU, found primarily in aerobic species, thus suggesting that these genes are necessary to accommodate the high demand for Fe-S clusters during aerobic nitrogen fixation., (© 2020 Wiley-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2020

2. Distribution of nitrogen fixation and nitrogenase-like sequences amongst microbial genomes.

Author

Dos Santos PC, Fang Z, Mason SW, Setubal JC, and Dixon R

Subjects

Amino Acid Sequence, Archaea classification, Archaea enzymology, Archaea genetics, Archaeal Proteins chemistry, Archaeal Proteins genetics, Bacteria classification, Bacteria enzymology, Bacteria genetics, Bacterial Proteins chemistry, Bacterial Proteins genetics, Base Sequence, Biodiversity, Biosynthetic Pathways genetics, Conserved Sequence genetics, Genes, Archaeal genetics, Genes, Bacterial genetics, Molecular Sequence Data, Nitrogenase chemistry, Nitrogenase metabolism, Phylogeny, Reference Standards, Sequence Alignment, Species Specificity, Genome, Archaeal genetics, Genome, Bacterial genetics, Nitrogen Fixation genetics, Nitrogenase genetics

Abstract

Background: The metabolic capacity for nitrogen fixation is known to be present in several prokaryotic species scattered across taxonomic groups. Experimental detection of nitrogen fixation in microbes requires species-specific conditions, making it difficult to obtain a comprehensive census of this trait. The recent and rapid increase in the availability of microbial genome sequences affords novel opportunities to re-examine the occurrence and distribution of nitrogen fixation genes. The current practice for computational prediction of nitrogen fixation is to use the presence of the nifH and/or nifD genes., Results: Based on a careful comparison of the repertoire of nitrogen fixation genes in known diazotroph species we propose a new criterion for computational prediction of nitrogen fixation: the presence of a minimum set of six genes coding for structural and biosynthetic components, namely NifHDK and NifENB. Using this criterion, we conducted a comprehensive search in fully sequenced genomes and identified 149 diazotrophic species, including 82 known diazotrophs and 67 species not known to fix nitrogen. The taxonomic distribution of nitrogen fixation in Archaea was limited to the Euryarchaeota phylum; within the Bacteria domain we predict that nitrogen fixation occurs in 13 different phyla. Of these, seven phyla had not hitherto been known to contain species capable of nitrogen fixation. Our analyses also identified protein sequences that are similar to nitrogenase in organisms that do not meet the minimum-gene-set criteria. The existence of nitrogenase-like proteins lacking conserved co-factor ligands in both diazotrophs and non-diazotrophs suggests their potential for performing other, as yet unidentified, metabolic functions., Conclusions: Our predictions expand the known phylogenetic diversity of nitrogen fixation, and suggest that this trait may be much more common in nature than it is currently thought. The diverse phylogenetic distribution of nitrogenase-like proteins indicates potential new roles for anciently duplicated and divergent members of this group of enzymes.

Published

2012

3. A substrate channel in the nitrogenase MoFe protein.

Author

Barney BM, Yurth MG, Dos Santos PC, Dean DR, and Seefeldt LC

Subjects

Azotobacter vinelandii genetics, Colorimetry, Electron Spin Resonance Spectroscopy, Genetic Complementation Test, Kinetics, Models, Molecular, Molybdenum analysis, Molybdoferredoxin genetics, Molybdoferredoxin metabolism, Mutagenesis, Site-Directed, Mutant Proteins chemistry, Mutant Proteins isolation & purification, Mutant Proteins metabolism, Nitrogenase metabolism, Software, Substrate Specificity genetics, Azotobacter vinelandii enzymology, Catalytic Domain, Molybdoferredoxin chemistry, Nitrogenase chemistry

Abstract

Nitrogenase catalyzes the six electron/six proton reduction of N2 to two ammonia molecules at a complex organometallocluster called "FeMo cofactor." This cofactor is buried within the alpha-subunit of the MoFe protein, with no obvious access for substrates. Examination of high-resolution X-ray crystal structures of MoFe proteins from several organisms has revealed the existence of a water-filled channel that extends from the solvent-exposed surface to a specific face of FeMo cofactor. This channel could provide a pathway for substrate and product access to the active site. In the present work, we examine this possibility by substituting four different amino acids that line the channel with other residues and analyze the impact of these substitutions on substrate reduction kinetic parameters. Each of the MoFe protein variants was purified and kinetic parameters were established for the reduction of the substrates N2, acetylene, azide, and propyne. For each MoFe protein, V (max) values for the different substrates were found to be nearly unchanged when compared with the values for the wild-type MoFe protein, indicating that electron delivery to the active site is not compromised by the various substitutions. In contrast, the K(m) values for these substrates were found to increase significantly (up to 22-fold) in some of the MoFe protein variants compared with the wild-type MoFe protein values. Given that each of the amino acids that were substituted is remote from the active site, these results are consistent with the water-filled channel functioning as a substrate channel in the MoFe protein.

