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Unequal Efficacy of Pyridinium Oximes in Acute Organophosphate Poisoning

Biljana Antonijevic, Institute of Toxicological Chemistry, Faculty of Pharmacy, University of Belgrade, Vojvode Stepe 450, 11221 Belgrade, Serbia
Milos P. Stojiljkovic, Department of Biochemistry, Pharmacology & Genetics, Odense University Hospital, University of Southern Denmark, Winsløwparken 19, DK-5000 Odense, Denmark

Reprint Requests: Biljana Antonijevic, Institute of Toxicological Chemistry, Faculty of Pharmacy, University of Belgrade, Vojvode Stepe 450, 11221 Belgrade, Serbia, Tel: 381-11-3970389/ext 650, Fax: 381-11-3972840, Email: abiljana{at}pharmacy.bg.ac.yu

Received: May 12, 2006.

Revised: July 28, 2006.

Accepted: October 10, 2006.

	Abstract

TOP Abstract Historical Overview Toxicological Relevance Mechanism of Action of... Treatment of Organophosphate... Conclusion References

 
The use of organophosphorus pesticides results in toxicity risk to non-target organisms. Organophosphorus compounds share a common mode of action, exerting their toxic effects primarily via acetylcholinesterase (AChE) inhibition. Consequently, acetylcholine accumulates in the synaptic clefts of muscles and nerves, leading to overstimulation of cholinergic receptors. Acute cholinergic crisis immediately follows exposure to organophosphate and includes signs and symptoms resulting from hyperstimulation of central and peripheral muscarinic and nicotinic receptors. The current view of the treatment of organophosphate poisoning includes three strategies, i.e. the use of an anticholinergic drug (e.g., atropine), cholinesterase-reactivating agents (e.g., oximes) and anticonvulsant drugs (e.g., benzodiazepines). Oximes, as a part of antidotal therapy, ensure the recovery of phosphylated enzymes via a process denoted as reactivation of inhibited AChE. However, both experimental results and clinical findings have demonstrated that different oximes are not equally effective against poisonings caused by structurally different organophosphorus compounds. Therefore, antidotal characteristics of conventionally used oximes can be evaluated regarding how close the certain substance is to the theoretical concept of the universal oxime. Pralidoxime (PAM-2), trimedoxime (TMB-4), obidoxime (LüH-6), HI-6 and HLö-7 have all been demonstrated to be very effective in experimental poisonings with sarin and VX. TMB-4 and LüH-6 may reactivate tabun-inhibited AChE, whereas HI-6 possesses the ability to reactivate the soman-inhibited enzyme. An oxime HLö-7 seems to be an efficient reactivator of AChE inhibited by any of the four organophosphorus warfare agents. According to the available literature, the oximes LüH-6 and TMB-4, although relatively toxic, are the most potent to induce reactivation of AChE inhibited by the majority of organophosphorus pesticides. Since there are no reports of controlled clinical trials on the use of TMB-4 in human organophosphate pesticide poisoning, LüH-6 may be a better option.

Key Words: Antidotal therapy • Efficacy • Organophosphates • Organophosphorus insecticides • Oximes • Reactivation

Highly toxic organophosphorus compounds (OPCs) are widely used for pest control and for the control of vector-borne diseases. These compounds also include the nerve poisons that are among the most toxic group of chemical warfare agents. Toxicology of organophosphates, as well as the therapeutic approaches in acute organophosphate poisoning, is of importance to many different groups of health professionals. The management of OPC poisoning is complex and includes nonspecific and specific measures. The dominant underlying toxicodynamic mechanism in organophosphate poisoning is inhibition of acetylcholinesterase (AChE). Oximes, as cholinesterase reactivators, are the only causal antidotes used against OPCs. Unfortunately, there are no known oximes that are efficient reactivators of cholinesterase inhibited by any of the known OPCs. Moreover, controlled clinical studies proving the efficacy of oximes in humans are mostly lacking.

	Historical Overview

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The first synthesis of an OPC was performed in the middle of the 19th century by Moschnine in Professor Wurtz’s laboratory in Paris. The first OPC ever synthesized was tetraethylpyrophosphate and the process was first published in 1854 by de Clermont. However, von Hofmann was the first scientist to synthesize an OPC with direct phosphorus-carbon linkage (methylphosphoryl dichloride) in 1873. In the next century, Lange and von Krueger synthesized dialkylphosphonofluoridates, obtaining many OPCs with insecticidal or fungicidal properties. Between 1934 and 1944 Schrader’s team synthesized approximately 2000 OPCs and in 1944 two well-known organophosphorus insecticides, diethyl-p-nitrophenylphosphate (paraoxon, E600) and diethyl-p-nitrophenylthiophosphate (parathion, E605), were synthesized. As early as 1935, the Nazi Germany government insisted on redefining Schrader’s primal aim from organophosphorus insecticides to organophosphorus chemical warfare agents (e.g., tabun, sarin, soman). In a series of fluorine-containing esters, besides sarin and soman, Schrader also developed diisopropyl phosphorofluoridate (DFP). Also during this same period, British and American scientists were evaluating the toxic properties of DFP and other alkyl phosphorofluoridates. Although initially designed as a potential chemical warfare agent, DFP became a model substance widely used throughout the pharmacological community for studying cholinergic neurotransmission. The fourth chemical warfare agent, VX, was synthesized a decade later in 1957 by Tammelin.¹

