Your search keyword '"Rokita SE"' showing total 94 results

1. Accumulation of thymine dimers in DNA

Author

Finch, AS, Ito, T, Rokita, SE, Finch, AS, Ito, T, and Rokita, SE

Published

2005

2. Polar Interactions between Substrate and Flavin Control Iodotyrosine Deiodinase Function.

Author

Lemen D and Rokita SE

Subjects

Flavins metabolism, Flavins chemistry, Substrate Specificity, Oxidation-Reduction, Kinetics, Flavin-Adenine Dinucleotide metabolism, Flavin-Adenine Dinucleotide chemistry, Flavin-Adenine Dinucleotide analogs & derivatives, Dinitrocresols metabolism, Dinitrocresols chemistry, Halogenation, Iodide Peroxidase metabolism, Iodide Peroxidase chemistry

Abstract

Flavin cofactors offer a wide range of chemical mechanisms to support a great diversity in catalytic function. As a corollary, such diversity necessitates careful control within each flavoprotein to limit its function to an appropriate subset of possible reactions and substrates. This task falls to the protein environment surrounding the flavin in most enzymes. For iodotyrosine deiodinase that catalyzes a reductive dehalogenation of halotyrosines, substrates can dictate the chemistry available to the flavin. Their ability to stabilize the necessary one-electron reduced semiquinone form of flavin strictly depends on a direct coordination between the flavin and α-ammonium and carboxylate groups of its substrates. While perturbations to the carboxylate group do not significantly affect binding to the resting oxidized form of the deiodinase, dehalogenation ( k cat / K m ) is suppressed by over 2000-fold. Lack of the α-ammonium group abolishes detectable binding and dehalogenation. Substitution of the ammonium group with a hydroxyl group does not restore measurable binding but does support dehalogenation with an efficiency greater than those of the carboxylate derivatives. Consistent with these observations, the flavin semiquinone does not accumulate during redox titration in the presence of inert substrate analogues lacking either the α-ammonium or carboxylate groups. As a complement, a nitroreductase activity based on hydride transfer is revealed for the appropriate substrates with perturbations to their zwitterion.

Published

2024

3. 19 F NMR Reveals the Dynamics of Substrate Binding and Lid Closure for Iodotyrosine Deiodinase as a Complement to Steady-State Kinetics and Crystallography.

Author

Greenberg HC, Majumdar A, Cheema EK, Kozyryev A, and Rokita SE

Subjects

Kinetics, Crystallography, X-Ray methods, Nuclear Magnetic Resonance, Biomolecular, Protein Conformation, Substrate Specificity, Humans, Fluorine chemistry, Fluorine metabolism, Models, Molecular, Protein Binding, Ligands, Iodide Peroxidase metabolism, Iodide Peroxidase chemistry, Catalytic Domain

Abstract

Active site lids are common features of enzymes and typically undergo conformational changes upon substrate binding to promote catalysis. Iodotyrosine deiodinase is no exception and contains a lid segment in all of its homologues from human to bacteria. The solution-state dynamics of the lid have now been characterized using 19 F NMR spectroscopy with a CF 3 -labeled enzyme and CF 3 O-labeled ligands. From two-dimensional 19 F- 19 F NMR exchange spectroscopy, interconversion rates between the free and bound states of a CF 3 O-substituted tyrosine (45 ± 10 s -1 ) and the protein label (40 ± 3 s -1 ) are very similar and suggest a correlation between ligand binding and conformational reorganization of the lid. Both occur at rates that are ∼100-fold faster than turnover, and therefore these steps do not limit catalysis. A simple CF 3 O-labeled phenol also binds to the active site and induces a conformational change in the lid segment that was not previously detectable by crystallography. Exchange rates of the ligand (130 ± 20 s -1 ) and protein (98 ± 8 s -1 ) in this example are faster than those above but remain self-consistent to affirm a correlation between ordering of the lid and binding of the ligand. Both ligands also protect the protein from limited proteolysis, as expected from their ability to stabilize a compact lid structure. However, the minimal turnover of simple phenol substrates indicates that such stabilization may be necessary but is not sufficient for efficient catalysis.

Published

2024

4. Misregulation of bromotyrosine compromises fertility in male Drosophila .

Author

Su Q, Xu B, Chen X, and Rokita SE

Subjects

Animals, Male, Drosophila melanogaster metabolism, Drosophila melanogaster genetics, Drosophila genetics, Drosophila metabolism, Animals, Genetically Modified, Hydrolases metabolism, Hydrolases genetics, Fertility, Drosophila Proteins metabolism, Drosophila Proteins genetics, Spermatogenesis, Tyrosine metabolism, Tyrosine analogs & derivatives

Abstract

Biological regulation often depends on reversible reactions such as phosphorylation, acylation, methylation, and glycosylation, but rarely halogenation. A notable exception is the iodination and deiodination of thyroid hormones. Here, we report detection of bromotyrosine and its subsequent debromination during Drosophila spermatogenesis. Bromotyrosine is not evident when Drosophila express a native flavin-dependent dehalogenase that is homologous to the enzyme responsible for iodide salvage from iodotyrosine in mammals. Deletion or suppression of the dehalogenase-encoding condet ( cdt ) gene in Drosophila allows bromotyrosine to accumulate with no detectable chloro- or iodotyrosine. The presence of bromotyrosine in the cdt mutant males disrupts sperm individualization and results in decreased fertility. Transgenic expression of the cdt gene in late-staged germ cells rescues this defect and enhances tolerance of male flies to bromotyrosine. These results are consistent with reversible halogenation affecting Drosophila spermatogenesis in a process that had previously eluded metabolomic, proteomic, and genomic analyses., Competing Interests: Competing interests statement:The authors declare no competing interest.

Published

2024

5. The 2'-hydroxy group of flavin mononucleotide influences the catalytic function and promiscuity of the flavoprotein iodotyrosine dehalogenase.

Author

Kozyryev A, Boucher PA, Quiñones-Jurgensen CM, and Rokita SE

Abstract

The isoalloxazine ring system of the flavin cofactor is responsible for much of the catalytic power and diversity associated with flavoproteins. While the specificity of these enzymes is greatly influenced by the surrounding protein environment, the ribityl group of the cofactor may also participate in stabilizing transient intermediates formed by substrates and flavin. A conserved interaction between the phenolate oxygen of l-iodotyrosine and the 2'-hydroxy group of flavin mononucleotide (FMN) bound to iodotyrosine deiodianase (IYD) implied such a contribution to catalysis. Reconstitution of this deiodinase with 2'-deoxyflavin mononucleotide (2'-deoxyFMN) decreased the overall catalytic efficiency of l-iodotyrosine dehalogenation ( k cat / K m ) by more than 5-fold but increased k cat by over 2-fold. These affects are common to human IYD and its homolog from Thermotoga neapolitana and are best explained by an ability of the 2'-hydroxy group of FMN to stabilize association of the substrate in its phenolate form. Loss of this 2'-hydroxy group did not substantially affect the formation of the one electron reduced semiquinone form of FMN but its absence released constraints that otherwise suppresses the ability of IYD to promote hydride transfer as measured by a competing nitroreductase activity. Generation of IYD containing 2'-deoxyFMN also removed steric constraints that had previously limited the use of certain mechanistic probes. For example, l- O -methyl iodotyrosine could be accommodated in the active site lacking the 2'-hydroxy of FMN and shown to be inert to dehalogenation as predicted from a mechanism requiring ketonization of the phenolic oxygen. In the future, ancillary sites within a cofactor should now be considered when engineering new functions within existing protein architectures as demonstrated by the ability of IYD to promote nitroreduction after loss of the 2'-hydroxy group of FMN., Competing Interests: The authors do not have conflicts of interest in this work., (This journal is © The Royal Society of Chemistry.)

Published

2023

6. Dynamic accumulation of cyclobutane pyrimidine dimers and its response to changes in DNA conformation.

Author

Moirangthem R, Gamage MN, and Rokita SE

Subjects

DNA genetics, DNA Repair, Ultraviolet Rays, Nucleic Acid Conformation, Pyrimidine Dimers radiation effects, DNA Damage

Abstract

Photochemical dimerization of adjacent pyrimidines is fundamental to the creation of mutagenic hotspots caused by ultraviolet light. Distribution of the resulting lesions (cyclobutane pyrimidine dimers, CPDs) is already known to be highly variable in cells, and in vitro models have implicated DNA conformation as a major basis for this observation. Past efforts have primarily focused on mechanisms that influence CPD formation and have rarely considered contributions of CPD reversion. However, reversion is competitive under the standard conditions of 254 nm irradiation as illustrated in this report based on the dynamic response of CPDs to changes in DNA conformation. A periodic profile of CPDs was recreated in DNA held in a bent conformation by λ repressor. After linearization of this DNA, the CPD profile relaxed to its characteristic uniform distribution over a similar time of irradiation to that required to generate the initial profile. Similarly, when a T tract was released from a bent conformation, its CPD profile converted under further irradiation to that consistent with a linear T tract. This interconversion of CPDs indicates that both its formation and reversion exert control on CPD populations long before photo-steady-state conditions are achieved and suggests that the dominant sites of CPDs will evolve as DNA conformation changes in response to natural cellular processes., (© The Author(s) 2023. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2023

7. Substrate Electronics Dominate the Rate of Reductive Dehalogenation Promoted by the Flavin-Dependent Iodotyrosine Deiodinase.