Published

2009

4. Alkyne substrate interaction within the nitrogenase MoFe protein.

Author

Dos Santos PC, Mayer SM, Barney BM, Seefeldt LC, and Dean DR

Subjects

Alkynes metabolism, Azotobacter vinelandii genetics, Azotobacter vinelandii growth & development, Azotobacter vinelandii metabolism, Binding Sites, Models, Molecular, Molecular Structure, Molybdoferredoxin genetics, Molybdoferredoxin metabolism, Nitrogenase genetics, Nitrogenase metabolism, Oxidation-Reduction, Alkynes chemistry, Molybdoferredoxin chemistry, Nitrogenase chemistry

Abstract

Nitrogenase catalyzes the biological reduction of N(2) to ammonia (nitrogen fixation), as well as the two-electron reduction of the non-physiological alkyne substrate acetylene (HC triple bond CH). A complex metallo-organic species called FeMo-cofactor provides the site of substrate reduction within the MoFe protein, but exactly where and how substrates interact with FeMo-cofactor remains unknown. Recent results have shown that the MoFe protein alpha-70(Val) residue, whose side chain approaches one Fe-S face of FeMo-cofactor, plays a significant role in defining substrate access to the active site. For example, substitution of alpha-70(Val) by alanine results in an increased capacity for the reduction of the larger alkyne propyne (HC triple bond C-CH(3)), whereas, substitution by isoleucine at this position nearly eliminates the capacity for the reduction of acetylene. These and complementary spectroscopic studies led us to propose that binding of short chain alkynes occurs with side-on binding to Fe atom 6 within FeMo-cofactor. In the present work, the alpha-70(Val) residue was substituted by glycine and this MoFe protein variant shows an increased capacity for reduction of the terminal alkyne, 1-butyne (HC triple bond C-CH(2)-CH(3)). This protein shows no detectable reduction of the internal alkyne 2-butyne (H(3)C-C triple bond C-CH(3)). In contrast, substitution of the nearby alpha-191(Gln) residue by alanine, in combination with the alpha-70(Ala) substitution, does result in significant reduction of 2-butyne, with the exclusive product being 2-cis-butene. These results indicate that the reduction of alkynes by nitrogenases involves side-on binding of the alkyne to Fe6 within FeMo-cofactor, and that a terminal acidic proton is not required for reduction. The successful design of amino acid substitutions that permit the targeted accommodation of an alkyne that otherwise is not a nitrogenase substrate provides evidence to support the current model for alkyne interaction within the nitrogenase MoFe protein.

Published

2007

5. Breaking the N2 triple bond: insights into the nitrogenase mechanism.

Author

Barney BM, Lee HI, Dos Santos PC, Hoffman BM, Dean DR, and Seefeldt LC

Subjects

Electron Spin Resonance Spectroscopy, Hydrazines chemistry, Imides chemistry, Models, Chemical, Models, Molecular, Molybdoferredoxin chemistry, Oxidation-Reduction, Protein Conformation, Nitrogen chemistry, Nitrogenase chemistry

Abstract

Nitrogenase is the metalloenzyme that performs biological nitrogen fixation by catalyzing the reduction of N2 to ammonia. Understanding how the nitrogenase active site metal cofactor (FeMo-cofactor) catalyzes the cleavage of the N2 triple bond has been the focus of intense study for more than 50 years. Goals have included the determination of where and how substrates interact with the FeMo-cofactor, and the nature of reaction intermediates along the reduction pathway. Progress has included the trapping of intermediates formed during turnover of non-physiological substrates (e.g., alkynes, CS2) providing insights into how these molecules interact with the nitrogenase FeMo-cofactor active site. More recently, substrate-derived species have been trapped at high concentrations during the reduction of N2, a diazene, and hydrazine, providing the first insights into binding modes and possible mechanisms for N2 reduction. A comparison of the current state of knowledge of the trapped species arising from non-physiological substrates and nitrogenous substrates is beginning to reveal some of the intricacies of how nitrogenase breaks the N2 triple bond.