During the same period, Russian scientists developed the so-called Russian VX (VR). Another structural analog of VX, known as Chinese VX (CVX), was also developed. Kuca and co-workers² showed that the VX agent was half-fold more toxic in comparison with VR with in vitro experiments using rat, pig and human brain homogenate. However, examination of reactivity towards human and pig AChE demonstrated the following rank order of inhibitory potency: VR>CVX>VX.³ Structural formulae of some organophosphorus chemical warfare agents are given in figure 1.

View larger version (10K): [in this window] [in a new window]   Figure 1. Structural formulas for organophosphorus chemical warfare agents.

After World War II, OPCs were reintroduced worldwide for pesticide use, as originally intended. In the decades since, numerous structurally different OPCs have been synthesized. Currently more than 100 different OPCs are used mainly as insecticides in agriculture and gardening.^5–7

	Toxicological Relevance

TOP Abstract Historical Overview Toxicological Relevance Mechanism of Action of... Treatment of Organophosphate... Conclusion References

 
In industrialized countries, severe intoxication of OPCs generally results from oral intake, whereas inhalation or dermal absorption does not play a major role. In developing countries, the most common cause of pesticide poisonings is due to occupational exposure. However, a review of poisoning studies in developing countries reveals that pesticide poisonings associated with high mortality rates are usually the result of self-poisoning. Particularly, a great number of victims was present in rural regions due to the widespread availability of acutely toxic pesticides used in agriculture.^8,9 Organophosphorus pesticides cause several hundreds of thousands of victims per year worldwide.⁶ While some of these intoxications may be attributed to accidental exposure, the majority of casualties result from suicidal attempts with ingestion of multiple lethal doses. Therefore, the indiscriminate use of these pesticides results in a toxicity risk to non-target organisms and environmental pollution.

Due to their high toxicity, OPCs bear a potential risk for use in war conflicts and terrorist attacks. Namely, the repeated use of nerve agents during the Iran–Iraq war in the 1980s,¹⁰ against civilians by Iraqi troops,¹¹ and during terrorist attacks by the Aum Shinrikyo sect in Japan^12–15 emphasize the constant threat and need for increased awareness of the potential for future homicidal attempts, as well as the urgent need for the development of an effective medical treatment regimen.^16,17

The mechanism of action of OPCs, as well as factors contributing to toxic response, will be briefly discussed in this paper. Treatment of acute poisoning caused by this class of substances will be considered through a correlation of experimental data and clinical findings, with special attention to oxime efficacy against chemically different cholinesterase inhibitors.

	Mechanism of Action of OPCs

TOP Abstract Historical Overview Toxicological Relevance Mechanism of Action of... Treatment of Organophosphate... Conclusion References

 
The basic chemical structure of all OPCs is described by Schrader’s formula (figure 2).¹⁸ The structural diversity of OPCs is due to different substituents at the phosphorus atom. Substituents at R1 and R2 are alkyl, alkoxy, alkylthio or amino groups, and substituent at X is a labile acyl residue (halide, cyano, phenol or thio group), known as the leaving group.

View larger version (6K): [in this window] [in a new window]   Figure 2. Schrader’s formula for organophosphorus compounds.

Inhibition of BuChE, whose physiological role is still unclear, can be ascertained by clinical laboratory procedures and will confirm the clinical diagnosis. Even more, BuChE has been recognized as a bioscavenger of OPCs, thereby decreasing the organophosphate concentration in the organism.²⁶ Namely, among the enzymes examined as potential scavengers of OPCs, significant advances have been made by using AChE and BuChE.^27–29 Human serum BuChE is proposed as an exogenously administered prophylactic for human use³⁰ due to the following facts: it reacts rapidly with all highly toxic OPCs, offering a broad range of protection for nerve agents including soman, sarin, tabun and VX; it possesses a very long retention time in human circulation and is readily absorbed from sites of injection; the enzyme is from a human source and should not produce any adverse immunological responses upon repeated administration to humans.³¹ However, the production of native human BuChE requires large amounts of plasma leading to the development of technologies to produce recombinant human BuChE.³²

