ABSTRACT
Cytochrome c oxidase (CcOX) containing binuclear heme a3-Cu B centre (BNC) mechanises the process of electron transfer in the last phase of cellular respiration. The molecular modelling based structural analysis of CcOX - heme a3-Cu B complex was performed and the disturbance to this complex under cyanide poisoning conditions was investigated. Taking into consideration the results of molecular docking studies, new chemical entities were developed for clipping cyanide from the enzyme and restoring its normal function. It was found that the molecules obtained by combining syringaldehyde, oxindole and chrysin moieties bearing propyl/butyl spacing groups occupy the BNC region and effectively remove cyanide bound to the enzyme. The binding constant of compound 2 with CN- was 2.3â¯×â¯105â¯M-1 and its ED50 for restoring the cyanide bound CcOX activity in 10â¯min was 16⯵M. The compound interacted with CN- over the pH range 5-10. The comparison of the loss of enzymatic activity in the presence of CN- and resumption of enzymatic activity by compound 2 mediated removal of CN- indicated the efficacy of the compound as antidote of cyanide.
Subject(s)
Cyanides/chemistry , Electron Transport Complex IV/chemistry , Enzyme Reactivators/chemistry , Flavonoids/chemistry , Indoles/chemistry , Antidotes/chemical synthesis , Antidotes/chemistry , Drug Design , Enzyme Reactivators/chemical synthesis , Flavonoids/chemical synthesis , Humans , Indoles/chemical synthesisABSTRACT
Caspase-8 constructs featuring an N-terminal FGG sequence allow for selective twofold recognition by cucurbit[8]uril, which leads to an increase of the enzymatic activity in a cucurbit[8]uril dose-dependent manner. This supramolecular switching has enabled for the first time the study of the same caspase-8 in its two extreme states; as full monomer and as cucurbit[8]uril induced dimer. A mutated, fully monomeric caspase-8 (D384A), which is enzymatically inactive towards its natural substrate caspase-3, could be fully reactivated upon addition of cucurbit[8]uril. In its monomeric state caspase-8 (D384A) still processes a small synthetic substrate, but not the natural caspase-3 substrate, highlighting the close interplay between protein dimerization and active site rearrangement for substrate selectivity. The ability to switch the caspase-8 activity by a supramolecular system thus provides a flexible approach to studying the activity of a protein at different oligomerization states.
Subject(s)
Bridged-Ring Compounds/chemistry , Caspase 8/metabolism , Enzyme Reactivators/chemistry , Imidazoles/chemistry , Caspase 8/genetics , Catalysis/drug effects , Humans , Point Mutation , Protein Multimerization/drug effectsABSTRACT
Organophosphorus agents are potent inhibitors of acetylcholinesterase. Inhibition involves successive chemical events. The first is phosphylation of the active site serine to produce a neutral adduct, which is a close structural analog of the acylation transition state. This adduct is unreactive toward spontaneous hydrolysis, but in many cases can be reactivated by nucleophilic medicinal agents, such as oximes. However, the initial phosphylation reaction may be followed by a dealkylation reaction of the incipient adduct. This reaction is called aging and produces an anionic phosphyl adduct with acetylcholinesterase that is refractory to reactivation. This review considers why the anionic aged adduct is unreactive toward nucleophiles. An alternate approach is to realkylate the aged adduct, which would render the adduct reactivatable with oxime nucleophiles. However, this approach confronts a considerable-and perhaps intractable-challenge: the aged adduct is a close analog of the deacylation transition state. Consequently, the evolutionary mechanisms that have led to transition state stabilization in acetylcholinesterase catalysis are discussed herein, as are the challenges that they present to reactivation of aged acetylcholinesterase.