Published

2006

6. Intermediates trapped during nitrogenase reduction of N triple bond N, CH3-N=NH, and H2N-NH2.

Author

Barney BM, Yang TC, Igarashi RY, Dos Santos PC, Laryukhin M, Lee HI, Hoffman BM, Dean DR, and Seefeldt LC

Subjects

Binding Sites, Catalytic Domain, Electron Spin Resonance Spectroscopy, Molybdoferredoxin chemistry, Oxidation-Reduction, Amides chemistry, Amines chemistry, Molybdoferredoxin metabolism, Nitrogen chemistry, Nitrogenase metabolism

Abstract

A high population intermediate has been trapped on the nitrogenase active site FeMo cofactor during reduction of N2. In addition, intermediates have been trapped during reduction of CH3-N=NH by the alpha-195Gln variant and during reduction of H2N-NH2 by the alpha-70Ala/alpha-195Gln variant. Each of these trapped states shows an EPR signal arising from an S = 1/2 state of the FeMo cofactor. 15N ENDOR shows that each intermediate has a nitrogenous species bound to the FeMo cofactor, with a single type of N seen for each bound intermediate. The g tensors are unique to each intermediate, g(e) = [2.084, 1.993, 1.969], g(m) = [2.083, 2.021, 1.993], g(l) = [2.082, 2.015, 1.987], as are the 15N hyperfine couplings at g1, which suggests that three distinct stages of NN reduction may have been trapped. The 1H ENDOR spectra show that the N2 intermediate is at a distinct and earlier stage of reduction from the other two, so at least two stages of NN reduction have been trapped. Some possible structures of the hydrazine intermediate are presented.

Published

2005

7. NifS-mediated assembly of [4Fe-4S] clusters in the N- and C-terminal domains of the NifU scaffold protein.

Author

Smith AD, Jameson GN, Dos Santos PC, Agar JN, Naik S, Krebs C, Frazzon J, Dean DR, Huynh BH, and Johnson MK

Subjects

Bacterial Proteins biosynthesis, Bacterial Proteins metabolism, Dimerization, Iron-Sulfur Proteins biosynthesis, Nitrogen Fixation, Protein Structure, Tertiary, Spectrum Analysis, Bacterial Proteins chemistry, Iron-Sulfur Proteins chemistry, Nitrogenase biosynthesis, Transaminases metabolism

Abstract

NifU is a homodimeric modular protein comprising N- and C-terminal domains and a central domain with a redox-active [2Fe-2S](2+,+) cluster. It plays a crucial role as a scaffold protein for the assembly of the Fe-S clusters required for the maturation of nif-specific Fe-S proteins. In this work, the time course and products of in vitro NifS-mediated iron-sulfur cluster assembly on full-length NifU and truncated forms involving only the N-terminal domain or the central and C-terminal domains have been investigated using UV-vis absorption and Mössbauer spectroscopies, coupled with analytical studies. The results demonstrate sequential assembly of labile [2Fe-2S](2+) and [4Fe-4S](2+) clusters in the U-type N-terminal scaffolding domain and the assembly of [4Fe-4S](2+) clusters in the Nfu-type C-terminal scaffolding domain. Both scaffolding domains of NifU are shown to be competent for in vitro maturation of nitrogenase component proteins, as evidenced by rapid transfer of [4Fe-4S](2+) clusters preassembled on either the N- or C-terminal domains to the apo nitrogenase Fe protein. Mutagenesis studies indicate that a conserved aspartate (Asp37) plays a critical role in mediating cluster transfer. The assembly and transfer of clusters on NifU are compared with results reported for U- and Nfu-type scaffold proteins, and the need for two functional Fe-S cluster scaffolding domains on NifU is discussed.

Published

2005

8. Trapping a hydrazine reduction intermediate on the nitrogenase active site.

Author

Barney BM, Laryukhin M, Igarashi RY, Lee HI, Dos Santos PC, Yang TC, Hoffman BM, Dean DR, and Seefeldt LC

Subjects

Azotobacter vinelandii enzymology, Binding Sites, Electron Spin Resonance Spectroscopy methods, Enzyme Inhibitors chemistry, Molybdoferredoxin chemistry, Molybdoferredoxin metabolism, Nitrogen chemistry, Nitrogen metabolism, Nitrogenase antagonists & inhibitors, Oxidation-Reduction, Protons, Substrate Specificity, Hydrazines chemistry, Nitrogenase chemistry, Nitrogenase metabolism