Despite the fact that both AChE and BuChE serve as diagnostic tools, after the exposure resulting in inhibition levels <20% with no clinical signs and symptoms of organophosphate poisoning, it is necessary to bear in mind the uncertainty due to marked inter-individual variations of AChE and BuChE activities and to intra-individual variation of BuChE activities.^16,33 Another factor complicating the interpretation of erythrocyte AChE activity is that inhibition of this enzyme probably overestimates the inhibition of AChE in the nervous system.³³ Namely, in the case of an irreversible inhibition, recovery of erythrocyte AChE depends on de novo production and release from the bone marrow of new erythrocytes with uninhibited AChE. The recovery rate of erythrocyte AChE has been estimated to be 1%, whereas the half-life of AChE resynthesis in the nervous system has been reported to be 5 to 7 days. Therefore, AChE in brain will recover earlier than in red blood cells.

Molecular Mechanisms of Organophosphate Toxicity
OPCs and their active metabolites are electrophilic molecules with moderate to high potency for phosphylation (denotes both phosphorylation and phosphonylation) of the serine hydroxyl group located at the active site of AChE. This phosphylation occurs by the loss of the leaving group and the establishment of a covalent bond with AChE through the serine hydroxyl. The resultant phosphylated AChE is typically very stable and is only slowly regenerated by spontaneous hydrolysis of the phosphate ester. While the AChE remains phosphylated, its enzyme activity is inhibited and therefore ACh accumulates in the synaptic clefts of muscles and nerves, leading to overstimulation of cholinergic receptors that is essentially "poisoning by endogenous ACh."

Additionally, OPCs may also interact (inhibit) with other serine esterases,^34,35 may have a direct action on muscarinic and nicotinic receptors binding to (with high/low affinity) and modulating the function of these receptors,³⁶ and may induce specific organ lesions.³⁷ Propyl, isopropyl, butyl, and higher alkyl phosphates and phosphonates are more likely than methyl or ethyl analogs to act with secondary targets.³⁵ The concentrations of OPCs required to act directly on nicotinic receptors are much higher than those on muscarinic receptors, suggesting that muscarinic receptors are more important as secondary targets in OPC action. Combination of possible interactions will produce resultant toxic effect(s) for the particular OPC. The spectrum of effects is further modulated by various toxicokinetic factors.³⁸

In phase I of biotransformation, metabolic transformation of OPCs occurs through six major reactions, most of which are activation pathways: (1) oxidative desulfurations (conversion of thiophosphate to the more toxic oxon form, e.g., parathion, malathion, fenitrothion, diazinon, dimethoate, azinphosmethyl, fonofos), (2) oxidative N-dealkylation (e.g., dicrotophos, monocrotophos, dimethoate, phosphamidon), (3) oxidative O-dealkylation (e.g., chlorfenvinphos), (4) thioether oxidation (e.g., disulfoton, phorate, fenthion, demethon-S-methyl), (5) side chain oxidation (e.g., fenitrothion, diazinon), and (6) various nonoxidative reactions (e.g., trichlorfon, naled). In phase II of biotransformation, which is by definition, the detoxification phase, OPCs undergo conjugation with endogenous substrates, such as glucuronides and sulfates. Organophosphates are detoxified by the action of carboxylesterases (CarbE) (e.g., malathion, fentoate, soman, sarin, tabun), phosphorylphosphatases (e.g., pyrimiphos methyl, diazinon, paraoxon, DFP, soman, sarin, tabun) and glutathione redox system (e.g., methyl parathion, methyl paraoxon, fenitrothion, diazinon, dichlorvos, bromophos, chlorfenvinphos, mevinphos), but are activated by the cytochrome P450 system, NADPH-cytochrome P450 reductase and flavin-containing monooxygenases.³⁹

CarbE plays an important role in the detoxification of OPCs via hydrolysis of ester bonds in OPCs (carboxyl ester side chain), as well as binding OPCs at the active site of CarbE that reduces the free concentration of the OPC potentially available to inhibit AChE.⁴⁰ Differences in CarbE levels contribute to species differences in the toxicity of OPCs among mammals.

The most common pathway for the metabolism of OPCs is via hydrolysis, which results in removal of the more labile leaving group. Products of such hydrolysis are excreted in urine and are biomarkers of exposure. These include dimethylphosphate, dimethylthiophosphate, dimethyldithiophosphate, dimethylphosphorothioate, diethyl-phosphate, diethylthiophosphate, diethyldithiophosphate and diethylphosphorothioate. Because insecticidal OPCs differ mostly in the structure of the leaving group, the rates of hydrolysis will differ from compound to compound, despite similarity in some of the resulting urinary metabolites.⁴¹ The enzymes (phosphorylphosphatases) involved in hydrolysis of OPCs, and therefore inactivation, are present in many tissues and have high activities in liver, intestine and plasma.

