Intersubunit Interactions in Plasmodium falciparumThioredoxin Reductase

Krnajski, Zita; Gilberger, Tim‐Wolf; Walter, Rolf D.; Müller, Sylke

doi:10.1074/jbc.m008443200

Cited by 23 publications

(26 citation statements)

References 28 publications

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“…The authors (15) suggested that the mobile selenenylsulfide containing a C-terminal tail not only serves as a third redox active group, but it also blocks oxidized glutathione from binding to the enzyme. In addition, the structure confirmed the obligatory ''head-to-tail'' arrangement of high-M r TrxR, with the redox-active C-terminal tail of one subunit interacting with the active site of the opposing subunit (36,37). Unfortunately, the observed conformation of the C-terminal tail precluded direct interaction with the active-site disulfide͞dithiol group, suggesting an additional catalytically competent structural arrangement must exist.…”

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confidence: 64%

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Crystal structures of oxidized and reduced mitochondrial thioredoxin reductase provide molecular details of the reaction mechanism

Biterova

Turanov

Gladyshev

et al. 2005

Proc. Natl. Acad. Sci. U.S.A.

107

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Thioredoxin reductase (TrxR) is an essential enzyme required for the efficient maintenance of the cellular redox homeostasis, particularly in cancer cells that are sensitive to reactive oxygen species. In mammals, distinct isozymes function in the cytosol and mitochondria. Through an intricate mechanism, these enzymes transfer reducing equivalents from NADPH to bound FAD and subsequently to an active-site disulfide. In mammalian TrxRs, the dithiol then reduces a mobile C-terminal selenocysteine-containing tetrapeptide of the opposing subunit of the dimer. Once activated, the C-terminal redox center reduces a disulfide bond within thioredoxin. In this report, we present the structural data on a mitochondrial TrxR, TrxR2 (also known as TR3 and TxnRd2). Mouse TrxR2, in which the essential selenocysteine residue had been replaced with cysteine, was isolated as a FAD-containing holoenzyme and crystallized (2.6 Å; R ‫؍‬ 22.2%; Rfree ‫؍‬ 27.6%). The addition of NADPH to the TrxR2 crystals resulted in a color change, indicating reduction of the active-site disulfide and formation of a species presumed to be the flavin-thiolate charge transfer complex. Examination of the NADP(H)-bound model (3.0 Å; R ‫؍‬ 24.1%; R free ‫؍‬ 31.2%) indicates that an active-site tyrosine residue must rotate from its initial position to stack against the nicotinamide ring of NADPH, which is juxtaposed to the isoalloxazine ring of FAD to facilitate hydride transfer. Detailed analysis of the structural data in conjunction with a model of the unusual C-terminal selenenylsulfide suggests molecular details of the reaction mechanism and highlights evolutionary adaptations among reductases.hioredoxins are the major cellular protein disulfide reductases and are responsible for the regulation of numerous biochemical processes within the cell (1). These proteins are maintained in a reduced state by thioredoxin reductases (TrxR), homodimeric f lavoproteins that catalyze the NADPHdependent reduction of thioredoxins (2, 3).Two forms of TrxRs have evolved with related but distinct modes of catalysis (2-5). Low-M r TrxRs (M r Ϸ 35 kDa) are typically found in prokaryotes, archaea, plants, and lower eukaryotes, whereas high-M r TrxRs (M r Ϸ 55 kDa) are observed in higher eukaryotes. To date, only the green algae Chlamydomonas reinhardtii has been shown to contain both a low-and a high-M r TrxR (6).The general features of catalysis are retained in both low-and high-M r TrxR (2, 4). TrxR transfers reducing equivalents from NADPH to its bound FAD, ultimately leading to the reduction of an active-site disulfide. In low-M r TrxRs, the catalytic cycle requires a large conformational change after dithiol activation (4,7,8). In high-M r TrxR, the active-site dithiol reduces a third redox active center in the highly mobile C terminus of the opposing subunit. This third group is responsible for the reduction of the disulfide bond within thioredoxin. Its nature is species-specific and ranges from a C-X-X-X-X-C disulfide in Plasmodium falciparum (9) to a vicinal disulfid...

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confidence: 64%

“…The precise mechanism of selenenylsulfide͞disulfide exchange has not yet been determined for mammalian TrxRs, but studies of D. melanogaster (DmTrxR1) (26,48,49) and P. falciparum (27,37,50) high-M r TrxRs provide considerable insight. DmTrxR1 exhibits significant sequence homology to mammalian TrxRs but is not a selenoprotein (26,48).…”

Section: Figmentioning

confidence: 99%

Crystal structures of oxidized and reduced mitochondrial thioredoxin reductase provide molecular details of the reaction mechanism

Biterova

Turanov

Gladyshev

et al. 2005

Proc. Natl. Acad. Sci. U.S.A.