Subject(s)
Acetylcholinesterase/chemistry , Cholinesterase Inhibitors/chemistry , Enzyme Reactivators/chemistry , Organophosphorus Compounds/chemistry , Catalysis , Catalytic Domain , Humans , Kinetics , Models, Molecular , Molecular Structure , Oximes/chemistry , Serine/chemistry , Structure-Activity Relationship , ThermodynamicsABSTRACT
Diol dehydratase-reactivase (DD-R) is a molecular chaperone that reactivates inactivated holodiol dehydratase (DD) by cofactor exchange. Its ADP-bound and ATP-bound forms are high-affinity and low-affinity forms for DD, respectively. Among DD-Rs mutated at the nucleotide-binding site, neither the Dα8N nor Dα413N mutant was effective as a reactivase. Although Dα413N showed ATPase activity, it did not mediate cyanocobalamin (CN-Cbl) release from the DD·CN-Cbl complex in the presence of ATP or ADP and formed a tight complex with apoDD even in the presence of ATP, suggesting the involvement of Aspα413 in the nucleotide switch. In contrast, Dα8N showed very low ATPase activity and did not mediate CN-Cbl release from the complex in the presence of ATP, but it did cause about 50% release in the presence of ADP. The complex formation of this mutant with DD was partially reversed by ATP, suggesting that Aspα8 is involved in the ATPase activity but only partially in the nucleotide switch. Among DD-Rs mutated at the Mg(2+)-binding site, only Eß31Q was about 30% as active as wild-type DD-R and formed a tight complex with apoDD, indicating that the DD-R ß subunit is not absolutely required for reactivation. If subunit swapping occurs between the DD-R ß and DD ß subunits, Gluß97 of DD would coordinate to Mg(2+). The complex of Eß97Q DD with CN-Cbl was not activated by wild-type DD-R. No complex was formed between this mutant and wild-type DD-R, indicating that the coordination of Gluß97 to Mg(2+) is essential for subunit swapping and therefore for (re)activation.
Subject(s)
Molecular Chaperones/chemistry , Nucleotides/metabolism , Propanediol Dehydratase/chemistry , Amino Acid Sequence , Bacterial Proteins/chemistry , Bacterial Proteins/physiology , Binding Sites , Enzyme Reactivators/chemistry , Humans , Kinetics , Klebsiella oxytoca/enzymology , Metals/chemistry , Models, Molecular , Molecular Sequence Data , Protein Binding , Protein Interaction Domains and Motifs/physiologyABSTRACT
An intriguing mystery about tryptophan 2,3-dioxygenase is its hydrogen peroxide-triggered enzyme reactivation from the resting ferric oxidation state to the catalytically active ferrous form. In this study, we found that such an odd Fe(III) reduction by an oxidant depends on the presence of L-Trp, which ultimately serves as the reductant for the enzyme. In the peroxide reaction with tryptophan 2,3-dioxygenase, a previously unknown catalase-like activity was detected. A ferryl species (δ = 0.055 mm/s and ΔE(Q) = 1.755 mm/s) and a protein-based free radical (g = 2.0028 and 1.72 millitesla linewidth) were characterized by Mössbauer and EPR spectroscopy, respectively. This is the first compound ES-type of ferryl intermediate from a heme-based dioxygenase characterized by EPR and Mössbauer spectroscopy. Density functional theory calculations revealed the contribution of secondary ligand sphere to the spectroscopic properties of the ferryl species. In the presence of L-Trp, the reactivation was demonstrated by enzyme assays and by various spectroscopic techniques. A Trp-Trp dimer and a monooxygenated L-Trp were both observed as the enzyme reactivation by-products by mass spectrometry. Together, these results lead to the unraveling of an over 60-year old mystery of peroxide reactivation mechanism. These results may shed light on how a metalloenzyme maintains its catalytic activity in an oxidizing environment.
Subject(s)
Bacterial Proteins/chemistry , Catalase/chemistry , Cupriavidus/enzymology , Enzyme Reactivators/chemistry , Hydrogen Peroxide/chemistry , Tryptophan Oxygenase/chemistry , Bacterial Proteins/metabolism , Catalase/metabolism , Electron Spin Resonance Spectroscopy , Enzyme Reactivators/metabolism , Hydrogen Peroxide/metabolism , Iron/chemistry , Iron/metabolism , Oxidation-Reduction , Tryptophan Oxygenase/metabolismABSTRACT
A new prenylated dihydroflavonol, 3-hydroxy-kenusanone B 1, as well as three other known isoflavanones, sophoronol 2, sophoraisoflavanone A 3 and kenusanone H 4, were isolated from the rhizomes of Echinosophora koreensis. The structures of these compounds were elucidated using spectroscopic analyses that included extensive 2D NMR, optical rotation spectrometry and mass spectrometry. All four flavonoids enhanced the activities of alcohol metabolizing enzymes such as alcohol dehydrogenase (ADH) and aldehyde dehydrogenase (ALDH) at micromolar concentrations. Sophoronol 2 showed a nine-fold increased activation of alcohol dehydrogenase and aldehyde dehydrogenase than a negative control group at concentrations of 100 microg/mL and 50 microg/mL, respectively. This study suggests that prenylated flavonoids have the potential to prevent 'hangovers' after alcohol intake.