Author

Kozyryev A, Lemen D, Dunn J, and Rokita SE

Subjects

Humans, Electron Transport, Catalysis, Flavins metabolism, Kinetics, Substrate Specificity, Oxidation-Reduction, Iodide Peroxidase metabolism, Organic Chemicals

Abstract

Iodotyrosine deiodinase (IYD) is unusual in its reliance on flavin to promote reductive dehalogenation of halotyrosines under aerobic conditions. Applications of this activity can be envisioned for bioremediation, but expansion of its specificity requires an understanding of the mechanistic steps that limit the rate of turnover. Key processes capable of controlling steady-state turnover have now been evaluated and described in this study. While proton transfer is necessary for converting the electron-rich substrate into an electrophilic intermediate suitable for reduction, kinetic solvent deuterium isotope effects suggest that this process does not contribute to the overall efficiency of catalysis under neutral conditions. Similarly, reconstituting IYD with flavin analogues demonstrates that a change in reduction potential by as much as 132 mV affects k cat by less than 3-fold. Furthermore, k cat / K m does not correlate with reduction potential and indicates that electron transfer is also not rate determining. Catalytic efficiency is most sensitive to the electronic nature of its substrates. Electron-donating substituents on the ortho position of iodotyrosine stimulate catalysis and conversely electron-withdrawing substituents suppress catalysis. Effects on k cat and k cat / K m range from 22- to 100-fold and fit a linear free-energy correlation with a ρ ranging from -2.1 to -2.8 for human and bacterial IYD. These values are consistent with a rate-determining process of stabilizing the electrophilic and nonaromatic intermediate poised for reduction. Future engineering can now focus on efforts to stabilize this electrophilic intermediate over a broad series of phenolic substrates that are targeted for removal from our environment.

Published

2023

8. Sequence Conservation Does Not Always Signify a Functional Imperative as Observed in the Nitroreductase Superfamily.

Author

Musila JM and Rokita SE

Subjects

Electron Transport, Flavins metabolism, Flavoproteins metabolism, Oxidation-Reduction, Flavin Mononucleotide chemistry, Nitroreductases metabolism

Abstract

Consensus sequences have the potential to help classify the structure and function of proteins and highlight key regions that may contribute to their biological properties. Often, the level of significance will track with the extent of sequence conservation, but this should not be considered universal. Arg and Lys dominate a position adjacent to the N1 and C2 carbonyl of flavin mononucleotide (FMN) bound in the proteins of the nitroreductase superfamily. Although this placement satisfies expectations for stabilizing the reduced form of FMN, the substitution of these residues in three subfamilies promoting distinct reactions demonstrates their importance to catalysis as only modest. Replacing Arg34 with Lys, Gln, or Glu enhances FMN binding to a flavin destructase (BluB) by twofold and diminishes FMN turnover by no more than 25%. Similarly, replacing Lys14 with Arg, Gln, or Glu in a nitroreductase (NfsB) does not perturb the binding of the substrate nitrofurazone. The catalytic efficiency does decrease by 21-fold for the K14Q variant, but no change in the midpoint potential of FMN was observed with any of the variants. Equivalent substitution at Arg38 in iodotyrosine deiodinase (IYD) affects catalysis even more modestly (<10-fold). While the Arg/Lys to Glu substitution inactivates NfsB and IYD, this change also stabilizes one-electron transfer in IYD contrary to predictions based on other classes of flavoproteins. Accordingly, functional correlations developed in certain structural superfamilies may not necessarily translate well to other superfamilies.

Published

2022

9. The minimal structure for iodotyrosine deiodinase function is defined by an outlier protein from the thermophilic bacterium Thermotoga neapolitana.

Author

Sun Z, Xu B, Spisak S, Kavran JM, and Rokita SE

Subjects

Humans, Protein Domains, Structure-Activity Relationship, Substrate Specificity, Bacterial Proteins chemistry, Iodide Peroxidase chemistry, Models, Molecular, Protein Folding, Thermotoga neapolitana enzymology

Abstract

The nitroreductase superfamily of enzymes encompasses many flavin mononucleotide (FMN)-dependent catalysts promoting a wide range of reactions. All share a common core consisting of an FMN-binding domain, and individual subgroups additionally contain one to three sequence extensions radiating from defined positions within this core to support their unique catalytic properties. To identify the minimum structure required for activity in the iodotyrosine deiodinase subgroup of this superfamily, attention was directed to a representative from the thermophilic organism Thermotoga neapolitana (TnIYD). This representative was selected based on its status as an outlier of the subgroup arising from its deficiency in certain standard motifs evident in all homologues from mesophiles. We found that TnIYD lacked a typical N-terminal sequence and one of its two characteristic sequence extensions, neither of which was found to be necessary for activity. We also show that TnIYD efficiently promotes dehalogenation of iodo-, bromo-, and chlorotyrosine, analogous to related deiodinases (IYDs) from humans and other mesophiles. In addition, 2-iodophenol is a weak substrate for TnIYD as it was for all other IYDs characterized to date. Consistent with enzymes from thermophilic organisms, we observed that TnIYD adopts a compact fold and low surface area compared with IYDs from mesophilic organisms. The insights gained from our investigations on TnIYD demonstrate the advantages of focusing on sequences that diverge from conventional standards to uncover the minimum essentials for activity. We conclude that TnIYD now represents a superior starting structure for future efforts to engineer a stable dehalogenase targeting halophenols of environmental concern., Competing Interests: Conflict of interest The authors declare that they have no conflicts of interest with the contents of this article., (Copyright © 2021 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2021

10. Unraveling Reversible DNA Cross-Links with a Biological Machine.

Author

Byrne SR and Rokita SE

Subjects

Alkylation, Cross-Linking Reagents chemistry, DNA chemistry, Indolequinones chemistry, Molecular Structure, Cross-Linking Reagents metabolism, DNA metabolism, Indolequinones metabolism

Abstract

The reversible generation and capture of certain electrophilic quinone methide intermediates support dynamic reactions with DNA that allow for migration and transfer of alkylation and cross-linking. This reversibility also expands the possible consequences that can be envisioned when confronted by DNA repair processes and biological machines. To begin testing the response to such an encounter, quinone methide-based modification of DNA has now been challenged with a helicase (T7 bacteriophage gene protein four, T7gp4) that promotes 5' to 3' translocation and unwinding. This model protein was selected based on its widespread application, well characterized mechanism and detailed structural information. Little over one-half of the cross-linking generated by a bisfunctional quinone methide remained stable to T7gp4 and did not suppress its activity. The helicase likely avoids the topological block generated by this fraction of cross-linking by its ability to shift from single- to double-stranded translocation. The remaining fraction of cross-linking was destroyed during T7gp4 catalysis. Thus, this helicase is chemically competent to promote release of the quinone methide from DNA. The ability of T7gp4 to act as a Brownian ratchet for unwinding DNA may block recapture of the QM intermediate by DNA during its transient release from a donor strand. Most surprisingly, T7gp4 releases the quinone methide from both the translocating strand that passes through its central channel and the excluded strand that was typically unaffected by other lesions. The ability of T7gp4 to reverse the cross-link formed by the quinone methide does not extend to that formed irreversibly by the nitrogen mustard mechlorethamine.

Published

2020

11. Directing Quinone Methide-Dependent Alkylation and Cross-Linking of Nucleic Acids with Quaternary Amines.

Author

Hutchinson MA, Deeyaa BD, Byrne SR, Williams SJ, and Rokita SE

Subjects

Acridines chemistry, Alkylation, DNA, Single-Stranded chemistry, Kinetics, Amines chemistry, DNA chemistry, Indolequinones chemistry

Abstract

Polyamine and polyammonium ion conjugates are often used to direct reagents to nucleic acids based on their strong electrostatic attraction to the phosphoribose backbone. Such nonspecific interactions do not typically alter the specificity of the attached reagent, but polyammonium ions dramatically redirected the specificity of a series of quinone methide precursors. Replacement of a relatively nonspecific intercalator based on acridine with a series of polyammonium ions resulted in a surprising change of DNA products. Piperidine stable adducts were generated in duplex DNA that lacked the ability to support a dynamic cross-linking observed previously with acridine conjugates. Minor reaction at guanine N7, the site of reversible reaction, was retained by a monofunctional quinone methide-polyammonium ion conjugate, but a bisfunctional analogue designed for tandem quinone methide formation modified guanine N7 in only single-stranded DNA. The resulting intrastrand cross-links were sufficiently dynamic to rearrange to interstrand cross-links. However, no further transfer of adducts was observed in duplex DNA. An alternative design that spatially and temporally decoupled the two quinone methide equivalents neither restored the dynamic reaction nor cross-linked DNA efficiently. While di- and triammonium ion conjugates successfully enhanced the yields of cross-linking by a bisquinone methide relative to a monoammonium equivalent, alternative ligands will be necessary to facilitate the migration of cross-linking and its potential application to disrupt DNA repair.