Abstract

A major challenge in understanding the mechanism of nitrogenase, the enzyme responsible for the biological fixation of N(2) to two ammonias, is to trap a nitrogenous substrate at the enzyme active site in a state that is amenable to further characterization. In the present work, a strategy is described that results in the trapping of the substrate hydrazine (H(2)N-NH(2)) as an adduct bound to the active site metal cluster of nitrogenase, and this bound adduct is characterized by EPR and ENDOR spectroscopies. Earlier work has been interpreted to indicate that nitrogenous (e.g., N(2) and hydrazine) as well as alkyne (e.g., acetylene) substrates can bind at a common FeS face of the FeMo-cofactor composed of Fe atoms 2, 3, 6, and 7. Substitution of alpha-70(Val) that resides over this FeS face by the smaller amino acid alanine was also previously shown to improve the affinity and reduction rate for hydrazine. We now show that when alpha-195(His), a putative proton donor near the active site, is substituted by glutamine in combination with substitution of alpha-70(Val) by alanine, and the resulting doubly substituted MoFe protein (alpha-70(Ala)/alpha-195(Gln)) is turned over with hydrazine as substrate, the FeMo-cofactor can be freeze-trapped in a S = (1)/(2) state in high yield ( approximately 70%). The presumed hydrazine-FeMo-cofactor adduct displays a rhombic EPR signal with g = [2.09, 2.01, 1.93]. The optimal pH for the population of this state was found to be 7.4. The EPR signal showed a Curie law temperature dependence similar to the resting state EPR signal. Mims pulsed ENDOR spectroscopy at 35 GHz using (15)N-labeled hydrazine reveals that the trapped intermediate incorporates a hydrazine-derived species bound to the FeMo-cofactor; in spectra taken at g(1) this species gives a single observed (15)N signal, A(g(1)) = 1.5 MHz.

Published

2005

9. Trapping H- bound to the nitrogenase FeMo-cofactor active site during H2 evolution: characterization by ENDOR spectroscopy.

Author

Igarashi RY, Laryukhin M, Dos Santos PC, Lee HI, Dean DR, Seefeldt LC, and Hoffman BM

Subjects

Binding Sites, Electron Spin Resonance Spectroscopy, Hydrogen metabolism, Hydrogen-Ion Concentration, Models, Molecular, Molybdoferredoxin metabolism, Nitrogenase metabolism, Oxidation-Reduction, Protons, Sulfides chemistry, Hydrogen chemistry, Molybdoferredoxin chemistry, Nitrogenase chemistry

Abstract

We here show that the iron-molybdenum (FeMo)-cofactor of the nitrogenase alpha-70(Ile) molybdenum-iron (MoFe) protein variant accumulates a novel S = (1)/(2) state that can be trapped during the reduction of protons to H(2). (1,2)H-ENDOR measurements disclose the presence of two protons/hydrides (H(+/)(-)) whose hyperfine tensors have been determined from two-dimensional field-frequency (1)H ENDOR plots. The two H(+/)(-) have large isotropic hyperfine couplings, A(iso)( )() approximately 23 MHz, which shows they are bound to the cofactor. The favored analysis for these plots indicates that the two H(+/)(-) have the same principal values, which indicates that they are chemically equivalent. The tensors are further related to each other by a permutation of the tensor components, which indicates an underlying symmetry of binding relative to the cofactor. At present, no model for the structure of the iron-molybdenum (FeMo)-cofactor in the S = (1)/(2) state trapped during the reduction of H(+) can be shown unequivocally to satisfy all of the constraints generated by the ENDOR analysis. The data disfavors any model that involves protonation of sulfides, and thus suggests that the intermediate instead contains two chemically equivalent bound hydrides; it appears unlikely that these are terminal monohydrides.

Published

2005

10. Substrate interactions with the nitrogenase active site.

Author

Dos Santos PC, Igarashi RY, Lee HI, Hoffman BM, Seefeldt LC, and Dean DR

Subjects

Alkynes chemistry, Binding Sites, Electron Spin Resonance Spectroscopy, Models, Molecular, Molecular Structure, Nitrogenase genetics, Propanols chemistry, Nitrogen chemistry, Nitrogen Fixation, Nitrogenase chemistry, Nitrogenase metabolism

Abstract

The chemical mechanism for biological cleavage of the N(2) triple bond at ambient pressure and temperature has been the subject of intense study for many years. The site of substrate activation and reduction has been localized to a complex cofactor, called FeMo cofactor, yet until now the complexity of the system has denied information concerning exactly where and how substrates interact with the metal-sulfur framework of the active site. In this Account, we describe a combined genetic, biophysical, and biochemical approach that was used to provide direct and detailed information concerning where alternative alkyne substrates interact with FeMo cofactor during catalysis. The relevance and limitations of this work with respect to N(2) binding and reduction also are discussed.