Subject(s)
Alcohol Dehydrogenase/metabolism , Aldehyde Dehydrogenase/metabolism , Enzyme Reactivators/pharmacology , Flavonols/pharmacology , Isoflavones/pharmacology , Sophora/chemistry , Enzyme Reactivators/chemistry , Enzyme Reactivators/isolation & purification , Flavonols/chemistry , Flavonols/isolation & purification , In Vitro Techniques , Isoflavones/chemistry , Isoflavones/isolation & purification , Molecular Structure , Plant Extracts/chemistry , Plant Extracts/pharmacology , PrenylationABSTRACT
Casualties caused by organophosphorus pesticides are a burden for health systems in developing and poor countries. Such compounds are potent acetylcholinesterase irreversible inhibitors, and share the toxic profile with nerve agents. Pyridinium oximes are the only clinically available antidotes against poisoning by these substances, but their poor penetration into the blood-brain barrier hampers the efficient enzyme reactivation at the central nervous system. In searching for structural factors that may be explored in future SAR studies, we evaluated neutral aryloximes as reactivators for paraoxon-inhibited Electrophorus eel acetylcholinesterase. Our findings may result into lead compounds, useful for development of more active compounds for emergencies and supportive care.
Subject(s)
Acetylcholinesterase/metabolism , Electrophorus/metabolism , Enzyme Reactivators/pharmacology , Oximes/pharmacology , Paraoxon/toxicity , Animals , Enzyme Reactivators/chemistry , Fish Proteins/metabolism , In Vitro Techniques , Molecular Structure , Oximes/chemistry , Structure-Activity RelationshipABSTRACT
One of the therapeutic approaches to organophosphate poisoning is to reactivate AChE with site-directed nucleophiles such as oximes. However, pyridinium oximes 2-PAM, HI-6, TMB-4 and obidoxime, found as the most effective reactivators, have limiting reactivating potency in tabun poisoning. We tested oximes varying in the type of ring (pyridinium and/or imidazolium), the length and type of the linker between rings, and in the position of the oxime group on the ring to find more effective oximes to reactivate tabun-inhibited human erythrocyte AChE. Three of our tested pyridinium oximes K027, K048, K074, along with TMB-4, were the most promising for AChE reactivation. Promising oximes were further tested in vivo on tabun poisoned mice not only as antidotes in combination with atropine but also as pretreatment drug. Herein, we showed that a promising treatment in tabun poisoning by selected oximes and atropine could be improved if oximes are also used in pretreatment. Since the reactivating efficacy of the oximes in vitro corresponded to their therapeutic efficacy in vivo, it seems that pharmacological effect of these oximes is indeed primarily related to the reactivation of tabun-phosphorylated AChE.
Subject(s)
Acetylcholinesterase/metabolism , Antidotes/therapeutic use , Cholinesterase Inhibitors/poisoning , Enzyme Reactivators/therapeutic use , Organophosphate Poisoning , Oximes/therapeutic use , Animals , Antidotes/chemistry , Antidotes/pharmacology , Enzyme Reactivators/chemistry , Enzyme Reactivators/pharmacology , Male , Mice , Mice, Inbred BALB C , Organophosphates , Oximes/chemistry , Oximes/pharmacology , Phosphorylation , Poisoning/drug therapyABSTRACT
Liver mitochondrial aldehyde dehydrogenase 2 (ALDH2) enzyme is responsible for the rapid conversion of acetaldehyde to acetic acid. ALDH2 (E487K) polymorphism results in an inactive allele (ALDH2*2) which cause dysfunctional acetaldehyde metabolism. The 3D structure of an enzyme is crucial to its functionality and a disruption in its structural integrity could result in its metabolic inefficiency and dysfunctionality. Allosteric targeting of polymorphs could facilitate the restoration of wildtype functionalities in ALDH2 polymorphs and serve as an advancement in the treatment of associated diseases. Therefore, structural insights into ALDH2*2 polymorph could reveal the varying degree of alterations which occur at its critical domains and accounts for enzymatic dysfunctionality. In this study, we report the structural characterization of ALDH2*2 polymorph and its critical domains using computational tools. Our findings revealed that the polymorph exhibited significant alterations in stability and flexibility at the catalytic and co-enzyme-binding domain. Moreover, there was an increase in the solvent-exposed surface residues and this indicates structural perturbations. Analysis of the interaction network at ALDH2*2 catalytic domain revealed residual displacement and interaction loss when compared to the wildtype thereby providing insight into the catalytic inefficiency of the polymorph. Interestingly, perturbations induced by ALDH2 polymorphism involves the re-orientation of surface residues, which resulted in the formation of surface exposed pockets. These identified pockets could be potential sites for allosteric targeting. The findings from this study will aid the design of novel site-specific small molecule reactivators with the propensity of restoring wildtype activities for treatment of polymorphic ALDH2 related diseases.