Published

2020

12. Migratory ability of quinone methide-generating acridine conjugates in DNA.

Author

Deeyaa BD and Rokita SE

Subjects

Alkylating Agents chemistry, Alkylation, DNA chemistry, DNA Adducts chemistry, Diffusion, Intercalating Agents chemistry, Acridines chemistry, DNA metabolism, Indolequinones chemistry

Abstract

The dynamic nature of nucleic acid alkylation by simple ortho quinone methides (QM) and their conjugates has provided numerous opportunities ranging from sequence selective targeting to bipedal walking in duplex DNA. To enhance the diffusion rate of adduct migration, one of two sites for QM generation was deleted from a bisQM conjugate of acridine to remove the covalent anchor to DNA that persists during QM regeneration. This conversion of a bisfunctional cross-linking agent to a monofunctional alkylating agent allowed adduct diffusion to traverse an extrahelical -TT- bulge that previously acted as a barrier for its bisfunctional analog. An electron rich derivative of the monofunctional acridine conjugate was additionally prepared to accelerate the rates of DNA alkylation and QM regeneration. The resulting stabilization of this QM effectively enhanced the rate of its release from adducts attached at guanine N7 in competition with an alternative and detrimental deglycosylation pathway. Intercalation by the acridine component was not sufficient to hold the transient QM intermediates within duplex DNA and consequently these electrophiles diffused into solution and were subject to quenching by solvent and a model nucleophile, β-mercaptoethanol.

Published

2020

13. Effect of Nucleosome Assembly on Alkylation by a Dynamic Electrophile.

Author

Byrne SR, Yang K, and Rokita SE

Subjects

Acridines chemistry, Alkylation, Animals, Cross-Linking Reagents chemistry, DNA Adducts chemistry, Escherichia coli genetics, Histones chemistry, Humans, Xenopus laevis, Alkenes chemistry, Cyclohexanones chemistry, DNA chemistry, Nucleosomes chemistry

Abstract

Quinone methides are reactive electrophiles that are generated during metabolism of various drugs, natural products, and food additives. Their chemical properties and cellular effects have been described previously, and now their response to packaging DNA in a nucleosome core is described. A model bisquinone methide precursor (bisQMP) was selected based on its ability to form reversible adducts with guanine N7 that allow for their redistribution and transfer after quinone methide regeneration. Assembly of Widom's 601 DNA with the histone octamer of H2A, H2B, H3, and H4 from Xenopus laevis significantly suppressed alkylation of the DNA. This result is a function of DNA packaging since addition of the octamer without nucleosome reconstitution only mildly protected DNA from alkylation. The lack of competition between nucleophiles of DNA and the histones was consistent with the limited number of adducts formed by the histones as detected by tryptic digestion and ultraperformance liquid chromatography-mass spectrometry. Only three peptide adducts were observed after reaction with a monofunctional analogue of bisQMP, and only two peptide adducts were observed after reaction with bisQMP. Histone reaction was also suppressed when reconstituted into the nucleosome core particle. However, bisQMP was capable of cross-linking the DNA and histones in moderate yields (∼20%) that exceeded expectations derived from reaction of cisplatin, nitrogen mustards, and diepoxybutane. The core histones also demonstrated a protective function against dynamic alkylation by trapping the reactive quinone methide after its spontaneous regeneration from DNA adducts.

Published

2019

14. Redox control of iodotyrosine deiodinase.

Author

Hu J, Su Q, Schlessman JL, and Rokita SE

Subjects

Amino Acid Substitution, Catalytic Domain, Humans, Iodide Peroxidase genetics, Kinetics, Mutation, Missense, Oxidation-Reduction, Dinitrocresols chemistry, Iodide Peroxidase chemistry

Abstract

The redox chemistry of flavoproteins is often gated by substrate and iodotyrosine deiodinase (IYD) has the additional ability to switch between reaction modes based on the substrate. Association of fluorotyrosine (F-Tyr), an inert substrate analog, stabilizes single electron transfer reactions of IYD that are not observed in the absence of this ligand. The co-crystal of F-Tyr and a T239A variant of human IYD have now been characterized to provide a structural basis for control of its flavin reactivity. Coordination of F-Tyr in the active site of this IYD closely mimics that of iodotyrosine and only minor perturbations are observed after replacement of an active site Thr with Ala. However, loss of the side chain hydroxyl group removes a key hydrogen bond from flavin and suppresses the formation of its semiquinone intermediate. Even substitution of Thr with Ser decreases the midpoint potential of human IYD between its oxidized and semiquinone forms of flavin by almost 80 mV. This decrease does not adversely affect the kinetics of reductive dehalogenation although an analogous Ala variant exhibits a 6.7-fold decrease in its k cat /K m . Active site ligands lacking the zwitterion of halotyrosine are not able to induce closure of the active site lid that is necessary for promoting single electron transfer and dehalogenation. Under these conditions, a basal two-electron process dominates catalysis as indicated by preferential reduction of nitrophenol rather than deiodination of iodophenol., (© 2018 The Protein Society.)

Published

2019

15. The importance of a halotyrosine dehalogenase for Drosophila fertility.

Author

Phatarphekar A, Su Q, Eun SH, Chen X, and Rokita SE

Subjects

Animals, Female, Fertility, Gene Expression Regulation, Enzymologic, Male, Testis metabolism, Drosophila enzymology, Drosophila physiology, Iodide Peroxidase metabolism

Abstract

The ability of iodotyrosine deiodinase to salvage iodide from iodotyrosine has long been recognized as critical for iodide homeostasis and proper thyroid function in vertebrates. The significance of its additional ability to dehalogenate bromo- and chlorotyrosine is less apparent, and none of these functions could have been anticipated in invertebrates until recently. Drosophila, as most arthropods, contains a deiodinase homolog encoded by CG6279 , now named condet ( cdt ), with a similar catalytic specificity. However, its physiological role cannot be equivalent because Drosophila lacks a thyroid and its associated hormones, and no requirement for iodide or halotyrosines has been reported for this species. We have now applied CRISPR/Cas9 technology to generate Drosophila strains in which the cdt gene has been either deleted or mutated to identify its biological function. As previously shown in larvae, expression of cdt is primarily limited to the fat body, and we now report that loss of cdt function does not enhance sensitivity of the larvae to the toxic effects of iodotyrosine. In adult flies by contrast, expression is known to occur in testes and is detected at very high levels in this tissue. The importance of cdt is most evident in the decrease in fertility observed when either males or females carry a deletion or mutation of cdt Therefore, dehalogenation of a halotyrosine appears essential for efficient reproduction in Drosophila and likely contributes to a new pathway for controlling viability in arthropods., (© 2018 Phatarphekar et al.)

Published

2018

16. The distribution and mechanism of iodotyrosine deiodinase defied expectations.

Author

Sun Z, Su Q, and Rokita SE

Subjects

Animals, Flavin-Adenine Dinucleotide chemistry, Flavin-Adenine Dinucleotide genetics, Flavin-Adenine Dinucleotide metabolism, Humans, Iodide Peroxidase genetics, Iodide Peroxidase metabolism, Iodides chemistry, Iodides metabolism, Nitroreductases genetics, Nitroreductases metabolism, Triiodothyronine chemistry, Triiodothyronine metabolism, Flavin-Adenine Dinucleotide analogs & derivatives, Iodide Peroxidase chemistry, Nitroreductases chemistry

Abstract

Iodotyrosine deiodinase (IYD) is unusual for its reliance on flavin to promote reductive dehalogenation under aerobic conditions. As implied by the name, this enzyme was first discovered to catalyze iodide elimination from iodotyrosine for recycling iodide during synthesis of tetra- and triiodothyronine collectively known as thyroid hormone. However, IYD likely supports many more functions and has been shown to debrominate and dechlorinate bromo- and chlorotyrosines. A specificity for halotyrosines versus halophenols is well preserved from humans to bacteria. In all examples to date, the substrate zwitterion establishes polar contacts with both the protein and the isoalloxazine ring of flavin. Mechanistic data suggest dehalogenation is catalyzed by sequential one electron transfer steps from reduced flavin to substrate despite the initial expectations for a single two electron transfer mechanism. A purported flavin semiquinone intermediate is stabilized by hydrogen bonding between its N5 position and the side chain of a Thr. Mutation of this residue to Ala suppresses dehalogenation and enhances a nitroreductase activity that is reminiscent of other enzymes within the same structural superfamily., (Copyright © 2017 Elsevier Inc. All rights reserved.)

