Induction of detoxification enzymes in phytophagous insects: Role of insecticide synergists,larval age,and species

Five insecticide synergists, all of which were either methylenedioxyphenyl compounds or analogs, were compared as to their effect on cytochrome P450 monooxygenase induction caused by an allelochemical in fall armyworm larvae. Feeding the synergists (piperonyl butoxide, safrole, isosafrole, MGK 264, and myristicin) individually to the larvae caused decreases in the microsomal aldrin epoxidase activities ranging from 38% to 74% when compared with controls. Feeding indole-3-carbinol resulted in a 4-fold increase in the microsomal epoxidase activity. However, cotreatment of any of the synergists and the inducer completely eliminated the induction. Sixth instar larvae were more inducible than second instar larvae with respect to microsomal epoxidase and glutathione transferase in the fall armyworm. Enzyme inducibility varied widely among the seven phytophagous Lepidoptera examined. When indole-3-carbinol was used as an inducer of microsomal epoxidase, the extent of inducibility of the enzyme was fall armyworm > velvetbean caterpillar > corn earworm > beet armyworm > tobacco budworm > cabbage looper > diamondback moth. When indole-3-acetonitrile was used as an inducer, the inducibility of glutathione transferase was fall armyworm > beet armyworm > corn earworm > cabbage looper > velvetbean caterpillar > tobacco budworm > diamondback moth. Inducibility of five microsomal oxidase systems also varied considerably in the corn earworm, indicating the multiplicity of cytochrome P450 in this species. Microsomal epoxidase and glutathione transferase were induced by cruciferous host plants such as cabbage and their allelochemicals in diamondback moth larve. © 1993 Wiley-Liss, Inc.     

CJX1, an amlodipine derivative, interacts with ATPase of human P-glycoprotein

Our aim has been to elucidate the possible mechanism of CJX1, an amlodipine derivative, in the modulation of P-gp function by determining its effect on P-gp ATPase activity. Basal P-gp ATPase activity was increased by CJX1 with half-maximal activity concentration (Km) of 8.6 ± 1.4 μM. Kinetic analysis indicated a non-competitive inhibition of Verapamil (Ver)-stimulated P-gp ATPase activity by CJX1 and competitive inhibition of CJX1-stimulated P-gp ATPase activity by tetrandrine (Tet). The effect of CsA on CJX1-stimulated and Ver-stimulated P-gp ATPase activity was non-competitive and competitive inhibition, respectively. These findings implying that CJX1 and Tet can bind P-gp either on overlapping sites or distinct but interacting sites, while CJX1 and Ver as well as CsA can bind P-gp on separated sites in K562/DOX cells. Furthermore, the combined effect of CJX1 and Ver has been evaluated isobolographically in numerous fixed-ratio combinations of 1:1, 1:2, 1:4, 1:8, 1:10 in K562/DOX cells. The results show that mixtures of both drugs at these fixed-ratios exerted synergistic interactions, indicating that when the two reverses that bind P-gp on separated sites are combined, each can contribute to the overall interaction with P-gp, leading to the greater effect than that by either agent alone.     

Use of 1-anilino-8-naphthalene-sulfonate as a probe of gastric vesicle transport.

The interaction of 1-anilino-8-naphthalene-sulfonate (ANS) with vesicles derived from hog fundic mucosa was studied in the presence of valinomycin and with the addition of ATP. Evidence was found for two classes of sites, those rapidly accessible to ANS with a KD of 7.5 micronM and those slowly accessible, but rapidly accessed in the presence of valinomycin with a KD of 2.5 micronM. ATP transiently increases the quantum yield of the latter ANS binding sites only in the presence of valinomycin, but does not alter the number of KD of those sites. The time course of this increase correlates with H+ uptake and Rb+ extrusion by those vesicles and H+ carries such as tetrachlorsalicylanilide or nigericin abolish the ATP response. With ATP addition in the presence of SC14N and valinomycin there is transient uptake of SCN-. It is concluded that ANS is acting as a probe of a structural change dependent on a potential and H+ gradient.     

Genotoxicity of an organophosphorus insecticide,dimethoate, in the mouse

The effects of dimethoate were investigated in the mouse after acute (10 mg/kg i.p.) or chronic treatment (0.6 ppm, 5 days a week for 7 weeks). Dominant lethal mutations were scored for a 7-week period after the acute dose, and immediately after exposure for the chronic dose. Chromosome damage was also analysed in bone marrow and spermatogonial cells at the same dose levels (from 12 to 48 h after treatment). MMS (60 mg/kg i.p.) was chosen as the positive control.In no experiment did dimethoate show any genotoxicity.     