107

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“…A key intermediate in catalysis is a charge transfer complex (the thiolate of Cys93 is the donor and flavin is the acceptor) characterized by a long-wavelength absorbance around 540 nm. [183,184] A high-throughput-screening program with 350 000 compounds of the Pfizer library yielded about 30 compounds that inhibit thioredoxin reductase. The bewildering chemical diversity among these hits was resolved by Davioud-Charvet et al, who noted that most of them were Mannich bases.…”

Section: Thioredoxin Reductase As a Validated Drug Targetmentioning

confidence: 99%

“…The gene was identified in the genome of P. falciparum, cloned, and expressed as a recombinant functional flavoenzyme. [152,[182][183][184] Subsequently, Müller and co-workers used gene-ablation and gene-substitution techniques to show that thioredoxin reductase is an essential enzyme for the blood stages of P. falciparum. [153,154] These studies validated thioredoxin reductase as a drug target.…”

Section: Thioredoxin Reductase As a Validated Drug Targetmentioning

confidence: 99%

Dithiol Proteins as Guardians of the Intracellular Redox Milieu in Parasites: Old and New Drug Targets in Trypanosomes and Malaria‐Causing Plasmodia

2005

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Parasitic diseases such as sleeping sickness, Chagas' heart disease, and malaria are major health problems in poverty-stricken areas. Antiparasitic drugs that are not only active but also affordable and readily available are urgently required. One approach to finding new drugs and rediscovering old ones is based on enzyme inhibitors that paralyze antioxidant systems in the pathogens. These antioxidant ensembles are essential to the parasites as they are attacked in the human host by strong oxidants such as peroxynitrite, hypochlorite, and H2O2. The pathogen-protecting system consists of some 20 thiol and dithiol proteins, which buffer the intraparasitic redox milieu at a potential of -250 mV. In trypanosomes and leishmania the network is centered around the unique dithiol trypanothione (N1,N8-bis(glutathionyl)spermidine). In contrast, malaria parasites have a more conservative dual antioxidative system based on glutathione and thioredoxin. Inhibitors of antioxidant enzymes such as trypanothione reductase are, indeed, parasiticidal but they can also delay or prevent resistance against a number of other antiparasitic drugs.

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“…These homodimeric proteins contain three redox-active centers that are in redox communication: a tightly bound FAD, a pair of redox-active cysteines on one of the subunits that we will refer to as the N-terminal pair (Cys-88 and Cys-93 in Scheme 1, for PfTrxR), and a pair of redox-active cysteines or a cysteine-selenocysteine pair that we will refer to as the C-terminal pair (Cys-535Ј and Cys-540Ј, for PfTrxR) located on the second subunit (15,22,23,24). The reductive and oxidative half-reactions of Drosophila melanogaster TrxR (DmTrxR) have been examined in some detail to obtain a better understanding of the underlying catalytic mechanism of high-M r TrxRs.…”

mentioning

confidence: 99%

Identification of Acid-Base Catalytic Residues of High-Mr Thioredoxin Reductase from Plasmodium falciparum

McMillan

Arscott

Ballou

et al. 2006

Journal of Biological Chemistry

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High-M r thioredoxin reductase from the malaria parasite Plasmodium falciparum (PfTrxR) contains three redox active centers (FAD, Cys-88/Cys-93, and Cys-535/Cys-540) that are in redox communication. The catalytic mechanism of PfTrxR, which involves dithiol-disulfide interchanges requiring acidbase catalysis, was studied by steady-state kinetics, spectral analyses of anaerobic static titrations, and rapid kinetics analysis of wild-type enzyme and variants involving the His-509-Glu-514 dyad as the presumed acid-base catalyst. The dyad is conserved in all members of the enzyme family. Substitution of His-509 with glutamine and Glu-514 with alanine led to TrxR with only 0.5 and 7% of wild type activity, respectively, thus demonstrating the crucial roles of these residues for enzymatic activity. The H509Q variant had rate constants in both the reductive and oxidative half-reactions that were dramatically less than those of wild-type enzyme, and no thiolateflavin charge-transfer complex was observed. Glu-514 was shown to be involved in dithiol-disulfide interchange between the Cys-88/Cys-93 and Cys-535/Cys-540 pairs. In addition, Glu-514 appears to greatly enhance the role of His-509 in acid-base catalysis. It can be concluded that the His-509-Glu-514 dyad, in analogy to those in related oxidoreductases, acts as the acid-base catalyst in PfTrxR.

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Intersubunit Interactions in Plasmodium falciparumThioredoxin Reductase

Cited by 23 publications

References 28 publications

Crystal structures of oxidized and reduced mitochondrial thioredoxin reductase provide molecular details of the reaction mechanism

Crystal structures of oxidized and reduced mitochondrial thioredoxin reductase provide molecular details of the reaction mechanism

Dithiol Proteins as Guardians of the Intracellular Redox Milieu in Parasites: Old and New Drug Targets in Trypanosomes and Malaria‐Causing Plasmodia

Identification of Acid-Base Catalytic Residues of High-Mr Thioredoxin Reductase from Plasmodium falciparum

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