Published

2017

17. Conversion of a Dehalogenase into a Nitroreductase by Swapping its Flavin Cofactor with a 5-Deazaflavin Analogue.

Author

Su Q, Boucher PA, and Rokita SE

Subjects

Flavins chemistry, Molecular Structure, Flavins metabolism, Hydrolases metabolism, Nitroreductases metabolism

Abstract

Natural and engineered nitroreductases have rarely supported full reduction of nitroaromatics to their amine products, and more typically, transformations are limited to formation of the hydroxylamine intermediates. Efficient use of these enzymes also requires a regenerating system for NAD(P)H to avoid the costs associated with this natural reductant. Iodotyrosine deiodinase is a member of the same structural superfamily as many nitroreductases but does not directly consume reducing equivalents from NAD(P)H, nor demonstrate nitroreductase activity. However, exchange of its flavin cofactor with a 5-deazaflavin analogue dramatically suppresses its native deiodinase activity and leads to significant nitroreductase activity that supports full reduction to an amine product in the presence of the convenient and inexpensive NaBH 4 ., (© 2017 Wiley-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2017

18. Active Site Binding Is Not Sufficient for Reductive Deiodination by Iodotyrosine Deiodinase.

Author

Ingavat N, Kavran JM, Sun Z, and Rokita SE

Subjects

Bacteroidetes enzymology, Flavin Mononucleotide metabolism, Humans, Models, Molecular, Oxidation-Reduction, Catalytic Domain, Halogenation, Iodide Peroxidase chemistry, Iodide Peroxidase metabolism

Abstract

The minimal requirements for substrate recognition and turnover by iodotyrosine deiodinase were examined to learn the basis for its catalytic specificity. This enzyme is crucial for iodide homeostasis and the generation of thyroid hormone in chordates. 2-Iodophenol binds only very weakly to the human enzyme and is dehalogenated with a k cat /K m that is more than 4 orders of magnitude lower than that for iodotyrosine. This discrimination likely protects against a futile cycle of iodinating and deiodinating precursors of thyroid hormone biosynthesis. Surprisingly, a very similar catalytic selectivity was expressed by a bacterial homologue from Haliscomenobacter hydrossis. In this example, discrimination was not based on affinity since 4-cyano-2-iodophenol bound to the bacterial deiodinase with a K d lower than that of iodotyrosine and yet was not detectably deiodinated. Other phenols including 2-iodophenol were deiodinated but only very inefficiently. Crystal structures of the bacterial enzyme with and without bound iodotyrosine are nearly superimposable and quite similar to the corresponding structures of the human enzyme. Likewise, the bacterial enzyme is activated for single electron transfer after binding to the substrate analogue fluorotyrosine as previously observed with the human enzyme. A cocrystal structure of bacterial deiodinase and 2-iodophenol indicates that this ligand stacks on the active site flavin mononucleotide (FMN) in a orientation analogous to that of bound iodotyrosine. However, 2-iodophenol association is not sufficient to activate the FMN chemistry required for catalysis, and thus the bacterial enzyme appears to share a similar specificity for halotyrosines even though their physiological roles are likely very different from those in humans.

Published

2017

19. Functional analysis of iodotyrosine deiodinase from drosophila melanogaster.

Author

Phatarphekar A and Rokita SE

Subjects

Amino Acid Substitution, Animals, Catalytic Domain, Drosophila Proteins genetics, Drosophila Proteins metabolism, Drosophila melanogaster, Iodide Peroxidase genetics, Iodide Peroxidase metabolism, Mutation, Missense, Substrate Specificity, Drosophila Proteins chemistry, Iodide Peroxidase chemistry, Tyrosine analogs & derivatives, Tyrosine chemistry

Abstract

The flavoprotein iodotyrosine deiodinase (IYD) was first discovered in mammals through its ability to salvage iodide from mono- and diiodotyrosine, the by-products of thyroid hormone synthesis. Genomic information indicates that invertebrates contain homologous enzymes although their iodide requirements are unknown. The catalytic domain of IYD from Drosophila melanogaster has now been cloned, expressed and characterized to determine the scope of its potential catalytic function as a model for organisms that are not associated with thyroid hormone production. Little discrimination between iodo-, bromo-, and chlorotyrosine was detected. Their affinity for IYD ranges from 0.46 to 0.62 μM (K d ) and their efficiency of dehalogenation ranges from 2.4 - 9 x 10 3 M -1 s -1 (k cat /K m ). These values fall within the variations described for IYDs from other organisms for which a physiological function has been confirmed. The relative contribution of three active site residues that coordinate to the amino acid substrates was subsequently determined by mutagenesis of IYD from Drosophila to refine future annotations of genomic and meta-genomic data for dehalogenation of halotyrosines. Substitution of the active site glutamate to glutamine was most detrimental to catalysis. Alternative substitution of an active site lysine to glutamine affected substrate affinity to the greatest extent but only moderately affected catalytic turnover. Substitution of phenylalanine for an active site tyrosine was least perturbing for binding and catalysis., (© 2016 The Protein Society.)

Published

2016

20. An Activator of an Adenylation Domain Revealed by Activity but Not Sequence Homology.

Author

Saha S and Rokita SE

Subjects

Amino Acids chemistry, Biocatalysis, Mycobacterium tuberculosis, Amino Acids metabolism, Bacterial Proteins metabolism, Peptide Synthases metabolism

Abstract

Nonribosomal peptide synthetases (NRPSs), which are responsible for synthesizing many medicinally important natural products, frequently use adenylation domain activators (ADAs) to promote substrate loading. Although ADAs are usually MbtH-like proteins (MLPs), a new type of ADA appears to promote an NRPS-dependent incorporation of a dihydropyrrole unit into sibiromycin. The adenylation and thiolation didomain of the NRPS SibD catalyzes the adenylation of a limited number of amino acids including l-Tyr, the precursor in dihydropyrrole biosynthesis, as determined by a standard radioactivity exchange assay. LC-MS/MS analysis confirmed loading of l-Tyr onto the thiolation domain. SibB, a small protein with no prior functional assignment or sequence homology to MLPs, was found to promote the exchange activity. MLPs from bacteria expressing homologous biosynthetic pathways were unable to replace this function of SibB. The discovery of this new type of ADA demonstrates the importance of searching beyond the conventional MLP standard for proteins affecting NRPS activity., (© 2016 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2016

21. Targeting duplex DNA with the reversible reactivity of quinone methides.

Author

Huang C, Liu Y, and Rokita SE

Abstract

DNA alkylation and crosslinking remains a common and effective strategy for anticancer chemotherapy despite its infamous lack of specificity. Coupling a reactive group to a sequence-directing component has the potential to enhance target selectivity but may suffer from premature degradation or the need for an external signal for activation. Alternatively, quinone methide conjugates may be employed if they form covalent but reversible adducts with their sequence directing component. The resulting self-adducts transfer their quinone methide to a chosen target without an external signal and avoid off-target reactions by alternative intramolecular self-trapping. Efficient transfer is shown to depend on the nature of the quinone methide and the sequence-directing ligand in applications involving alkylation of duplex DNA through a triplex recognition motif. Success required an electron-rich derivative that enhanced the stability of the transient quinone methide intermediate and a polypyrimidine strand of DNA to associate with its cognate polypurine/polypyrimidine target. Related quinone methide conjugates with peptide nucleic acids were capable of quinone methide transfer from their initial precursor but not from their corresponding self-adduct. The active peptide nucleic acid derivatives were highly selective for their complementary target., Competing Interests: COMPETING INTERESTS The authors declare no conflict of interest.

Published

2016

22. Single Amino Acid Switch between a Flavin-Dependent Dehalogenase and Nitroreductase.

Author

Mukherjee A and Rokita SE

Subjects

Amino Acids genetics, Flavins metabolism, Gene Expression Regulation, Enzymologic, Molecular Structure, Mutation, Nitroreductases chemistry, Nitroreductases metabolism, Oxidoreductases chemistry, Oxidoreductases metabolism, Amino Acids chemistry, Flavins chemistry, Nitroreductases genetics, Oxidoreductases genetics

Abstract

A single mutation within a flavoprotein is capable of switching the catalytic activity of a dehalogenase into a nitroreductase. This change in function correlates with a destabilization of the one-electron-reduced flavin semiquinone that is differentially expressed in the nitro-FMN reductase superfamily during redox cycling. The diversity of function within such a superfamily therefore has the potential to arise from rapid evolution, and its members should provide a convenient basis for developing new catalysts with an altered specificity of choice.