Mutation in ace1 associated with an insecticide resistant population of Plutella xylostella

Insensitive acetylcholinesterase (AChE) was determined to be involved in an EPN-resistant (ER) strain and a contaminated susceptible (CS) strain of diamondback moth (DBM, Plutella xylostella L.), as estimated by AChE inhibition assay using DDVP as a inhibitor in a nondenaturing electrophoresis gel. The ER strain exhibited very high AChE insensitivity, high resistance ratio, and two point mutations (G324A, A298S) in ace1-type AChE gene (Pxace1). The CS strain showed low AChE insensitivity, low resistance ratio, and it has only one point mutation (G324A). These findings suggest that the A298S mutation, along with reported G324A mutation (Baek et al, 2005), can be important in the development of organophosphate resistance. These results also suggest that the A298S mutation could be a good candidate for a molecular diagnosis marker for resistance monitoring. Three molecular diagnosis methods (Quantitative Sequencing; QS, PCR amplification of specific alleles; PASA and restriction fragment length polymorphism; RFLP) were developed which successfully detected specific resistance associated point mutations. Seven local population DBMs were surveyed and showed high insecticide resistance levels and a A298S mutation in Pxace1. These methods can be used to monitor the resistance allele in field population of DBMs and resistance management strategy.     

The effect of mixtures of Bacillus thuringiensis-based insecticide and multiple nucleopolyhedrovirus of Lymantria dispar L. in combination with an optical brightener on L. dispar larvae

BioControl - This study evaluated the efficacy of the commercially available insecticide Lepidocide based on Bacillus thuringiensis var. kurstaki and Lymantria dispar multiple nucleopolyhedrovirus...     

Nitrogen fixation and indole acetic acid production by Azospi-rillum sp. as influenced by an insecticide, carbofuran

Both indole acetic acid (IAA) accumulation and nitrogen fixation were increased in Azospirillum cultures isolated from rice roots and soils by carbofuran (2, 3-dihydro-2, 2-dimethyl-7-benzofuranyl-N-methyl carbamate), an insecticide widely used in rice cultivation. Addition of carbofuran at 5 and 10 parts/10₆ significantly stimulated nitrogen fixation in Azospirillum. Indole acetic acid accumulation by Azospirillum cultures was more pronounced at a lower level (250 g/50 ml) of carbofuran. Evidence is provided for carbofuran degradation by Azospirillum cultures. The 7-benzofuranol (2, 3-dihydro-2–2-dimethyl-7 benzofuranol), a major degradation product of carbofuran, however, did not enhance the IAA accumulation. The higher accumulation of IAA in Azospirillum in the presence of carbofuran is probably related to the increased growth due to fixed N present in the insecticide. Results indicate the involvement of parent compound carbofuran and/or compounds other than the 7-benzofuranol in the higher accumulation of IAA by Azospirillum sp.     

氨基甲酸酯杀虫剂灭蚜威及其与阿维菌素的混配制剂对美洲斑潜蝇的防治效果

田间试验表明 ,氨基甲酸酯新杀虫剂灭蚜威单剂与生物农药阿维菌素混剂对美洲斑潜蝇Liro myzasativae防治效果优良。 5 0 %灭蚜威可湿粉使用剂量 2 5g(a .i.) 667m2 的 3～ 1 1d校正防效为85 2 8%～ 86 3 9% ,1 8 75g(a.i.) 667m2 相应药效为 83 0 1 %～ 84 0 4%。 3种不同配比的灭蚜威与阿维菌素混剂使用剂量 1 0g(a .i.) 667m2 ,药后 3～ 1 1d防效为 85 90 %～ 90 3 3 % ,7 5g(a .i.) 667m2 相应药效为 83 48%～ 88 5 2 %。     

Inhibition by talipexole, a thiazolo-azepine derivative, of dopaminergic neurons in the ventral tegmental area.

A microiontophoretic study using rats anesthetized with chloral hydrate and immobilized with gallamine triethiodide was carried out to compare the effect of talipexole (B-HT 920 CL2:2-amino-6-allyl-5,6,7,8-tetrahydro-4H-thiazolo [4,5-d]-azepine-dihydrochloride), a dopamine autoreceptor agonist, on dopaminergic neurons in the ventral tegmental area (VTA) to non-dopaminergic neurons in the VTA. VTA neurons were classified into two types according to the responses to antidromic stimulation of the nucleus accumbens (Acc): type I neurons with a long spike latency (8.69 +/- 0.24 msec) upon Acc stimulation and low spontaneous firing rate (6.80 +/- 1.34/sec), and type II neurons with a short latency (2.76 +/- 0.20 msec) and high spontaneous firing rate (26.77 +/- 7.05/sec), probably corresponding to dopaminergic and non-dopaminergic neurons, respectively. In type I neurons, microiontophoretic application of talipexole and dopamine inhibited antidromic spike generation elicited by Acc stimulation, and talipexole-induced inhibition was antagonized by domperidone (dopamine D-2 antagonist). In type II neurons, however, the antidromic spikes were not affected by either talipexole or dopamine. Furthermore, spontaneous firing was also inhibited by iontophoretically applied talipexole and dopamine in most type I neurons, but rarely affected by either drug. Inhibitory effects of talipexole were antagonized by domperidone. These results suggest that talipexole acts on dopamine D-2 receptors, thereby inhibiting the dopaminergic neurons in the VTA.     