Whether activation or detoxification will be a dominant reaction largely depends on the chemical structure of the OPC and its interaction with enzyme systems. Toxicity depends on the relative prevalence and intensity of these competing metabolic pathways. Chemicals that provoke induction of the enzymes involved in activation of OPCs can make them more toxic, as well as the chemicals that inhibit enzymes included in the detoxification phase and vice versa.^40,42–44 However, clinical impact of interactions due to inhibition/induction of enzymes involved in detoxification or activation is difficult to predict because they often produce effects on several enzyme systems.

Critical Toxic Effects
Exposure to OPCs can induce four different clinical syndromes: (1) acute cholinergic crisis as a result of AChE inhibition, (2) intermediate syndrome whose underlying mechanism(s) is still unclear, (3) organophosphate-induced delayed neuropathy that has been explained by the inhibition of neuropathy target esterase, and (4) chronic organophosphate induced neuropsychiatric disorder due to long-term low-level exposure.

Acute cholinergic crisis immediately follows exposure to OPC and includes signs and symptoms resulting from hyperstimulation of muscarinic receptors (e.g., bradycardia, bronchoconstriction, bronchorrhoea, hypotension, increased gastrointestinal motility, abdominal cramps, miosis, hypersalivation), nicotinic receptors (e.g., hypertension, tachycardia, fibrillation, fasciculation, necrosis of striated muscles), and both central muscarinic and nicotinic receptors (e.g., tremor, movement incoordination, seizures, central depression of respiration, coma, death). If death ensues, it is usually due to asphyxia, i.e., after cessation of respiration followed by hypoxaemia and cyanosis. The so-called lung muscarinic syndrome (laryngospasm, bronchoconstriction and bronchorrhoea) and a depolarization paralysis of the respiratory muscles also contribute to the occurrence of asphyxia and death. Although the immediate cause of death could also be cardiac arrest or heart failure, central respiratory failure due to loss of respiratory drive is by far the most frequent cause of death after intoxication with OPCs.⁵

	Treatment of Organophosphate Poisoning

TOP Abstract Historical Overview Toxicological Relevance Mechanism of Action of... Treatment of Organophosphate... Conclusion References

 
The current view of the treatment of OPC poisoning includes three strategies: (1) the use of an anticholinergic drug (e.g., atropine), (2) cholinesterase-reactivating agents (e.g., oximes) and (3) anticonvulsant drugs (e.g., benzodiazepines). The development of treatment against OPC poisoning started with recognition of the efficacy of atropine as an antidote for their parasympathomimetic effects. Atropine, an alkaloid isolated from Atropa belladonna L. by Main in 1835, first successfully used against a cholinesterase-inhibiting agent by Fraser in 1863, has remained the cornerstone of the therapy of OPC intoxication ever since. As far as chemical warfare agents are concerned, Eberhard Gross, after a remark that OPCs could exert their toxic action in a similar manner as carbamates (including physostigmine), suggested the use of atropine in the treatment of OPC poisoning.¹ Experimental work performed after World War II has revealed that atropine affords much less efficient protection against OPCs than against carbamate intoxications, making atropine monotherapy insufficient in severe acute organophosphate poisoning. This is mainly due to the fact that atropine, as an antimuscarinic drug, is not capable of counteracting effects provoked by nicotinic hyperstimulation, while at the same time, possesses only limited antimuscarinic action in the central nervous system (CNS). Also, convulsions can be blocked by atropine only for a very limited time after exposure to OPCs since other transmitter systems have become involved in cholinergic overstimulation in the brain (e.g., -aminobutyric acid, glutamate). Nevertheless, atropine is the initial drug of choice in acute organophosphate poisoning.

The most important anticonvulsant in present use is diazepam.^45,46 The combination of atropine and diazepam is more effective than atropine or oxime alone in reducing mortality.⁴⁷ Basically, the benzodiazepines potentiate the action of the inhibitory neurotransmitter -aminobutyric acid at its receptors.^48–51 In the cholinergic nervous system, diazepam probably decreases the synaptic release of ACh.⁵² The main consequence of the action of benzodiazepines in CNS is hyperpolarization of neurons which makes them significantly less susceptible to cholinergically-induced depolarization. The ultimate result is cessation of propagation of convulsions.⁵³ Diazepam is of benefit in organophosphate poisoned patients by reducing anxiety, restlessness and muscle fasciculations, terminating convulsions, and reducing morbidity and mortality when used in conjunction with atropine and oxime. Diazepam should be given to patients poisoned with OPCs whenever convulsions or pronounced muscle fasciculation are present. In severe poisoning, diazepam administration should be considered even before these complications develop.⁵⁴