Subject(s)
Aldehyde Dehydrogenase, Mitochondrial/chemistry , Ethanol/metabolism , Aldehyde Dehydrogenase, Mitochondrial/genetics , Alleles , Allosteric Site , Enzyme Activation , Enzyme Reactivators/chemistry , Humans , Molecular Dynamics Simulation , Polymorphism, Genetic , Protein Conformation , Structure-Activity Relationship , Surface PropertiesABSTRACT
Adenosylcobalamin-dependent diol and glycerol dehydratases are isofunctional enzymes and undergo mechanism-based inactivation by a physiological substrate glycerol during catalysis. Inactivated holoenzymes are reactivated by their own reactivating factors that mediate the ATP-dependent exchange of an enzyme-bound, damaged cofactor for free adenosylcobalamin through intermediary formation of apoenzyme. The reactivation takes place in two steps: (a) ADP-dependent cobalamin release and (b) ATP-dependent dissociation of the resulting apoenzyme-reactivating factor complexes. The in vitro experiments with purified proteins indicated that diol dehydratase-reactivating factor (DDR) cross-reactivates the inactivated glycerol dehydratase, whereas glycerol dehydratase-reactivating factor (GDR) did not cross-reactivate the inactivated diol dehydratase. We investigated the molecular basis of their specificities in vitro by using purified preparations of cognate and noncognate enzymes and reactivating factors. DDR mediated the exchange of glycerol dehydratase-bound cyanocobalamin for free adeninylpentylcobalamin, whereas GDR cannot mediate the exchange of diol dehydratase-bound cyanocobalamin for free adeninylpentylcobalamin. As judged by denaturing PAGE, the glycerol dehydratase-DDR complex was cross-formed, although the diol dehydratase-GDR complex was not formed. There were no specificities of reactivating factors in the ATP-dependent dissociation of enzyme-reactivating factor complexes. Thus, it is very likely that the specificities of reactivating factors are determined by the capability of reactivating factors to form complexes with apoenzymes. A modeling study based on the crystal structures of enzymes and reactivating factors also suggested why DDR cross-forms a complex with glycerol dehydratase, and why GDR does not cross-form a complex with diol dehydratase.
Subject(s)
Bacterial Proteins/chemistry , Cobamides/chemistry , Enzyme Reactivators/chemistry , Hydro-Lyases/chemistry , Propanediol Dehydratase/chemistry , Adenosine Triphosphate/pharmacology , Apoenzymes/antagonists & inhibitors , Bacterial Proteins/metabolism , Cobamides/metabolism , Crystallography, X-Ray , Enzyme Reactivators/metabolism , Hydro-Lyases/metabolism , Klebsiella pneumoniae/enzymology , Propanediol Dehydratase/metabolism , Time Factors , Vitamin B 12/chemistry , Vitamin B 12/metabolismABSTRACT
Oximes (especially oximate anions) are used as potential reactivators of OP-inhibited AChE due to their unique alpha-effect nucleophilic reactivity. In the present study, by applying the DFT approach at the B3LYP/6-311G(d,p) level and the Møller-Plesset perturbation theory at the MP2/6-311G(d,p) level, the formoximate-induced reactivation patterns of the sarin-AChE adduct and the corresponding reaction mechanism have been investigated. The potential energy surface along the pathway of the reactivation reaction of sarin-inhibited AChE by oxime reveals that the reaction can occur quickly due to the relatively low energy barriers. A two-step process is a major pathway proposed for the studied reactivation reaction. Through the nucleophilic attack, the oximate first binds to the sarin-AChE adduct to form a relatively stable phosphorus complex. The regeneration of the serine takes place subsequently through an elimination step, which is expected to be competitive with the nucleophilic attacking process. The polarizable continuum model (PCM) has been applied to evaluate the solvate effects on the pathway. It is concluded that the reaction energy barriers are also low enough for the reaction to easily occur in solvent. The results derived from both the gas-phase model and the aqueous solvation model suggest that the studied oximate anion is an efficient antidote reagent for sarin-inhibited AChE.