Metaretinochrome in membranes as an effective donor of 11-cis retinal for the synthesis of squid rhodopsin

Aporetinochrome, which is a protein moiety of retinochrome without chromophore retinal, is found in the membrane containing retinochrome. All of the prosthetic retinal of retinochrome in membranes, which is all-trans retinal, is bound to the chromophoric site on the protein moiety, with protonated Schiff bases showing an absorption band with the maximum at 495 nm. On exposure to light, retinochrome is converted to metaretinochrome at room temperature. The prosthetic retinals of metaretinochrome in membranes, which are 11-cis retinals, are in two states: retinals bound to the chromophoric site with protonated Schiff bases, and the free retinals, which are separated from the protein moiety. These states are suggested from the following observations. (a) The ratio of the absorbance at 470 nm of metaretinochrome to that at 495 nm of the parental retinochrome differs because of differences in samples and is higher in the purer preparations. (b) The difference spectrum of absorption of metaretinochrome caused by alkalinization shows two minimum peaks at approximately 420 and 470 nm. (c) The rate of bleaching of metaretinochrome in membranes with dilute NH2OH is much faster than that of retinochrome, and the absorption band in the near- UV region is more susceptible to NH2OH than the visible absorption band. The state of the prosthetic retinals in metaretinochrome was confirmed directly by the reaction of metaretinochrome in membranes with NaBH4. After treatment with NaBH4, the sodium dodecyl sulfate- polyacrylamide gel electrophoretic pattern shows two fluorescent bands: one at the position that corresponds to the retinochrome protein (mol wt 27,000 +/- 2,000), and another at the front of migration, where no band of protein is observed. Retinoids extracted from the NaBH4-treated metaretinochrome in membranes and analyzed with high-pressure liquid chromatography show a main peak of 11-cis retinol. The results of this and earlier (Seki et al., 1982) papers are summarized, and it is strongly suggested that metaretinochrome in the squid retina may play the role of 11-cis retinal donor for opsin and contribute to the synthesis of the squid rhodopsin.     

Understory vegetation as an indicator of soil characteristics in the Hyrcanian area,N. Iran

The mesic Caspian (Hyrcanian) forest and ecotone communities provide a marked contrast to the arid and semiarid landscapes associated with most of the territory of Iran. To date, the ecological characteristics of these habitats, threatened and of conservation importance, have been little studied. Accordingly, ecological profiles of some important plant species of these communities have been assessed along two altitudinal gradients (300–2300 m a.s.l.). Vegetation and soils were sampled every 100 m in elevation, with the data subsequently analyzed using TWINSPAN and corrected frequency (CF) analyses. Relationships between soil variables (subdivided into three classes, the lowest, the middle and the upper third of all values) and herbaceous and shrub species (presence/absence data) were analyzed by the polythetic divisive classification method. 379 plant species and eleven soil variables – N, P, K, CaCO₃, EC, pH, organic matter, C/N ratio and percentage of sand, clay and silt – were considered. The ecological profile method was used to evaluate the affinity and significance of associations between the probability of species’ occurrence and topsoil characteristics found by the polythetic method. Five vegetation groups were identified: two groups, with Acer campestre and Quercus macranthera in the tree layer and Veronica mazanderanae and Phuopsis stylosa as herbs, were restricted to forest-steppe ecotones and the upper mountain areas. Three groups, with Acer velutinum, Ruscus hyrcanus, Carpinus betulus, Danae racemosa, Fagus orientalis and Aruncus vulgaris as indicator species, occurred in the forest itself. Of the 42 plant species assessed as being of particular importance, 13 had significant relationships with eight soil factors. Thus, certain species, including endemic plant species of restricted distribution and conservation importance, can be used as indicators of particular soil conditions in the Hyrcanian forest area.     

Use of rare-earth elements as labels for studying biologically active compounds. IV. Luminescence spectra and structure of compounds of europium with nucleotides]

Spectra of europium coordinating nucleotides are investigated. Europium is shown to coordinate phosphate, but the way of coordination may change. Conditions of nitrogen bases coordination are determined. The evidence or the existence of coordinated immobilized water is found.     