Oxime Therapy
The first successful (in vitro) destruction of phosphylated AChE was accomplished by hydroxylamine in 1951.¹ Additionally, in in vitro experiments, hydroxylamine also induced reactivation of AChE inhibited by tetraethylpyrophosphate.⁵⁵ In the following years, development of specific antidotes, originally aimed to regenerate AChE inhibited by nerve agents, has been based on the presumption that successful regeneration of inhibited enzymes could be achieved by the nucleophilic attack of a compound structurally similar to the chemical structure of ACh, meaning a presence of a quaternary ammonia group in a molecule of reactivators. Namely, pralidoxime (PAM-2), the first pyridinium oxime, could reactivate the phosphylated enzyme about a million times faster than hydroxylamine.⁵⁶ By 1956, the scientific public was introduced to the use of the newly synthesized oxime, PAM-2, which was administered against parathion poisoning in Japan.⁵⁷ Further investigations in this area resulted in synthesis of bispyridinium oximes: trimedoxime (TMB-4), obidoxime (LüH-6), HI-6, and HLö-7 (figure 3). These oximes were synthesized and introduced as antidotes in 1957, 1964, 1967 and 1986, respectively.

View larger version (10K): [in this window] [in a new window]   Figure 3. Structural formulas for pyridinium oximes.

Commercially available oximes are PAM-2 salts (e.g., chloride, mesylate, methylsulphate, iodide) and LüH-6 chloride. TMB-4 and HI-6 were in clinical use, however, now these oximes are reserved for military use and are present in auto-injectors of several armies.^71–73 Although there are no data on the clinical use of HLö-7, auto-injectors with this oxime were also developed.⁷⁰

Pyridinium oximes were formulated as different salts (e.g., chloride, iodide, bromide, lactate, methylsulphate, methanesulfonate), which mostly differ in their stability and solubility. Generally, PAM-2, TMB-4 and LüH-6 are stable in aqueous solutions and can be prepared in liquid form in ampules, whereas HI-6 and HLö-7 are not stable in aqueous solutions and therefore can be kept for longer time only as powder that is dissolved immediately before use.^74,75 Consequently, HI-6 and HLö-7 are formulated as dry/wet auto-injectors. Most papers on PAM-2 refer to the chloride or methanesulfonate (mesylate, P2S) salts. These salts replaced the first PAM-2 salt developed, PAM-2 iodide, because of its limited solubility. It was also reported that PAM-2 iodide might induce iodism.⁷⁶ The anionic component of PAM-2, however, does not significantly influence its antidotal properties.⁷⁷

Comparative studies on the two salts of HI-6 (i.e., chloride and methanesulfonate) showed that HI-6 dimethanesulfonate (DMS) is much more soluble and that its absolute water-solubility is two and five times higher at 20°C and 5°C, respectively.⁷⁸ Moreover, comparative studies on reactivation potency, pharmacokinetics and pharmacodynamics have demonstrated that the two HI-6 salts are equipotent in reactivating erythrocyte AChE inhibited by highly toxic OPCs and that the two HI-6 salts have a similar pharmacokinetic profile.^79,80 In the frame of the Chemical Biological Radiological Nuclear Research and Technology Initiative, a project was launched aimed at developing auto-injectors based on HI-6 DMS.⁸¹ In the final stage of the project, preclinical efficacy and toxicology data for jointly administered HI-6 DMS, atropine and avizafone will be obtained that will enable a phase 1 clinical trial to be conducted, thereby determining the safety of the new nerve agent antidote system.

Mechanism of Action of Pyridinium Oximes
Reactivation of inhibited AChE by removal of the phosphyl moiety from the AChE active site serine is considered to be the primary mechanism of action for oximes. Clinical data obtained in organophosphorus pesticide-poisoned patients provide evidence for the validity of this assumption.^82–84

As generally visualized, the oxime is oriented proximally to exert a nucleophilic attack on the phosphorus of the enzyme-inhibitor complex. Intermediate in the reactivation is a complex between the phosphylated enzyme and the reactivator. The enzyme-inhibitor-oxime complex is then split off, leaving the regenerated enzyme. However, phosphylated oximes formed during the reactivation process might be potent inhibitors of cholinesterases, which could cause re-inhibition of the previously reactivated enzyme.⁸⁵ Re-inhibition of AChE can be faster than reactivation in the case when a phosphylated oxime inhibits the enzyme at a rate higher than that of its elimination or decay to non-toxic products.^84,86