Published

2015

23. Rapid kinetics of dehalogenation promoted by iodotyrosine deiodinase from human thyroid.

Author

Bobyk KD, Ballou DP, and Rokita SE

Subjects

Biocatalysis, Catalytic Domain, Dinitrocresols chemistry, Humans, Kinetics, Monoiodotyrosine chemistry, Oxidation-Reduction, Protein Binding, Iodide Peroxidase chemistry, Thyroid Gland enzymology

Abstract

Reductive dehalogenation such as that catalyzed by iodotyrosine deiodinase (IYD) is highly unusual in aerobic organisms but necessary for iodide salvage from iodotyrosine generated during thyroxine biosynthesis. Equally unusual is the dependence of this process on flavin. Rapid kinetics have now been used to define the basic processes involved in IYD catalysis. Time-dependent quenching of flavin fluorescence was used to monitor halotyrosine association to IYD. The substrates chloro-, bromo-, and iodotyrosine bound with similar rate constants (kon) ranging from 1.3 × 10(6) to 1.9 × 10(6) M(-1) s(-1). Only the inert substrate analogue fluorotyrosine exhibited a significantly (5-fold) slower kon (0.3 × 10(6) M(-1) s(-1)). All data fit a standard two-state model and indicated that no intermediate complex accumulated during closure of the active site lid induced by substrate. Subsequent halide elimination does not appear to limit reactions of bromo- and iodotyrosine since both fully oxidized the reduced enzyme with nearly equivalent second-order rate constants (7.3 × 10(3) and 8.6 × 10(3) M(-1) s(-1), respectively) despite the differing strength of their carbon-halogen bonds. In contrast to these substrates, chlorotyrosine reacted with the reduced enzyme approximately 20-fold more slowly and revealed a spectral intermediate that formed at approximately the same rate as the bromo- and iodotyrosine reactions.

Published

2015

24. Identification of the dioxygenase-generated intermediate formed during biosynthesis of the dihydropyrrole moiety common to anthramycin and sibiromycin.

Author

Saha S, Li W, Gerratana B, and Rokita SE

Subjects

Aminoglycosides metabolism, Anthramycin metabolism, Dioxygenases metabolism, Magnetic Resonance Spectroscopy, Molecular Structure, Pyrroles chemistry, Aminoglycosides chemistry, Anthramycin chemistry, Dioxygenases chemistry, Pyrroles metabolism

Abstract

A description of pyrrolo[1,4]benzodiazepine (PBD) biosynthesis is a prerequisite for engineering production of analogs with enhanced antitumor activity. Predicted dioxygenases Orf12 and SibV associated with dihydropyrrole biosynthesis in PBDs anthramycin and sibiromycin, respectively, were expressed and purified for activity studies. UV-visible spectroscopy revealed that these enzymes catalyze the regiospecific 2,3-extradiol dioxygenation of l-3,4-dihydroxyphenylalanine (l-DOPA) to form l-2,3-secodopa (λmax=368 nm). (1)H NMR spectroscopy indicates that l-2,3-secodopa cyclizes into the α-keto acid tautomer of l-4-(2-oxo-3-butenoic-acid)-4,5-dihydropyrrole-2-carboxylic acid (λmax=414 nm). Thus, the dioxygenases are key for establishing the scaffold of the dihydropyrrole moiety. Kinetic studies suggest the dioxygenase product is relatively labile and is likely consumed rapidly by subsequent biosynthetic steps. The enzymatic product and dimeric state of these dioxygenases are conserved in dioxygenases involved in dihydropyrrole and pyrrolidine biosynthesis within both PBD and non-PBD pathways., (Copyright © 2014 Elsevier Ltd. All rights reserved.)

Published

2015

25. A switch between one- and two-electron chemistry of the human flavoprotein iodotyrosine deiodinase is controlled by substrate.

Author

Hu J, Chuenchor W, and Rokita SE

Subjects

Biocatalysis, Catalytic Domain, Crystallography, X-Ray, Electron Transport, Escherichia coli genetics, Escherichia coli metabolism, Flavin Mononucleotide metabolism, Flavins chemistry, Flavins metabolism, Gene Expression, Humans, Hydrogen-Ion Concentration, Iodide Peroxidase genetics, Iodide Peroxidase metabolism, Iodides chemistry, Iodides metabolism, Models, Molecular, Monoiodotyrosine metabolism, Oxidation-Reduction, Protein Binding, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Substrate Specificity, Tyrosine analogs & derivatives, Tyrosine chemistry, Tyrosine metabolism, Electrons, Flavin Mononucleotide chemistry, Iodide Peroxidase chemistry, Monoiodotyrosine chemistry

Abstract

Reductive dehalogenation is not typical of aerobic organisms but plays a significant role in iodide homeostasis and thyroid activity. The flavoprotein iodotyrosine deiodinase (IYD) is responsible for iodide salvage by reductive deiodination of the iodotyrosine derivatives formed as byproducts of thyroid hormone biosynthesis. Heterologous expression of the human enzyme lacking its N-terminal membrane anchor has allowed for physical and biochemical studies to identify the role of substrate in controlling the active site geometry and flavin chemistry. Crystal structures of human IYD and its complex with 3-iodo-l-tyrosine illustrate the ability of the substrate to provide multiple interactions with the isoalloxazine system of FMN that are usually provided by protein side chains. Ligand binding acts to template the active site geometry and significantly stabilize the one-electron-reduced semiquinone form of FMN. The neutral form of this semiquinone is observed during reductive titration of IYD in the presence of the substrate analog 3-fluoro-l-tyrosine. In the absence of an active site ligand, only the oxidized and two-electron-reduced forms of FMN are detected. The pH dependence of IYD binding and turnover also supports the importance of direct coordination between substrate and FMN for productive catalysis., (© 2015 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2015

26. A walk along DNA using bipedal migration of a dynamic and covalent crosslinker.

Author

Fakhari F and Rokita SE

Subjects

Acridines chemistry, Biological Transport, Indolequinones chemical synthesis, Intercalating Agents chemistry, Interspersed Repetitive Sequences genetics, Cross-Linking Reagents chemistry, DNA chemistry, Indolequinones chemistry, Nucleic Acid Conformation drug effects

Abstract

DNA has previously served as an excellent scaffold for molecular transport based on its non-covalent base pairing to assemble both stationary and mobile elements. Use of DNA can now be extended to transport systems based on reversible covalent chemistry. Autonomous and bipedal-like migration of crosslinking within helical DNA is made possible by tandem exchange of a quinone methide intermediate. In this report, net transport is illustrated to proceed over 10 base pairs. This process is driven towards its equilibrium distribution of crosslinks and consumes neither the walker nor the track irreversibly. Successful migration requires an electron-rich quinone methide to promote its regeneration and a continuous array of nucleophilic sites along its DNA track. Accordingly, net migration can be dramatically influenced by the presence of noncanonical structures within duplex DNA as demonstrated with a backbone nick and extrahelical bulge.

Published

2014

27. Oxidative quenching of quinone methide adducts reveals transient products of reversible alkylation in duplex DNA.

Author

McCrane MP, Hutchinson MA, Ad O, and Rokita SE

Subjects

Alkylation, DNA chemistry, Oxidation-Reduction, DNA Adducts chemistry, Hydrocarbons, Halogenated chemistry, Indolequinones chemistry, Oligonucleotides chemistry

Abstract

ortho-Quinone methides (ortho-QM) and para-quinone methides are generated by xenobiotic metabolism of numerous compounds including environmental toxins and therapeutic agents. These intermediates are highly electrophilic and have the potential to alkylate DNA. Assessing their genotoxicity can be difficult when all or some of their resulting adducts form reversibly. Stable adducts are most easily detected but are not necessarily the most prevalent products formed initially as DNA repair commences. Selective oxidation of ortho-QM-DNA adducts by bis[(trifluoroacetoxy)iodo]benzene (BTI) rapidly quenches their reversibility to prevent QM regeneration and allows for observation of the kinetic products. The resulting derivatives persist through standard enzymatic digestion, chromatography, and mass spectral analysis. The structural standards required for this approach have been synthesized and confirmed by two-dimensional NMR spectroscopy. The adducts of dA N(6), dG N1, dG N(2), and guanine N7 are converted to the expected para-quinol derivatives within 5 min after addition of BTI under aqueous conditions (pH 7). Concurrently, the adduct of dA N1 forms a spiro derivative comparable to that characterized previously after oxidation of the corresponding dC N3 adduct. By application of this oxidative quenching strategy, the dC N3 and dA N1 adducts have been identified as the dominant products formed by both single- and double-stranded DNA under initial conditions. As expected, however, these labile adducts dissipate within 24 h if not quenched with BTI. Still, the products favored by kinetics are responsible for inducing the first response to ortho-QM exposure in cells, and hence, they are also key to establishing the relationship between biological activity and molecular structure.

Published

2014

28. Electron transport in DNA initiated by diaminonaphthalene donors alternatively bound by non-covalent and covalent association.