Subject(s)
Acetylcholinesterase/chemistry , Chemistry, Physical/methods , Oximes/chemistry , Sarin/pharmacology , Anions , Biophysics/methods , Enzyme Activation , Enzyme Reactivators/chemistry , Kinetics , Models, Chemical , Models, Molecular , Models, Theoretical , Solvents/chemistry , Temperature , ThermodynamicsABSTRACT
A search for co-ordinated amino acid changes in the hsp60 family of chaperonins suggested that cysteine residues at positions 137 and 518 in the Escherichia coli chaperonin GroEL may interact with each other. In order to determine whether this interaction indeed exists we constructed a double-mutant cycle comprising wild-type GroEL, the single mutants Cys137-->Ser and Cys518-->Ser and the corresponding double mutant. The effects of the two mutations on the function of GroEL, in assisting the refolding of a non-folded protein substrate (rhodanese), are shown to be non-additive. It is also shown that ADP by itself specifically destabilizes the Cys518-->Ser mutant GroEL particle with this effect being suppressed in the double mutant. The observed pattern of co-ordinated mutations in the hsp60 family of chaperonins is thus shown to reflect a real interaction, though most likely indirect, between Cys137 and Cys518 in GroEL. Our study demonstrates that patterns of co-ordinated mutations combined with double-mutant cycle analysis can provide structural information on interactions in a protein without an available three-dimensional structure at atomic resolution.
Subject(s)
Bacterial Proteins/chemistry , Heat-Shock Proteins/chemistry , Bacterial Proteins/genetics , Bacterial Proteins/physiology , Base Sequence , Chaperonin 60 , Cysteine , Enzyme Reactivators/chemistry , Heat-Shock Proteins/genetics , Heat-Shock Proteins/physiology , Molecular Sequence Data , Mutagenesis, Site-Directed , Protein Conformation , Structure-Activity Relationship , Thiosulfate Sulfurtransferase/metabolismABSTRACT
It is now well established that alpha-cyclodextrin (alpha-CD) is a valuable folding agent in refolding processes of several denatured enzyme solutions. The refolding of Gu-HCl denatured alpha-amylase in the dilution-additive mode revealed that alpha-CD enhanced the refolding yield by 20-30% depending upon alpha-CD concentration. However, the refolding efficiency of the Gu-HCl denatured alpha-amylase through the artificial chaperone-assisted method indicated that alpha-CD enhanced the activity recovery of denatured alpha-amylase by almost 50% and also increased the reactivation rate constant relative to the unassisted control sample. The higher refolding efficiency should be due to different mechanism played by alpha-CD in this technique. In addition, our data indicated that higher refolding yields are obtained when the residual Gu-HCl concentration is low in the refolding environment and when the capture agent is removed not in a stepwise manner from the protein-detergent complexes in the stripping step of the whole process. Collectively, the results of this investigation expand the range of procedural variations used to refold different denatured proteins through artificial chaperone-assisted method.
Subject(s)
Molecular Chaperones/chemistry , Protein Folding , alpha-Amylases/chemistry , alpha-Cyclodextrins/chemistry , Cetrimonium , Cetrimonium Compounds/chemistry , Circular Dichroism , Detergents , Enzyme Reactivators/chemistry , Guanidine/chemistry , Kinetics , Protein DenaturationABSTRACT
Certain proteins utilize the high reactivity of radicals for catalysing chemically challenging reactions. These proteins contain or form a radical and therefore named 'radical enzymes'. Radicals are introduced by enzymes themselves or by (re)activating proteins called (re)activases. The X-ray structures of radical enzymes and their (re)activases revealed some structural features of these molecular apparatuses which solved common enigmas of radical enzymesi.e. how the enzymes form or introduce radicals at the active sites, how they use the high reactivity of radicals for catalysis, how they suppress undesired side reactions of highly reactive radicals and how they are (re)activated when inactivated by extinction of radicals. This review highlights molecular architectures of radical B12 enzymes, radical SAM enzymes, tyrosyl radical enzymes, glycyl radical enzymes and their (re)activating proteins that support their functions. For generalization, comparisons of the recently reported structures of radical enzymes with those of canonical radical enzymes are summarized here.