Early reports suggested this possibility on the basis of in vitro experiments with LüH-6 and dimethoate,⁸⁷ and LüH-6 and PAM-2 with soman.⁸⁸ Generally, phosphyloxime accumulation may occur in the many reactivation/re-inhibition cycles, particularly with the more stable compounds deriving from 4-pyridinium oximes and may alter the efficacy of the 4-pyridinium oximes.^89–91 It remains doubtful whether this occurs in humans with the usual dose regimens. It was also demonstrated that human paraoxonase with the prevailing Q192 phenotype⁹² is able to hydrolyze effectively O, O-diethylphosphoryl LüH-6.⁹³ This enzyme, however, is apparently unable to inactivate phosphonyl oxime derivatives.⁹⁴

Mechanistic studies of oxime action have also shown that two binding sites are involved, i.e., cholinesterases have two binding sites for reversible ligands: (1) an acylation (catalytic) site at the base of the active site gorge and (2) a peripheral (allosteric) site at its mouth.⁹⁵ Reversible ligands, such as the oximes, may bind to cholinesterases either at the catalytic site or at the allosteric site, or at both sites of the enzymes, thus explaining the mechanism of protection afforded by oxime administration.⁹⁶ Bearing in mind the underlying mechanisms of reactivation and protection, it becomes clear that stereochemical arrangements of oximes can play a role in the difference in their therapeutic efficacy. Finally, so-called direct pharmacological effects such as direct reaction with OPCs, anticholinergic and sympathomimetic effects, as well as some pre-junctional properties that decrease the amount of liberated acetylcholine into the synaptic cleft,^97–101 are also relevant for the interpretation of antidotal potency of oximes.

Regarding the aforementioned mechanism of protection, it is possible to administer oximes before the poisoning occurs, i.e., prophylactically. Oximes, as reversible ligands, protect cholinesterases from phosphylation by OPCs (i.e., oximes slow down the rate of phosphylation).²⁶ Oximes might be able to reactivate the enzyme before a significant amount of aging has time to occur. This approach has been tried by the British who used P2S tablets as a pretreatment.¹⁰² However, short elimination half-lives of the oximes make them inappropriate for pre-treatment.^83,103–105 Another prophylactic approach is a combination of cholinesterase and an oxime pre-treatment that has been explored as a pseudo-catalytic bioscavenger, such that the catalytic activity of inhibited cholinesterase can rapidly and continuously be restored in the presence of an oxime.²⁸

Clinical Use of Oximes
A particular problem in interpreting the beneficial role and efficacy of oximes in clinical practice is a deficiency of published data, especially those evaluated in controlled clinical trials. In this section, in order to illustrate heterogeneity of therapeutic approaches (i.e., dose regimen, oxime choice and final outcome of the treatment) a few studies are presented in chronological order of publication.

Sixty patients acutely poisoned with various organophosphorus insecticides were treated with atropine, diazepam and HI-6 (500 mg every 6 hours intramuscularly) for 2 to 7 days, depending on the severity of the organophosphate poisoning. In addition, in a small series of patients (n=9), PAM-2 was administered instead in 1 g doses every 6 hours over the same period of time. The recovery of erythrocyte AChE was rapid in patients suffering from severe phorate, quinalphos, dichlorvos and pyridafenthion poisonings with reactivation half-lives ranging from 0.5 to 3.5 hours. Malathion-inhibited enzyme was reactivated much more slowly (reactivation half-life=10.1 hours), while HI-6 was ineffective against AChE inhibition caused by dimethoate and phosphoramidon. While nearly 100% reactivation of the enzyme was obtained after only 2 days of HI-6 treatment, PAM-2 could reactivate only 40% of the enzyme activity by the end of the eighth day. No adverse effects were noted in patients treated with oximes.⁸²

Nine patients intoxicated with organophosphorus insecticides were treated with PAM-2 methylsulphate (Contrathion) using a dose of 4.42 mg/kg as a bolus injection followed by continuous infusion 2.14 mg/kg/h.¹⁰⁶ In patients with ethylparathion and methylparathion poisonings, enzyme reactivation could be obtained in some at oxime concentrations as low as 2.88 mg/L. In others, however, oxime concentration as high as 14.6 mg/L were ineffective. The therapeutic effect of the oxime seemed to depend on the plasma concentrations of ethylparathion and methylparathion. Due to enzyme AChE re-inhibition, reactivation was absent as long as these concentrations remained above 30 µg/L.