Author

Campbell NP and Rokita SE

Subjects

2-Naphthylamine chemistry, Electron Transport, 2-Naphthylamine analogs & derivatives, DNA chemistry

Abstract

Covalent conjugation is typically used to fix a potential charge donor to a chosen site for studying either hole or excess electron transport in duplex DNA. A model system based on oligonucleotides containing an abasic site and (Br)dU was previously developed to provide a rapid method of screening new donors without the need of synthetic chemistry. While this strategy is effective for discovering important lead compounds, it is not appropriate for establishing extensive correlations between molecular structure and donor efficiency as demonstrated with a series of closely related electron donors based on diaminonaphthalene. The non-covalent system accurately identified the ability of the donors to reduce a distal (Br)dU in DNA, but their varying efficiencies were not recapitulated when attached covalently to an equivalent sequence of DNA. Reduction within the covalent system was not sensitive to the strong donor potentials as consistent with charge recombination dominating the net migration of charge.

Published

2014

29. Iodotyrosine deiodinase: a unique flavoprotein present in organisms of diverse phyla.

Author

Phatarphekar A, Buss JM, and Rokita SE

Subjects

Animals, Catalytic Domain, Diiodotyrosine metabolism, Evolution, Molecular, Gene Expression Regulation, Enzymologic, Halogenation, Iodide Peroxidase chemistry, Iodides metabolism, Mice, Protein Conformation, Iodide Peroxidase genetics, Iodide Peroxidase metabolism, Thyroid Hormones biosynthesis, Tyrosine metabolism

Abstract

Iodide is required for thyroid hormone synthesis in mammals and other vertebrates. The role of both iodide and iodinated tyrosine derivatives is currently unknown in lower organisms, yet the presence of a key enzyme in iodide conservation, iodotyrosine deiodinase (IYD), is suggested by genomic data from a wide range of multicellular organisms as well as some bacteria. A representative set of these genes has now been expressed, and the resulting enzymes all catalyze reductive deiodination of diiodotyrosine with kcat/Km values within a single order of magnitude. This implies a physiological presence of iodotyrosines (or related halotyrosines) and a physiological role for their turnover. At least for Metazoa, IYD should provide a new marker for tracing the evolutionary development of iodinated amino acids as regulatory signals through the tree of life.

Published

2014

30. Enhancing excess electron transport in DNA.

Author

Fakhari F, Chen YY, and Rokita SE

Subjects

Anthracenes chemistry, Base Sequence, Electron Transport, Purines chemistry, Pyrimidines chemistry, DNA chemistry

Abstract

The efficiency of excess electron transport in duplex DNA can be enhanced by limiting the pathways available for migration and using a donor of moderate strength that suppresses radical recombination through selective electron transfer to distal pyrimidines rather than proximal purines.

Published

2013

31. Accumulation of the cyclobutane thymine dimer in defined sequences of free and nucleosomal DNA.

Author

Finch AS, Davis WB, and Rokita SE

Subjects

Animals, Base Sequence radiation effects, DNA genetics, Dimerization, Genes, rRNA, Nucleosomes genetics, Nucleosomes radiation effects, Pyrimidine Dimers genetics, Ultraviolet Rays, Xenopus, DNA chemistry, Nucleosomes chemistry, Pyrimidine Dimers analysis

Abstract

Photochemical cyclobutane dimerization of adjacent thymines generates the major lesion in DNA caused by exposure to sunlight. Not all nucleotide sequences and structures are equally susceptible to this reaction or its potential to create mutations. Photostationary levels of the cyclobutane thymine dimer have now been quantified in homogenous samples of DNA reconstituted into nucleosome core particles to examine the basis for previous observations that such structures could induce a periodicity in dimer yield when libraries of heterogeneous sequences were used. Initial rate studies did not reveal a similar periodicity when a homogenous core particle was analyzed, but this approach examined only formation of this photochemically reversible cyclobutane dimer. Photostationary levels result from competition between dimerization and reversion and, as described in this study, still express none of the periodicity within two alternative core particles that was evident in heterogeneous samples. Such periodicity likely arises from only a limited set of sequences and structural environments that are not present in the homogeneous and well-characterized assemblies available to date.

Published

2013

32. Expression of a soluble form of iodotyrosine deiodinase for active site characterization by engineering the native membrane protein from Mus musculus.

Author

Buss JM, McTamney PM, and Rokita SE

Subjects

Amino Acid Sequence, Animals, Base Sequence, Catalytic Domain, Escherichia coli enzymology, Iodide Peroxidase chemistry, Iodide Peroxidase genetics, Mice, Molecular Sequence Data, Pichia enzymology, Protein Engineering, Protein Structure, Tertiary, Solubility, Iodide Peroxidase biosynthesis, Recombinant Proteins biosynthesis

Abstract

Reductive deiodination is critical for thyroid function and represents an unusual exception to the more common oxidative and hydrolytic mechanisms of dehalogenation in mammals. Studies on the reductive processes have been limited by a lack of convenient methods for heterologous expression of the appropriate proteins in large scale. The enzyme responsible for iodide salvage in the thyroid, iodotyrosine deodinase, is now readily generated after engineering its gene from Mus musculus. High expression of a truncated derivative lacking the membrane domain at its N-terminal was observed in Sf9 cells, whereas expression in Pichia pastoris remained low despite codon optimization. Ultimately, the desired expression in Escherichia coli was achieved after replacing the two conserved Cys residues of the deiodinase with Ala and fusing the resulting protein to thioredoxin. This final construct provided abundant enzyme for crystallography and mutagenesis. Utility of the E. coli system was demonstrated by examining a set of active site residues critical for binding to the zwitterionic portion of substrate.

Published

2012

33. Inducible alkylation of DNA by a quinone methide-peptide nucleic acid conjugate.

Author

Liu Y and Rokita SE

Subjects

Alkylation, DNA metabolism, Drug Delivery Systems, Drug Design, Hydrolysis, Indolequinones metabolism, Nucleic Acid Heteroduplexes chemistry, Nucleic Acid Heteroduplexes metabolism, Oxidation-Reduction, Peptide Nucleic Acids metabolism, Thermodynamics, DNA chemistry, Indolequinones chemistry, Peptide Nucleic Acids chemical synthesis

Abstract

The reversibility of alkylation by a quinone methide intermediate (QM) avoids the irreversible consumption that plagues most reagents based on covalent chemistry and allows for site specific reaction that is controlled by the thermodynamics rather than kinetics of target association. This characteristic was originally examined with an oligonucleotide QM conjugate, but broad application depends on alternative derivatives that are compatible with a cellular environment. Now, a peptide nucleic acid (PNA) derivative has been constructed and shown to exhibit an equivalent ability to delivery the reactive QM in a controlled manner. This new conjugate demonstrates high selectivity for a complementary sequence of DNA even when challenged with an alternative sequence containing a single T/T mismatch. Alternatively, alkylation of noncomplementary sequences is only possible when a template strand is present to colocalize the conjugate and its target. For efficient alkylation in this example, a single-stranded region of the target is required adjacent to the QM conjugate. Most importantly, the intrastrand self-adducts formed between the PNA and its attached QM remained active and reversible over more than 8 days in aqueous solution prior to reaction with a chosen target added subsequently.

Published

2012

34. Classical Cys2His2 zinc finger peptides are rapidly oxidized by either H2O2 or O2 irrespective of metal coordination.

Author

Lee SJ, Michalek JL, Besold AN, Rokita SE, and Michel SL

Subjects

DNA chemistry, Oxidation-Reduction, Cysteine chemistry, Histidine chemistry, Hydrogen Peroxide chemistry, Oxygen chemistry, Peptides chemistry, Zinc Fingers

Abstract

ZIF268, a member of the classical zinc finger protein family, contains three Cys(2)His(2) zinc binding domains that together recognize the DNA sequence 5'-AGCGTGGGCGT-3'. These domains can be fused to an endonuclease to make a chimeric protein to target and cleave specific DNA sequences. A peptide corresponding to these domains, named ZIF268-3D, has been prepared to determine if the zinc finger domain itself can promote DNA cleavage when a redox active metal ion, Fe(II), is coordinated. The UV-vis absorption spectrum of Fe(II)-ZIF268-3D is indicative of Fe(II) coordination. Using fluorescence anisotropy, we demonstrate that Fe(II)-ZIF268-3D binds selectively to its target DNA in the same manner as Zn(II)-ZIF268-3D. In the presence of added oxidant, H(2)O(2) or O(2), DNA cleavage is not observed by Fe(II)-ZIF268-3D. Instead, the peptide itself is rapidly oxidized. Similarly, Zn(II)-ZIF268-3D and apo-ZIF268-3D are rapidly oxidized by H(2)O(2) or O(2), and we propose that ZIF268-3D is highly susceptible to oxidation., (© 2011 American Chemical Society)

Published

2011

35. A new solvatochromic fluorophore for exploring nonpolar environments created by biopolymers.

Author

Fakhari M A and Rokita SE

Subjects

Base Sequence, DNA analysis, Hexanes chemistry, Naphthalenes chemistry, Quantum Theory, Solvents chemistry, Spectrometry, Fluorescence methods, Water chemistry, Biopolymers chemistry

Abstract

The fluorescence of a new aminocyanonaphthalene exhibits exquisite sensitivity to its environment and responds to a solvent change from water to hexane with greater than a 100-fold increase in intensity and 100 nm shift in λ(max.em). These properties should support many applications including the detection of abasic sites within duplex DNA as illustrated below.