Subject(s)
Enzyme Activators/metabolism , Enzyme Reactivators/metabolism , Enzymes/metabolism , Free Radicals/chemistry , Models, Molecular , Animals , Biocatalysis , Catalytic Domain , Enzyme Activators/chemistry , Enzyme Reactivators/chemistry , Enzymes/chemistry , Humans , Protein ConformationABSTRACT
The aim of the present study was to develop a novel strategy to deliver intracellularly the peptide GSE24.2 for the treatment of Dyskeratosis congenita (DC) and other defective telomerase disorders. For this purpose, biodegradable polymeric nanoparticles using poly(lactic-co-glycolic acid) (PLGA NPs) or poly(lactic-co-glycolic acid)-poly ethylene glycol (PLGA-PEG NPs) attached to either polycations or cell-penetrating peptides (CPPs) were prepared in order to increase their cellular uptake. The particles exhibited an adequate size and zeta potential, with good peptide loading and a biphasic pattern obtained in the in vitro release assay, showing an initial burst release and a later sustained release. GSE24.2 structural integrity after encapsulation was assessed using SDS-PAGE, revealing an unaltered peptide after the NPs elaboration. According to the cytotoxicity results, cell viability was not affected by uncoated polymeric NPs, but the incorporation of surface modifiers slightly decreased the viability of cells. The intracellular uptake exhibited a remarkable improvement of the internalization, when the NPs were conjugated to the CPPs. Finally, the bioactivity, addressed by measuring DNA damage rescue and telomerase reactivation, showed that some formulations had the lowest cytotoxicity and highest biological activity. These results proved that GSE24.2-loaded NPs could be delivered to cells, and therefore, become an effective approach for the treatment of DC and other defective telomerase syndromes.
Subject(s)
Biocompatible Materials/chemistry , Cell Cycle Proteins/chemistry , Drug Delivery Systems , Enzyme Reactivators/chemistry , Nanoparticles/chemistry , Nuclear Proteins/chemistry , Peptide Fragments/chemistry , Animals , Biocompatible Materials/adverse effects , Biological Transport , Cell Cycle Proteins/administration & dosage , Cell Cycle Proteins/adverse effects , Cell Cycle Proteins/genetics , Cell Line , Cell Survival/drug effects , Cell-Penetrating Peptides/adverse effects , Cell-Penetrating Peptides/chemistry , Cells, Cultured , Chemical Phenomena , Delayed-Action Preparations/administration & dosage , Delayed-Action Preparations/adverse effects , Delayed-Action Preparations/chemistry , Delayed-Action Preparations/therapeutic use , Drug Compounding , Drug Delivery Systems/adverse effects , Drug Liberation , Drug Stability , Dyskeratosis Congenita/drug therapy , Enzyme Reactivators/administration & dosage , Enzyme Reactivators/adverse effects , Enzyme Reactivators/therapeutic use , Humans , Lactic Acid/adverse effects , Lactic Acid/chemistry , Mice , Nanoparticles/adverse effects , Nuclear Proteins/administration & dosage , Nuclear Proteins/adverse effects , Nuclear Proteins/genetics , Peptide Fragments/administration & dosage , Peptide Fragments/adverse effects , Peptide Fragments/genetics , Polyamines/adverse effects , Polyamines/chemistry , Polyelectrolytes , Polyethylene Glycols/adverse effects , Polyethylene Glycols/chemistry , Polyglactin 910/adverse effects , Polyglactin 910/chemistry , Polyglycolic Acid/adverse effects , Polyglycolic Acid/chemistry , Polylactic Acid-Polyglycolic Acid Copolymer , Protein Stability , Recombinant Proteins/administration & dosage , Recombinant Proteins/adverse effects , Recombinant Proteins/chemistry , Recombinant Proteins/therapeutic useABSTRACT
Although, several studies have been reported on the effects of oxidants on the structure and function of other molecular chaperones, no reports have been made so far for the chaperonin GroEL. The ability of GroEL to function under oxidative stress was investigated in this report by monitoring the effects of hydrogen peroxide (H(2)O(2)) on the structure and refolding activity of this protein. Using fluorescence spectroscopy and light scattering, we observed that GroEL showed increases in exposed hydrophobic sites and changes in tertiary and quaternary structure. Differential sedimentation, gel electrophoresis, and circular dichroism showed that H(2)O(2) treated GroEL underwent irreversible dissociation into monomers with partial loss of secondary structure. Relative