In a series of five case reports, LüH-6 (Toxogonin) 250 mg was given as an intravenous bolus followed by continuous infusion of 750 mg/24 hours in cases of life-threatening parathion poisoning. This dose was effective, especially when the dose of parathion absorbed was relatively low.⁸³

In a clinical study of 63 patients poisoned with organophosphorus insecticides, patients were divided into three groups: one was treated with atropine only, while the other two received atropine and either PAM-2 or LüH-6. Loading and maintenance intravenous doses for PAM-2 were 30 mg/kg and 8 mg/kg/h, respectively and 8 mg/kg and 2 mg/kg/h, respectively, for LüH-6. There were no statistically significant differences in the major clinical findings or AChE activities on admission among the groups. Although the severity of intoxications (based on respiratory complications and duration of hospitalization) was higher in the atropine plus oxime groups, no mortality was found in the PAM-2 plus atropine group, whereas 12% and 50% of patients in the atropine and atropine plus LüH-6 groups died, respectively. Incidence of recurrent twitching and convulsions, repeated respiratory arrest, required mechanical respiration, required intensive care unit therapy and duration of hospitalization were smaller in the atropine plus LüH-6 group than in the atropine plus PAM-2 group. Three of the patients who received the LüH-6 combination therapy developed hepatitis and two of them died due to liver failure, which may indicate overdosage of LüH-6.¹⁰⁷

The usual therapeutic regimen of LüH-6 is comprised of a 250 mg intravenous (or intramuscular) bolus immediately after the first atropine injection. Then if no recovery is apparent during the next 15 to 30 minutes, an intravenous infusion of 750 mg/24 h is started for as long as necessary. Children can be treated with a 4 mg/kg bolus followed by an infusion with 0.45 mg/kg/h. PAM-2 chloride can be used according to the following scheme: 1 g intravenous bolus followed by up to 0.5 g/h as an infusion. In children, a loading dose of 25 to 50 mg/kg PAM-2 can be used, followed by continuous infusion of 10 to 20 mg/kg/h.¹⁷ Other PAM-2 salts are also on the market (i.e., iodide, methylsulfate and mesylate) and can be used in corresponding doses.

Drawbacks and Limitations of Oxime Therapy
AChE inhibited by OPCs may undergo a secondary reaction, i.e., spontaneous dealkylation through alkyl-oxygen bond scission (aging), resulting in an irreversibly inactivated enzyme. Velocity of aging has a great impact on the treatment procedures and therapeutic efficacy of antidotes because aged enzyme cannot be reactivated by oxime therapy. The aging kinetics depend on the structure of the respective compound. Thus, OPCs leading to dimethylphosphoryl-AChE (e.g., malaoxon) have a much shorter aging half-life (about 4 hours) than compounds resulting in the diethylphosphoryl-enzyme (e.g., paraoxon, diazinon).¹⁰⁸

Oximes are not equally effective and rank order of effectiveness changes with the OPC involved. Even if the same dosage regimen of an oxime is administered, due to interindividual variations, different plasma concentrations will be obtained.¹⁰⁹

Differences in their efficacy will be given not only throughout interactions with organophosphorus insecticides but also via their ability to counteract toxic effects of chemical nerve agents (sarin, soman, tabun, and VX). This approach is due to the permanent intention and effort of the scientific community to develop an oxime with universal antidotal properties, i.e., an oxime that is relatively efficient against all OPCs, including chemical nerve agents.^69,110–113

PAM-2 is very efficient in reactivating AChE inhibited with sarin or VX,^12,114–118 but is inefficient in the reactivation of the tabun-inhibited or soman-inhibited enzyme.^119–121 Experiments have shown that TMB-4 is a powerful reactivator and was the first oxime efficient in the treatment of animals intoxicated with tabun^65,122,123 and also effective against experimental sarin or VX poisoning. However, TMB-4 is totally ineffective against soman,^65,119 and at the same time is the most toxic oxime demonstrated in mice to have a median lethal dose (LD₅₀) of 3, 4 and 8 times less than the ones for LüH-6, PAM-2 and HI-6, respectively.⁹⁷ Oxime LüH-6, recognized as a good AChE reactivator, shares similar antidotal properties with TMB-4. Although potent against tabun, sarin and VX,^119,124 LüH-6 is also ineffective against soman poisoning in mice,⁶⁵ guinea pigs¹¹⁹ and primates.¹²⁵ LüH-6 is somewhat more efficient than TMB-4 as an antidote against tabun intoxication.¹²⁶ Although being less toxic than TMB-4, this oxime shows hepatotoxic potential.^56,127

HI-6 is more potent than LüH-6 in protection of various rodent species from intoxication with soman,^117,119,128 as well as sarin, and especially, VX.⁶⁵ The only drawback of HI-6 is that this oxime cannot reactivate tabun-inhibited AChE.^129,130 The per se toxicity of HI-6 is low, actually the lowest among the aforementioned oximes.^65,97,131