Published

2005

11. NifU and NifS are required for the maturation of nitrogenase and cannot replace the function of isc-gene products in Azotobacter vinelandii.

Author

Johnson DC, Dos Santos PC, and Dean DR

Subjects

Azotobacter vinelandii enzymology, Multigene Family, Azotobacter vinelandii metabolism, Bacterial Proteins physiology, Genes, Bacterial, Nitrogenase metabolism

Abstract

In recent years, it has become evident that [Fe-S] proteins, such as hydrogenase, nitrogenase and aconitase, require a complex machinery to assemble and insert their associated [Fe-S] clusters. So far, three different types of [Fe-S] cluster biosynthetic systems have been identified and these have been designated nif, isc and suf. In the present work, we show that the nif-specific [Fe-S] cluster biosynthetic system from Azotobacter vinelandii, which is required for nitrogenase maturation, cannot functionally replace the isc [Fe-S] cluster system used for the maturation of other [Fe-S] proteins, such as aconitase. The results indicate that, in certain cases, [Fe-S] cluster biosynthetic machineries have evolved to perform only specialized functions.

Published

2005

12. Substrate interaction at an iron-sulfur face of the FeMo-cofactor during nitrogenase catalysis.

Author

Barney BM, Igarashi RY, Dos Santos PC, Dean DR, and Seefeldt LC

Subjects

Acetylene chemistry, Alanine chemistry, Azotobacter vinelandii metabolism, Binding Sites, Catalysis, Dose-Response Relationship, Drug, Hydrazines chemistry, Hydrazines pharmacology, Hydrogen-Ion Concentration, Iron chemistry, Isoleucine chemistry, Kinetics, Macromolecular Substances, Models, Chemical, Models, Molecular, Nitrogen chemistry, Oxidation-Reduction, Protein Binding, Substrate Specificity, Molybdoferredoxin chemistry, Nitrogenase chemistry

Abstract

Nitrogenase catalyzes biological dinitrogen fixation, the reduction of N(2) to 2NH(3). Recently, the binding site for a non-physiological alkyne substrate (propargyl alcohol, HC triple bond C-CH(2)OH) was localized to a specific Fe-S face of the FeMo-cofactor approached by the MoFe protein amino acid alpha-70(Val). Here we provide evidence to indicate that the smaller alkyne substrate acetylene (HC triple bond CH), the physiological substrate dinitrogen, and its semi-reduced form hydrazine (H(2)N-NH(2)) interact with the same Fe-S face of the FeMo-cofactor. Hydrazine is a relatively poor substrate for the wild-type (alpha-70(Val)) MoFe protein. Substitution of the alpha-70(Val) residue by an amino acid having a smaller side chain (alanine) dramatically enhanced hydrazine reduction activity. Conversely, substitution of alpha-70(Val) by an amino acid having a larger side chain (isoleucine) significantly lowered the capacity of the MoFe protein to reduce dinitrogen, hydrazine, or acetylene.

Published

2004

13. Localization of a catalytic intermediate bound to the FeMo-cofactor of nitrogenase.

Author

Igarashi RY, Dos Santos PC, Niehaus WG, Dance IG, Dean DR, and Seefeldt LC

Subjects

Acetylene, Alanine chemistry, Azotobacter, Binding Sites, Catalytic Domain, Electron Spin Resonance Spectroscopy, Histidine chemistry, Hydrogen-Ion Concentration, Imidazoles chemistry, Iron, Kinetics, Magnetics, Models, Chemical, Models, Molecular, Protein Binding, Valine chemistry, Azotobacter vinelandii enzymology, Molybdoferredoxin chemistry, Nitrogenase chemistry