The detoxication enzymes causing organophosphate resistance in the housefly; Properties, inhibition, and the action of inhibitors as synergists

A comparison of the breakdown enzymes in OP-resistant houseflies and the ali-esterase of susceptible flies shows differences as well as similarities. In general both are rapidly phosphorylated by the OP-compounds, but only in the case of the breakdown enzymes dephosphorylation can take place. The rate of phosphorylation of the breakdown enzymes by the toxicants is sometimes higher, sometimes lower than that of the ali-esterase with the same compound. Studies of the breakdown reaction showed the Km to be in the order of 10^–6–10^–8 M, the turnover numbers to range from 0.05–0.7 per minute. Whether dephosphorylation takes place depends on the type of breakdown enzyme and the nature of the phosphoryl group. For instance, in the malathion-resistant strains only the dimethyl phosphorylated enzymes are dephosphorylated, but the dimethyl and dipropyl phosphorylated enzymes are not. Dephosphorylation of the enzymes of diazinon-resistant strains occurs with both dimethyl and diethyl, but not with dipropyl compounds. Consequently hydrolysis of some OP-compounds can be blocked by the addition of others that irreversibly phosphorylate the enzymes. Substances that can block the reaction have a marked synergistic action when sublethal doses are applied simultaneously with the OP-compound to which a strain is resistant. There is evidence that the breakdown enzymes can still hydrolyse methyl butyrate and some other esters although at a rate which is only a few percents of that of the aliesterase. The problem as to how enzymes with a rather low breakdown capacity could confer high resistance is discussed.

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Zusammenfassung In phosphorsäureester-resistenten Stubenfliegen sind Abbaufermente vorhanden, die die Fähigkeit zur Hydrolyse von Sauerstoffderivaten derjenigen Verbindungen besitzen, gegen die Resistenz aufgetreten ist. Diese Enzyme entstehen an Stelle einer in anfälligen Fliegen vorkommenden Ali-Esterase. Das Auftreten der Ali-Esterase und der Abbaufermente unterliegt dem Einfluß verschiedener Allele eines Gens. Durch eine Kombination biochemischer, genetischer und toxikologischer Arbeitsmethoden wurden Bedeutung und Eigenschaften dieser Enzyme untersucht.Die Hemmung der Ali-Esterase durch organische Phosphorverbindungen wird durch eine irreversible Reaktion hervorgerufen, bei der eine Dialkylphosphorylierung des Enzyms stattfindet. Die modifizierten Ali-Esterasen oder Abbaufermente unterscheiden sich von der Ali-Esterase dadurch, daß der Reaktion mit den Produkten, gegen die Resistenz besteht, eine langsam fortschreitende Dephosphorylierung folgt. Diese Fähigkeit zur Hydrolyse bestimmter Verbindungen muß die Selektion der Allele hervorgerufen haben, die für die Bildung dieser Enzyme verantwortlich sind. Darüber hinaus wurden aber noch andere Veränderungen herbeigeführt: ein Verlust der Ali-Esterase-Aktivität, eine Änderung in der Affinität einer Azahl Phosphorverbindungen gegenüber und eine Verminderung der Stabilität.Vier verschiedene Abbaufermente sind in verschiedenen resistenten Stämmen vorhanden. Zwei von ihnen können Diäthylverbindungen mit einer Umsatzzahl von 0.05 und 0.25 pro Minute hydrolysieren. Das Enzym mit der höheren Umsatzzahl spaltet auch Dimethyl-Derivate; die Affinität für diese Verbindungen erscheint aber zur Ausbildung eines hohen Resistenzgrades zu niedrig. Zwei andere Fermente finden sich in Malathion-resistenten Stämmen, von denen eines wegen seiner wahrscheinlichen Instabilität in vitro nicht untersucht werden konnte. Das andere Enzym spaltet Malaoxon und einige weitere Methylverbindungen, wobei die Affinität Malaoxon gegenüber höher ist, was möglicherweise die Ursache der ziemlich hohen Spezifizität bildet.Obwohl die Umsatzzahlen sehr niedrig sind und die Enzyme wohl nur einen geringen Teil des in vivo applizierten Giftes zu hydrolysieren vermögen, gestattet aber anscheinend ihre hohe Affinität für Phosphorverbindungen die für die Cholinesterasehemmung notwendige Inhibitormenge zu reduzieren und verursacht so die Resistenz.Die Abbaufermente können bestimmte Typen von Phosphorsäureestern hydrolysieren; sie werden aber noch durch andere Verbindungen dieser Stoffklasse irreversibel gehemmt. Solche Präparate sind zur Blockierung der in vitro stattfindenden Hydrolyse befähigt und besitzen einen stark synergistischen Effekt, wenn sie mit den Thioverbindungen, gegen die Resistenz besteht, gleichzeitig appliziert werden. So werden die Abbaufermente der Malathion- und Parathion-resistenten Stämme durch Propylparaoxon irreversibel phosphoryliert. Sublethale Mengen dieser Substanz reduzieren die Resistenz beträchtlich.