to other proteins, GroEL was found to be highly resistant to oxidative damage. Interestingly, GroEL monomers produced under these conditions can facilitate the reactivation of H(2)O(2)-inactivated rhodanese but not urea-denatured rhodanese. Recovery of approximately 84% active rhodanese was obtained with either native or oxidized GroEL in the absence of GroES or ATP. In comparison, urea-denatured GroEL, BSA and the refolding mixture in the absence of proteins resulted in the recovery of 72, 50, and 49% rhodanese activity, respectively. Previous studies have shown that GroEL monomers can reactivate rhodanese. Here, we show that oxidized monomeric GroEL can reactivate oxidized rhodanese suggesting that GroEL retains the ability to protect proteins during oxidative stress.
Subject(s)
Chaperonin 60/chemistry , Enzyme Reactivators/chemistry , Hydrogen Peroxide/pharmacology , Protein Structure, Secondary/drug effects , Thiosulfate Sulfurtransferase/antagonists & inhibitors , Dose-Response Relationship, Drug , Electrophoresis, Polyacrylamide Gel , Oxidation-Reduction , Protein Folding , Recombinant Proteins/chemistry , Scattering, Radiation , Spectrometry, Fluorescence , Surface Properties/drug effects , Thiosulfate Sulfurtransferase/metabolism , UreaABSTRACT
Approximately 50% of men aged over 40 suffer from male erectile dysfunction. Treatment options have widened since the launch of the phosphodiesterase type 5 (PDE5) inhibitor, sildenafil citrate (Viagra trade mark ). However, a certain portion of the patient population, such as diabetics, do not gain significant benefit from PDE5 inhibitors, possibly due to a lack of endogenous nitric oxide. Therefore, new treatment modalities based on the absence of endogenous nitric oxide have been developed. Among them are Rho-kinase inhibitors, soluble guanylate cyclase activators and nitric oxide-releasing PDE5 inhibitors. The available data concerning these compounds will be summarised and their therapeutic potential for male erectile dysfunction will be discussed.
Subject(s)
3',5'-Cyclic-GMP Phosphodiesterases/antagonists & inhibitors , Enzyme Inhibitors/pharmacology , Enzyme Reactivators/pharmacology , Erectile Dysfunction/drug therapy , Erectile Dysfunction/enzymology , Guanylate Cyclase/metabolism , Nitric Oxide/metabolism , Protein Serine-Threonine Kinases/antagonists & inhibitors , 3',5'-Cyclic-GMP Phosphodiesterases/metabolism , Animals , Cyclic Nucleotide Phosphodiesterases, Type 5 , Enzyme Inhibitors/chemistry , Enzyme Inhibitors/therapeutic use , Enzyme Reactivators/chemistry , Enzyme Reactivators/therapeutic use , Humans , Intracellular Signaling Peptides and Proteins , Male , Phosphodiesterase Inhibitors/chemistry , Phosphodiesterase Inhibitors/pharmacology , Phosphodiesterase Inhibitors/therapeutic use , Protein Serine-Threonine Kinases/metabolism , rho-Associated KinasesABSTRACT
The potential of using immobilized Heat Shock Protein 70 (HSP 70) in combination with other molecular chaperones to ameliorate problems of enzyme denaturation was investigated. Firefly luciferase was used as a model enzyme due to its sensitivity to thermal denaturation, and the availability of a sensitive chemiluminescent assay method for determination of relative activity of this enzyme. Control experiments and development of effective combinations of HSP with other chaperones involved re-activation of enzyme in bulk solution. A combination of HSP 70, alpha-crystallin and reticulocyte lysate (RL) in bulk solution were found to re-activate soluble firefly luciferase to about 60% of the initial activity after the enzyme activity had been reduced to less than 2% by thermal denaturation. HSP 70 that was covalently immobilized onto glass surfaces was also able to re-activate denatured enzyme that was in bulk solution. Over 30% of the initial activity could be regained from heat denatured enzyme when using immobilized HSP in the presence of other chaperones. The activity of soluble enzyme decayed to negligible values in a period of days when stored at room temperature. In the presence of immobilized HSP and chaperones, activity stabilized at about 10% of the initial activity even after many weeks. The results suggest that immobilized molecular chaperones such as HSP 70 may provide some potential for stabilization and re-activation of enzymes that are trapped in thin aqueous films for applications in biosensors and reactors.