Published

2011

36. Trapping a labile adduct formed between an ortho-quinone methide and 2'-deoxycytidine.

Author

McCrane MP, Weinert EE, Lin Y, Mazzola EP, Lam YF, Scholl PF, and Rokita SE

Subjects

Alkylation, Molecular Structure, Oxidation-Reduction, Stereoisomerism, Deoxycytidine chemistry, Indolequinones chemistry

Abstract

Selective oxidation by bis[(trifluoroacetoxy)iodo]benzene (BTI) provides an effective trap for quenching adducts formed reversibly between dC and an ortho-quinone methide (QM) under physiological conditions. A model adduct generated by 4-methyl-o-QM and 2'-deoxycytidine is rapidly converted by intramolecular cyclization and loss of aromaticity to a characteristic product for quantifying QM alkylation. However, BTI induces a surprising rearrangement driven by overoxidation of a derivative lacking an alkyl substituent at the 4-position of the QM.

Published

2011

37. Few constraints limit the design of quinone methide-oligonucleotide self-adducts for directing DNA alkylation.

Author

Rossiter CS, Modica E, Kumar D, and Rokita SE

Subjects

Alkylation, Base Sequence, Molecular Sequence Data, Nucleic Acid Conformation, DNA chemistry, DNA Adducts chemistry, Indolequinones chemistry, Oligodeoxyribonucleotides chemistry

Abstract

Nucleotide sequences minimally containing adenosine, cytosine or guanosine are sufficient to form intrastrand oligonucleotide quinone methide self-adducts reversibly for subsequent alkylation of complementary DNA. The general lack of sequence restrictions should now allow for alkylation of most any target of interest although reaction is most efficient when the self-adducts contain guanine residues and do not form hairpin structures.

Published

2011

38. Efficient use and recycling of the micronutrient iodide in mammals.

Author

Rokita SE, Adler JM, McTamney PM, and Watson JA Jr

Subjects

Animals, Humans, Iodide Peroxidase genetics, Iodide Peroxidase metabolism, Micronutrients metabolism, Mutagenesis, Site-Directed, Thyroid Gland metabolism, Iodides metabolism

Abstract

Daily ingestion of iodide alone is not adequate to sustain production of the thyroid hormones, tri- and tetraiodothyronine. Proper maintenance of iodide in vivo also requires its active transport into the thyroid and its salvage from mono- and diiodotyrosine that are formed in excess during hormone biosynthesis. The enzyme iodotyrosine deiodinase responsible for this salvage is unusual in its ability to catalyze a reductive dehalogenation reaction dependent on a flavin cofactor, FMN. Initial characterization of this enzyme was limited by its membrane association, difficult purification and poor stability. The deiodinase became amenable to detailed analysis only after identification and heterologous expression of its gene. Site-directed mutagenesis recently demonstrated that cysteine residues are not necessary for enzymatic activity in contrast to precedence set by other reductive dehalogenases. Truncation of the N-terminal membrane anchor of the deiodinase has provided a soluble and stable source of enzyme sufficient for crystallographic studies. The structure of an enzyme.substrate co-crystal has become invaluable for understanding the origins of substrate selectivity and the mutations causing thyroid disease in humans., (Copyright (c) 2010 Elsevier Masson SAS. All rights reserved.)

Published

2010

39. Dynamic cross-linking is retained in duplex DNA after multiple exchange of strands.

Author

Wang H and Rokita SE

Subjects

Alkylation, Indolequinones chemistry, Nucleic Acid Conformation, Cross-Linking Reagents chemistry, Oligonucleotides chemistry

Published

2010

40. Modulating the ground- and excited-state oxidation potentials of diaminonaphthalene by sequential N-methylation.

Author

Campbell NP, Finch AS, and Rokita SE

Abstract

A series of 1,5-diaminonaphthalene derivatives were synthesized and characterized to provide ground- and excited-state electron donors of similar structure but varying potential. Electrochemical and spectroscopic properties of the series are reported and together illustrate two opposing consequences of alkyl substitution on the aryl amines. Inductive effects of methylation are evident from the decrease in ground-state oxidation potential for derivatives containing monomethylamino substituents. In contrast, steric effects seem to dominate the increase in the ground-state oxidation potential of derivatives containing dimethylamino substituents since the conformational constraints created by dimethylation suppress delocalization of the nonbonding electrons. Absorption and emission properties also respond to increasing levels of N-methylation, and the excited-state oxidation potentials of the parent 1,5-diaminonaphthalene and its monomethylamine derivatives (ca. -3.2 V) are approximately 200 mV lower than the corresponding dimethylamino derivatives (-3.0 V).

Published

2010

41. A mammalian reductive deiodinase has broad power to dehalogenate chlorinated and brominated substrates.

Author

McTamney PM and Rokita SE

Subjects

Electron Spin Resonance Spectroscopy, Flavins chemistry, Flavins metabolism, Hydrocarbons, Brominated metabolism, Hydrocarbons, Chlorinated metabolism, Iodide Peroxidase metabolism, Kinetics, Oxidation-Reduction, Hydrocarbons, Brominated chemistry, Hydrocarbons, Chlorinated chemistry, Iodide Peroxidase chemistry

Abstract

Iodotyrosine deiodinase is essential for iodide homeostasis and proper thyroid function in mammals. This enzyme promotes a net reductive deiodination of 3-iodotyrosine to form iodide and tyrosine. Such a reductive dehalogenation is uncommon in aerobic organisms, and its requirement for flavin mononucleotide is even more uncommon in catalysis. Reducing equivalents are now shown to transfer directly from the flavin to the halogenated substrate without involvement of other components typically included in the standard enzymatic assay. Additionally, the deiodinase has been discovered to act as a debrominase and a dechlorinase. These new activities expand the possible roles of flavin in biological catalysis and provide a foundation for determining the mechanism of this unusual process.

Published

2009

42. Crystal structure of iodotyrosine deiodinase, a novel flavoprotein responsible for iodide salvage in thyroid glands.

Author

Thomas SR, McTamney PM, Adler JM, Laronde-Leblanc N, and Rokita SE

Subjects

Animals, Binding Sites, Carbon chemistry, Cell Line, Crystallization, Diiodotyrosine metabolism, Flavin Mononucleotide chemistry, Flavin Mononucleotide metabolism, Iodide Peroxidase genetics, Iodine chemistry, Mice, Models, Molecular, Mutation, Protein Binding, Protein Structure, Tertiary, Spodoptera, Substrate Specificity, X-Ray Diffraction, Iodide Peroxidase chemistry, Iodide Peroxidase metabolism, Iodides metabolism, Thyroid Gland metabolism

Abstract

The flavoprotein iodotyrosine deiodinase (IYD) salvages iodide from mono- and diiodotyrosine formed during the biosynthesis of the thyroid hormone thyroxine. Expression of a soluble domain of this membrane-bound enzyme provided sufficient material for crystallization and characterization by x-ray diffraction. The structures of IYD and two co-crystals containing substrates, mono- and diiodotyrosine, alternatively, were solved at resolutions of 2.0, 2.45, and 2.6 A, respectively. The structure of IYD is homologous to others in the NADH oxidase/flavin reductase superfamily, but the position of the active site lid in IYD defines a new subfamily within this group that includes BluB, an enzyme associated with vitamin B(12) biosynthesis. IYD and BluB also share key interactions involving their bound flavin mononucleotide that suggest a unique catalytic behavior within the superfamily. Substrate coordination to IYD induces formation of an additional helix and coil that act as an active site lid to shield the resulting substrate.flavin complex from solvent. This complex is stabilized by aromatic stacking and extensive hydrogen bonding between the substrate and flavin. The carbon-iodine bond of the substrate is positioned directly over the C-4a/N-5 region of the flavin to promote electron transfer. These structures now also provide a molecular basis for understanding thyroid disease based on mutations of IYD.

Published

2009

43. Hydrogen peroxide and dioxygen activation by dinuclear copper complexes in aqueous solution: hydroxyl radical production initiated by internal electron transfer.

Author

Zhu Q, Lian Y, Thyagarajan S, Rokita SE, Karlin KD, and Blough NV

Subjects

Electrons, Hydroxyl Radical chemistry, Organometallic Compounds chemistry, Pyridines chemistry, Solutions, Water chemistry, Copper chemistry, Hydrogen Peroxide chemistry, Oxygen chemistry

Abstract

Dinuclear Cu(II) complexes, CuII2Nn (n = 4 or 5), were recently found to specifically cleave DNA in the presence of a reducing thiol and O2 or in the presence of H2O2 alone. However, CuII2N3 and a closely related mononuclear Cu(II) complex exhibited no selective reaction under either condition. Spectroscopic studies indicate an intermediate is generated from CuII2Nn (n = 4 or 5) and mononuclear Cu(II) solutions in the presence of H2O2 or from CuI2Nn (n = 4 or 5) in the presence of O2. This intermediate decays to generate OH radicals and ligand degradation products at room temperature. The lack of reactivity of the intermediate with a series of added electron donors suggests the intermediate discharges through a rate-limiting intramolecular electron transfer from the ligand to the metal peroxo center to produce an OH radical and a ligand-based radical. These results imply that DNA cleavage does not result from direct reaction with a metal-peroxo intermediate but instead arises from reaction with either OH radicals or ligand-based radicals.