Abstract

Nitrogenase catalyzes the biological reduction of N(2) to ammonia (nitrogen fixation) as well as the reduction of a number of alternative substrates, including acetylene (HC identical with CH) to ethylene (H2C=CH2). It is known that the metallocluster FeMo-cofactor located within the nitrogenase MoFe protein component provides the site of substrate reduction, but the exact site where substrates bind and are reduced on the FeMo-cofactor remains unknown. We have recently shown that the alpha-70 residue of the MoFe protein plays a significant role in defining substrate access to the active site; alpha-70 approaches one face of the FeMo-cofactor, and when valine is substituted by alanine at this position, the substituted nitrogenase is able to accommodate a reduction of the larger alkyne propargyl alcohol (HC identical with CCH(2)OH, propargyl-OH). During this reduction, a substrate-derived intermediate can be trapped on the FeMo-cofactor resulting in an S = 1/2 spin system with a novel electron paramagnetic resonance spectrum. In the present work, trapping of the propargyl-OH-derived or propargyl amine (HC identical with CCH(2)NH(2), propargyl-NH(2))-derived intermediates is shown to be dependent on pH and the presence of histidine at position alpha-195. It is concluded that these catalytic intermediates are stabilized and thereby trapped by H-bonding interactions between either the-OH group or the-NH(3)(+)group and the imidazole epsilon-NH of alpha-195(His). Thus, for the first time it is possible to establish the location of a bound substrate-derived intermediate on the FeMo-cofactor. Refinement of the binding mode and site was accomplished by the use of density functional and force field calculations pointing to an eta(2) coordination at Fe-6 of the FeMo-cofactor.

Published

2004

14. An organometallic intermediate during alkyne reduction by nitrogenase.

Author

Lee HI, Igarashi RY, Laryukhin M, Doan PE, Dos Santos PC, Dean DR, Seefeldt LC, and Hoffman BM

Subjects

Alkynes metabolism, Azotobacter vinelandii enzymology, Carbon Isotopes, Electron Spin Resonance Spectroscopy methods, Models, Molecular, Molecular Conformation, Molybdoferredoxin chemistry, Molybdoferredoxin metabolism, Nitrogenase metabolism, Oxidation-Reduction, Propanols chemistry, Propanols metabolism, Alkynes chemistry, Nitrogenase chemistry

Abstract

Nitrogenase is the metalloenzyme that catalyzes the nucleotide-dependent reduction of N(2), as well as reduction of a variety of other triply bonded substrates, including the alkyne, acetylene. Substitution of the alpha-70(Val) residue in the nitrogenase MoFe protein by alanine expands the range of substrates to include short-chain alkynes not reduced by the unaltered protein. Rapid freezing of the alpha-70(Ala) nitrogenase MoFe protein during reduction of the alkyne propargyl alcohol (HC triple bond CH(2)OH; PA) traps an S = (1)/(2) intermediate state of the active-site metal cluster, the FeMo-cofactor. We have combined CW and pulsed (13)C ENDOR (electron-nuclear double resonance) with two quantitative 35 GHz (1,2)H ENDOR techniques, Mims pulsed ENDOR and the newly devised "stochastic field-modulated" ENDOR, to study this intermediate prepared with isotopically substituted ((13)C, (1,2)H) propargyl alcohol in H(2)O and D(2)O buffers. These measurements allow the first description of a trapped nitrogenase reduction intermediate. The S = (1)/(2) turnover intermediate generated during the reduction of PA contains the 3-carbon chain of PA and exhibits resolved (1,2)H ENDOR signals from three protons, two strongly coupled (H(a)) and one weakly coupled (H(b)); H(a)(c) originates as the C3 proton of PA, while H(a)(s) and H(b) are solvent-derived. The two H(a) protons have identical hyperfine tensors, despite having different origins. The equality of the (H(a)(s), H(a)(c)) hyperfine tensors strongly constrains proposals for the structure of the cluster-bound reduced PA. Through consideration of model structures found in the Cambridge Structural Database, we propose that the intermediate contains a novel bio-organometallic complex in which a reduction product of propargyl alcohol binds as a metalla-cyclopropane ring to a single Fe atom of the Fe-S face of the FeMo-cofactor that is composed of Fe atoms 2, 3, 6, and 7. Of the two most attractive structures, one singly reduced at C3 (4), the other being the doubly reduced allyl alcohol product (6), we tentatively favor 6 because of the "natural" assignment it affords for H(b).

Published

2004

15. Formation and insertion of the nitrogenase iron-molybdenum cofactor.

Author

Dos Santos PC, Dean DR, Hu Y, and Ribbe MW

Subjects

Amino Acid Sequence, Models, Molecular, Molecular Sequence Data, Molybdoferredoxin biosynthesis, Molybdoferredoxin metabolism, Nitrogenase metabolism, Oxidation-Reduction, Molybdoferredoxin chemistry, Nitrogenase chemistry

Published

2004