Evaluation of the antimutagenic and antiradical potentials of extracts from the tubers of (Tunisian) Cyperus rotundus

The mutagenic potential of aqueous, total oligomers flavonoids (TOF), ethyl acetate and methanol extracts from tubers of Cyperus rotundus L. was assessed using Ames Salmonella tester strains TA98 and TA100, and SOS chromotest strain Escherichia coli PQ37 with and without metabolic activation (S9). None of the different extracts produced a mutagenic effect. Likewise, the antimutagenicity of the same extracts was tested using the “Ames test” and the “SOS chromotest”. Our results showed that C. rotundus extracts possess antimutagenic effects against S. typhimurium TA98 and TA100 strains towards the mutagen aflatoxin B1 (AFB1), similar to E. coli PQ37 strain against AFB1 and Nifuroxazide mutagens using the SOS chromotest assay. A free radical scavenging test was used in order to explore the antioxidant capacity of the extracts obtained from the tubers of C. rotundus. TOF, ethyl acetate and methanol extracts showed an important free radical scavenging activity towards the 1,1-diphenyl-2-picrylhydrazine (DPPH) free radical. These extracts showed an IC50 value of respectively 5, 20 and 65?µg?mL^?1. The beneficial effects of TOF, ethyl acetate and methanol extracts of C. rotundus were assessed by antioxidant and antimutagenic activities.     

Benzo[a]pyrene oxidation and microsomal enzyme activity in the mussel (Mytilus edulis) and other bivalve mollusc species from the Western North Atlantic

Analysis of subcellular fractions revealed a complement of microsomal electron transport components including reductases and heme proteins in several organs of the three bivalve species Mytilus edulis, Macrocallista maculata and Area zebra. Dithionite difference spectroscopy of CO-treated microsomes yielded spectra typical of cytochrome P-450 in digestive gland and gill, with absorption maxima at 450 nm. A time-dependent reduction of cytochrome P-450 was also observed. The levels of these components and rates of microsomal benzo[a]pyrene (BP) metabolism were highest in the digestive gland, and were very similar between species. In M. edulis there was a suggested seasonal variation in BP metabolism but no population differences in this activity or in levels of other components. Digestive gland microsomal metabolites of BP identified by HPLC retention and UV spectroscopy included BP-1.6-quinone, BP-3,6-quinone and BP-6,12-quinone, which comprised 65% of the total metabolites, and dihydrodiols and phenols, the latter products consistent with cytochrome P-450 monooxygenation and expoxide hydrolase function. However, the inconsistent dependence of BP metabolism on NADPH, and inconsistent inhibition by CO suggest that catalyst(s) additional to cytochrome P-450 may be acting in BP metabolism. Based on these results and the prominent quinone formation, we speculate that peroxidative mechanism(s) may be involved. The role of peroxidative as well as well as monooxygenase reactions in the in-vivo disposition and effects of foreign chemicals in bivalves, and also the major function of cytochrome P-450 in these bivalves, remain to be established.Some of these results have appeared in preliminary form; J. J. Stegeman, Sea Grant Annual Report, Words Hole Oceanographic Institution, p 15, 1981     

利用SOS/umu测试方法鉴定沙颍河河水中的遗传毒性物质

采用HPLC分割导向的SOS/umu测试方法鉴定了沙颍河河水中的遗传毒性物质。当采用TA1535/pSK1002菌株测定HPLC分割的各馏分时,如果不经大鼠肝微粒体酶(S9)代谢活化,只有馏分F10显示遗传毒性,加入大鼠肝微粒体酶代谢活化后,馏分F10和馏分F15都显示有遗传毒性,说明河水中存在某些需经过大鼠肝微粒体酶代谢活化才能显示出遗传毒性的物质。当采用过量表达O-乙酰转移酶(O-AT),对芳香胺类物质和硝基芳烃化合物有特殊响应的NM2009菌株测定时,馏分F8、F9和F10均呈现遗传毒性;特别是对于馏分F10,用NM2009菌株测定的遗传毒性远高于原始菌,说明这3个馏分中都含有芳香胺类或硝基芳烃类物质。     