Subject(s)
Enzyme Reactivators/chemistry , Heat-Shock Proteins/chemistry , Luciferases/chemistry , Molecular Chaperones/chemistry , Animals , Coleoptera/chemistry , Enzyme Stability , Enzymes, Immobilized , HSP70 Heat-Shock Proteins/chemistry , Hot Temperature , Humans , Protein Denaturation , Rabbits , Reticulocytes/chemistry , Spectrometry, Fluorescence , alpha-Crystallins/chemistryABSTRACT
A biosensor for detection of formate at submicromolar concentrations has been developed by co-immobilizing formate dehydrogenase (FDH, E.C. 1.2.1.2), salicylate hydroxylase (SHL, E.C. 1.14.13.1) and NAD(+) linked to polyethylene glycol (PEG-NAD(+)) in a poly(vinyl alcohol) (PVA) matrix in front of a Clark-electrode. The principle of the bi-enzyme scheme is as follows: formate dehydrogenase converts formate into carbon dioxide using PEG-NAD(+). Corresponding PEG-NADH produced is then oxidized to PEG-NAD(+) by salicylate hydroxylase using sodium salicylate and oxygen. The oxygen consumption is monitored with the Clark-electrode. The advantages of this biosensor approach are the effective re-oxidation of PEG-NADH, and the entrapment of PEG-NAD(+) resulting in avoiding the addition of expensive cofactor to the working medium for each measurement. This bi-enzyme sensor has achieved a linear range of 1-300 microM and a detection limit of 1.98 x 10(-7) M for formate (S/N=3), with the response time of 4 min. The working stability is limited to 7 days due to the inactivation of the enzymes. Only sodium salicylate was needed in milli-molar amounts.
Subject(s)
Biosensing Techniques/instrumentation , Electrochemistry/instrumentation , Formate Dehydrogenases/chemistry , Formates/analysis , Microchemistry/instrumentation , Mixed Function Oxygenases/chemistry , NAD/chemistry , Biosensing Techniques/methods , Coenzymes/chemistry , Electrochemistry/methods , Enzyme Reactivators/chemistry , Enzyme Stability , Enzymes, Immobilized/chemistry , Equipment Design , Equipment Failure Analysis , Equipment Reuse , Feasibility Studies , Formates/chemistry , Microchemistry/methods , Multienzyme Complexes/chemistry , Reproducibility of Results , Sensitivity and SpecificityABSTRACT
The isomerization of non-native disulfide bonds often limits the rate of protein folding. Small-molecule dithiols can catalyze this process. Here, a symmetric trithiol, tris(2-mercaptoacetamidoethyl)amine, is designed on the basis of criteria known to be important for efficient catalysis of oxidative protein folding. The trithiol is synthesized and attached to two distinct solid supports via one of its three sulfhydryl groups. The resulting immobilized dithiol has an apparent disulfide E degrees ' = -208 mV, which is close to that of protein disulfide isomerase (E degrees ' = -180 mV). Incubation of the dithiol immobilized on a TentaGel resin with a protein containing non-native disulfide bonds produced only a 2-fold increase in native protein. This dithiol appeared to be inaccessible to protein. In contrast, incubation of the dithiol immobilized on styrene-glycidyl methacrylate microspheres with the non-native protein produced a 17-fold increase in native protein. This increase was 1.5-fold greater than that of a monothiol immobilized on the microspheres. Thus, the choice of both the solid support and thiol can affect catalysis of protein folding. The use of dithiol-decorated microspheres is an effective new strategy for preparative protein folding in vitro.