HLö-7 reactivates AChE inhibited by any of the four major nerve agents.^132–134 In addition, HLö-7, more efficiently than PAM-2, LüH-6 and HI-6, restored the neuromuscular transmission impaired by in vitro superfusion of the neuromuscular preparation with tabun, sarin, soman or cyclosarin.¹³⁵ It was found that HLö-7 induced a significant reactivation of AChE in mice diaphragms previously inhibited with tabun, sarin, soman and cyclosarin.¹³⁶ Although both HI-6 and HLö-7 can antagonize sarin-induced hypothermia (thus proving that they can pass the blood-brain barrier and gain access to the CNS when given with atropine),^136,137 the LD₅₀ of HLö-7 is 2.5 times less than that of HI-6, indicating the higher per se toxicity of the newer oxime.¹³⁶ The cardiovascular tolerability of HLö-7 was close, but still not as good as HI-6, at least in anesthetized guinea pigs.¹³⁸ On the scale of efficacy, HLö-7 turned out to be somewhat more effective than HI-6 against tabun and VX poisoning and less effective against sarin and soman, as well as cyclosarin intoxication.^139,140 In guinea pigs, a species considered the closest model to the primate, HLö-7-induced protection against tabun poisoning was significantly better than that of HI-6, while HI-6 was only slightly more efficient than HLö-7 in soman poisoning.¹⁴¹

In cases of intoxications with organophosphorus insecticides, the worst therapeutic results are obtained with HI-6 and HLö-7 and, to some extent, PAM-2, while the most efficient oximes are TMB-4 and LüH-6.^83,142–144 Worek and co-workers^86,143,145 have proved that equimolar concentrations of LüH-6 are more effective than PAM-2, HI-6 and HLö-7 in in vitro reactivation of human erythrocyte AChE inhibited by several organophosphorus insecticides. Also, a 10 µmol/L concentration of LüH-6, ten times less than PAM-2 (100 µmol/L), was necessary to restore the contractility of isolated mouse diaphragm previously treated with paraoxon. Although efficient in patients intoxicated by low parathion doses, LüH-6 failed to antagonize the effects of high parathion doses, probably due to a high re-inhibition rate.⁸³ However, in the same clinical study, LüH-6 was completely ineffective against oxydemethon-methyl intoxication. Unfortunately, there is no published clinical evidence on the use of TMB-4 in patients poisoned by organophosphorus insecticides; therefore, its comparison is impossible.

A clinical study of HI-6 administered intramuscularly at doses up to 500 mg was performed in 22 healthy volunteers and revealed no adverse effects. In patients poisoned by several organophosphorus insecticides, HI-6 ensured fast reactivation of erythrocyte AChE in almost all cases, except in the cases of dimethoate and phosphamidon.^82,103

However, AChE inhibited by several organophosphorus insecticides, including dimethoate, demethon, triamiphos, ethoprophos, profenofos, fenamiphos and pyridafenthion, resists any attempt at reactivation with any oxime, probably due to variations in phosphoryl moiety and distribution of electronic charge.^56,86,142 Finally, a systematic review of two randomized controlled clinical trials did not result in final proof of the efficacy of PAM-2 in the treatment of poisonings induced by organophosphorus insecticides in humans,¹⁴⁶ probably due to the methodological gaps in the trials included, as indicated in the original publication.

	Conclusion

TOP Abstract Historical Overview Toxicological Relevance Mechanism of Action of... Treatment of Organophosphate... Conclusion References

 
There are many factors that influence oxime efficacy. Among them it seems most important to mention the inhibitory potential of OPCs and its toxicokinetics, aging kinetics of inhibited AChE, reactivating property of oximes, and its pharmacokinetics. However, the assessment of oximes effectiveness in patients severely poisoned with organophosphates is hampered by sedation, artificial ventilation and other therapeutic measures, as well as by varying individual clinical courses due to differences in type and amount of poison ingested or time elapsed before treatment starts. Substantial species differences hamper the extrapolation of experimental data to humans. Furthermore, frequently high and unrealistic doses/concentrations of oximes are chosen for the investigations, creating a serious problem for interpretation of experimental data. Aimed at overcoming these uncertainties, by combining different parameters, a promising dynamic model has been developed which may serve as a tool for defining effective oxime concentrations, for optimizing oxime treatment and for developing animal models.^134,147 This model enables the simulation of dynamic changes in AChE activity by including enzyme kinetic (i.e., inhibition, reactivation, aging), pharmacokinetic and toxicokinetic parameters. Validation of the model using in vitro enzyme kinetic constants and distinct in vivo inhibitor and oxime concentrations demonstrated a good agreement between patient and calculated AChE activities for parathion poisoning treated with LüH-6.

Based on the results of the reactivation studies for organophosphorus insecticide-inhibited human AChE, LüH-6 seems to be the logical first choice therapy. However, due to the paucity of published clinical data, further studies are needed to establish the optimal therapeutic regimen. This comprises a permanent search for an oxime with universal antidotal characteristics, as well as carefully designed and harmonized protocols for experimental and clinical studies, thus enabling reliable data that can be implemented in comprehensive (re)assessment procedures with a minimum of uncertainties.

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