Nickel toxicity in partially hepatectomized rats: I. accumulation of radioactive nickel in various organs and subcellular fractions of liver

The distribution of radioactive nickel (50 μmol/kg/200μ Ci S.C.) was studied in various organs as well as in the hepatic subcellular fractions of sham operated and partially hepatectomized rats at 16 hr after injection. ⁶³Ni was maximally accumulated in kidney followed by lung, liver, heart and spleen. The incorporation of ⁶³Ni was lowered in partially hepatectomized rats compared to sham operated ones. Subcellular binding of ⁶³Ni showed significantly high affinity of nickel to cytosol followed by nuclear, mitochondria and microsomes in both the groups.     

Comparative in vitro metabolism of chloroxylenol,chlorophene, and triclosan with rat,mouse, and human hepatic microsomes

A number of studies have reported the presence of chlorinated phenols, commonly used as antiseptics, in the environment. Chloroxylenol, chlorophene, and triclosan are three such chemicals believed to have leached into water supplies through the wastewater treatment facilities. Understanding how these compounds are metabolized is important in determining the risks of chemical exposure. In this study, we compared the in vitro metabolism of these three chlorinated phenols with rat, mouse, and human liver microsomes. The structures of the metabolites formed during the microsomal reactions were identical when rat, mouse, and human liver extracts were used, but variations existed in the kinetics of the reactions.     

Supramolecular complex formation,a possible antigenotoxic mechanism of glucomannan against aflatoxin B1

Abstract

Glucomannan is a highly branched polysaccharide with glycosidic linkages, constituted of mannoses and glucoses. In recent years, its usefulness due to its immunological, antioxidant and antimutagenic activity has been recognized. The aim of the study was to determine the antigenotoxic ability of glucomannan extracted from Candida utilis orally administered (100–700?mg/kg) to mice, which subsequently received 1?mg/kg aflatoxin B₁. Hepatocytes obtained from these animals 4–16?h post administration were examined by means of the comet assay. The antigenotoxic effect was found to be higher than that observed in previous studies with α-mannan and β-D-glucan isolated from Saccharomyces cerevisiae., In order to explore the possibility of formation of a supramolecular complex between glucomannan and aflatoxin B₁, both compounds were co-crystallized, their melting points determined, and the complex analyzed through ultraviolet spectroscopy. The spectroscopy data suggest that the protective effect of glucomannan is related to the formation of a supramolecular complex between the two compounds.     

Studies on cytochrome P450 in Mytilus galloprovincialis: induction by Na-phenobarbital and ability to biotransform xenobiotics

Mytilus galloprovincialis has a hepatopancreatic monooxygenase activity cytochrome P₄₅₀-dependent. The present paper studies the induction of this activity in the hepatopancreatic microsomes after treatment of M. galloprovincialis with Na-phenobarbital. Mussels were collected from the Gulf of La Spezia in 1985. We measured the increase in levels of cytochrome P₄₅₀, b₅, and P₄₂₀ and the 7-ethoxycoumarin deethylase activity. Furthermore, the fraction of mouse liver was replaced by the correspondent mussels' hepatopancreatic fraction in the yeast genotoxicity test to determine the ability of mussels to biotransform cyclophosphamide and styrene oxide. The results suggest that edible mussels are capable of detoxicating styrene oxide but not of bioactivating cyclophosphamide.     