Published

2008

44. Flavoprotein iodotyrosine deiodinase functions without cysteine residues.

Author

Watson JA Jr, McTamney PM, Adler JM, and Rokita SE

Subjects

Amino Acid Sequence, Cell Line, Cell Membrane enzymology, Cysteine genetics, Cysteine metabolism, Flavoproteins genetics, Homeostasis, Humans, Iodide Peroxidase genetics, Iodides chemistry, Kinetics, Molecular Structure, Flavoproteins chemistry, Flavoproteins metabolism, Iodide Peroxidase chemistry, Iodide Peroxidase metabolism

Published

2008

45. Immortalizing a transient electrophile for DNA cross-linking.

Author

Wang H, Wahi MS, and Rokita SE

Subjects

Base Sequence, Cross-Linking Reagents chemistry, DNA chemistry

Published

2008

46. Self-repair of thymine dimer in duplex DNA.

Author

Holman MR, Ito T, and Rokita SE

Subjects

Base Composition, Base Sequence, Oligonucleotides chemical synthesis, Oligonucleotides chemistry, Photochemistry, DNA chemistry, DNA radiation effects, DNA Repair, Pyrimidine Dimers chemistry

Published

2007

47. Substituents on quinone methides strongly modulate formation and stability of their nucleophilic adducts.

Author

Weinert EE, Dondi R, Colloredo-Melz S, Frankenfield KN, Mitchell CH, Freccero M, and Rokita SE

Subjects

Binding, Competitive, Drug Stability, Kinetics, Nuclear Magnetic Resonance, Biomolecular, Nucleosides chemistry, Photolysis, Structure-Activity Relationship, Indolequinones chemistry

Abstract

Electronic perturbation of quinone methides (QM) greatly influences their stability and in turn alters the kinetics and product profile of QM reaction with deoxynucleosides. Consistent with the electron-deficient nature of this reactive intermediate, electron-donating substituents are stabilizing and electron-withdrawing substituents are destabilizing. For example, a dC N3-QM adduct is made stable over the course of observation (7 days) by the presence of an electron-withdrawing ester group that inhibits QM regeneration. Conversely, a related adduct with an electron-donating methyl group is very labile and regenerates its QM with a half-life of approximately 5 h. The generality of these effects is demonstrated with a series of alternative quinone methide precursors (QMP) containing a variety of substituents attached at different positions with respect to the exocyclic methylene. The rates of nucleophilic addition to substituted QMs measured by laser flash photolysis similarly span 5 orders of magnitude with electron-rich species reacting most slowly and electron-deficient species reacting most quickly. The reversibility of QM reaction can now be predictably adjusted for any desired application.

Published

2006

48. Targeted guanine oxidation by a dinuclear copper(II) complex at single stranded/double stranded DNA junctions.

Author

Li L, Murthy NN, Telser J, Zakharov LN, Yap GP, Rheingold AL, Karlin KD, and Rokita SE

Subjects

3-Mercaptopropionic Acid chemistry, Crystallography, X-Ray, Electrochemistry, Electron Spin Resonance Spectroscopy, Free Radical Scavengers chemistry, Magnetic Resonance Spectroscopy, Models, Molecular, Molecular Structure, Organometallic Compounds chemical synthesis, Oxidation-Reduction, Sensitivity and Specificity, Spectrometry, Mass, Electrospray Ionization, Copper chemistry, DNA chemistry, DNA, Single-Stranded chemistry, Guanine chemistry, Organometallic Compounds chemistry

Abstract

A dinuclear copper(II) complex [Cu(II)2(PD'O-)(H2O)2](ClO4)3 (5) with terminal Cu(II)-H(2)O moieties and a Cu...Cu distance of 4.13 A (X-ray structure) has been synthesized and characterized by EPR spectroscopy (ferromagnetic coupling observed) and cyclic voltammetry. Dizinc(II) and mononuclear copper(II) analogues [Zn(II)2(PD'O-)(H2O)2]3+ (7) and [Cu(II)(mPD'OH)(H2O)]2+ (6), respectively, have also been synthesized and structurally characterized. Reacting 5/MPA/O(2) (MPA = 3-mercaptopropionic acid) with DNA leads to a highly specific oxidation of guanine (G) at a junction between single- and double-stranded DNA. Mass spectrometric analysis of the major products indicates a gain of +18 and +34 amu relative to initial DNA strands. The most efficient reaction requires G at the first and second unpaired positions of each strand extending from the junction. Less reaction is observed for analogous targets in which the G cluster is farther from the junction or contains less than four Gs. Consistent with our previous systems, the multinuclear copper center is required for selective reaction; mononuclear complex 6 is not effective. Hydrogen peroxide as a substitute for MPA/O2 also does not lead to activity. Structural analysis of a [Cu(II)2(PD'O-)(G)]3+ complex (8) and dizinc analogue [Zn(II)(2)(PD'O-)(G)](ClO4)3 (9) (G = guanosine) reveals coordination of the G O6 and N7 atoms with the two copper (or zinc) centers and suggests that copper-G coordination likely plays a role in recognition of the DNA target. The Cu2-O2 intermediate responsible for guanine oxidation appears to be different from that responsible for direct-strand scission induced by other multinuclear copper complexes; the likely course of reaction is discussed.

Published

2006

49. Selective DNA strand scission with binuclear copper complexes: implications for an active Cu2-O2 species.

Author

Thyagarajan S, Murthy NN, Narducci Sarjeant AA, Karlin KD, and Rokita SE

Subjects

3-Mercaptopropionic Acid chemistry, DNA metabolism, Free Radical Scavengers chemistry, Hydrogen Peroxide chemistry, Ligands, Nucleic Acid Heteroduplexes chemistry, Oxidation-Reduction, Oxygen chemistry, Spectrophotometry, Ultraviolet, Copper chemistry, DNA chemistry

Abstract

A homologous series of binuclear copper(II) complexes [Cu(II)(2)(Nn)(Y)(2)](2+) (1-3) (n = 3-5 and Y = (ClO(4))(-) or (NO(3))(-)) were studied to investigate the intermediate(s) responsible for selective DNA strand scission in the presence of MPA/O(2) (MPA = 3-mercaptopropanoic acid). While the N3 complex does not react, the N4 and N5 analogues show comparable activity with strand scission occurring at a single-strand/double-strand junction. Identical reactivity is also observed in the alternate presence of H(2)O(2). Spectroscopic and reactivity studies with [Cu(II)(2)(N4)(Y)(2)](2+) (2) and H(2)O(2) are consistent with DNA oxidation mediated by formation of a side-on peroxodicopper(II) (Cu(2)-O(2)) complex.

Published

2006

50. Iodotyrosine deiodinase is the first mammalian member of the NADH oxidase/flavin reductase superfamily.

Author

Friedman JE, Watson JA Jr, Lam DW, and Rokita SE

Subjects

Amino Acid Sequence, Animals, Conserved Sequence, Cysteine, FMN Reductase classification, FMN Reductase isolation & purification, Humans, Iodide Peroxidase classification, Iodide Peroxidase isolation & purification, Microsomes enzymology, Protein Structure, Tertiary, Sequence Analysis, Swine, Thyroid Gland enzymology, FMN Reductase chemistry, Iodide Peroxidase chemistry

Abstract

The enzyme responsible for iodide salvage in the thyroid, iodotyrosine deiodinase, was solubilized from porcine thyroid microsomes by limited proteolysis with trypsin. The resulting protein retained deiodinase activity and was purified using anion exchange, dye, and hydrophobic chromatography successively. Peptide sequencing of the final isolate identified the gene responsible for the deiodinase. The amino acid sequence of the porcine enzyme is highly homologous to corresponding genes in a variety of mammals including humans, and the mouse gene was expressed in human embryonic kidney 293 cells to confirm its identity. The amino acid sequence of the deiodinase suggests the presence of three domains. The N-terminal domain provides a membrane anchor. The intermediate domain contains the highest sequence variability and lacks homology to structural motifs available in the common databases. The C-terminal domain is highly conserved and resembles bacterial enzymes of the NADH oxidase/flavin reductase superfamily. A three-dimensional model of the deiodinase based on the coordinates of the minor nitroreductase of Escherichia coli indicates that a Cys common to all of the mammal sequences is located adjacent to bound FMN. However, the deiodinase is not structurally related to other known flavoproteins containing redox-active cysteines or the iodothyronine deiodinases containing an active site selenocysteine.

Published

2006