恩诺沙星在鲫鱼肝微粒体中的代谢及代谢关键酶的确定

抗生素因具有抗菌谱广、杀菌性强等特点使其被广泛应用于人类医药、畜牧业、农业和水产养殖业。其进入水生生物体内后，会在药物代谢酶的作用下发生代谢转化，产生生态毒性。本研究采用鲫鱼肝微粒体体外孵育法，探究恩诺沙星细胞色素P450酶作用下的代谢转化过程，并通过代谢抑制实验确定关键的代谢酶。实验结果表明，恩诺沙星体外代谢过程符合一级动力学方程，当恩诺沙星暴露浓度为1 mg·L-1时，其在肝微粒体中的消除速率常数k最大为0.00303 min-1，半衰期t1/2最短为228.8 min，应用HPLC-MS/MS技术，检测到了恩诺沙星脱乙基产物和羟基化产物；代谢抑制实验结果表明，CYP3A4在恩诺沙星代谢过程中起主要作用，是恩诺沙星代谢的关键酶。本研究结果为深入了解恩诺沙星在水生生物体内的代谢转化及其生态风险提供了基础数据。     

Toxicokinetics,metabolism, and microsomal studies of chlorpropham in rats

A study on the toxicokinetic behavior, metabolism of chlorpropham, and its effect on cytochrome P₄₅₀ from liver microsomes was carried out in albino rats after a single and consecutive oral administration at 500?mg?kg^?1 body weight for 10 and 20 days. Chlorpropham was detected in the blood at 0.08?h (11.43?±?1.72?µg?mL^?1) reaching a maximum concentration at 2?h (30.90?±?2.55?µg?mL^?1) and a minimum at 48?h (1.95?±?0.20?µg?mL^?1) after a single oral administration of 500?mg?kg^?1. The absorption rate constant (K _a) was 0.66?±?0.48?h^?1. The Vd _area (18.01?±?2.78?L?kg^?1) and t _1/2 β (12.23?±?1.96?h) values suggested a wide distribution and long persistence of the compound in the body, respectively. The higher Cl_R (0.82?±?0.00?L?kg^?1?h^?1) compared to Cl_H (0.18?±?0.02?L?kg^?1?h^?1) value indicated that a major portion of chlorpropham was excreted through the urine (30%) compared to the faeces (2.81%). Chlorpropham residue was detected in all tissues of rat at 0.25?h while its metabolite, meta-chloroaniline was detected in liver, kidney, heart, lung, and spleen tissue at 0.25?h. Meta-chloroaniline was not detected in skeletal muscle, brain, fat, and stomach tissue at any time of the observation period. Maximum concentrations of chlorpropham and meta-chloroaniline were detected at 2?h (except in the spleen), and minimum concentrations of chlorpropham at 24 (heart, lung, spleen, skeletal muscle, and stomach) and 48?h (liver, kidney, brain, and fat tissue) respectively; and meta-chloroaniline at 24?h (except heart and spleen). The tissue half-life of chlorpropham in rat varied from 3.80 to 11.60?h. Repeated oral administration of chlorpropham at 500?mg?kg^?1 for 10 and 20 days caused an induction of the liver microsomal pellet of rat.     

金矿区中国林蛙体内DNA甲基化水平

采集金矿附近山区河流水质、沉积物和当地两栖类动物中国林蛙样品,应用高效液相色谱仪测定污染区和对照区林蛙体内各组织器官的胞嘧啶(c)和5-甲基胞嘧啶(5-mc)含量,探讨因金矿开采引起的汞污染以及对林蛙体内组织器官DNA甲基化水平的变化,研究汞胁迫下,两栖类动物体内分子水平的影响。结果表明:金矿开采区河流水质和沉积物已受到甲基汞污染,污染区林蛙体内甲基汞含量远高于对照区;林蛙体内各组织器官中DNA甲基化水平发生不同的变化:污染区林蛙肝脏和皮肤中DNA甲基化水平高于对照区,肌肉和脑干DNA甲基化水平低于对照区;雄性林蛙肝脏和脑干DNA甲基化水平高于雌性,肌肉和皮肤DNA甲基化水平却低于雌性。以上结果说明汞胁迫下,中国林蛙体内组织器官DNA甲基化水平可以发生一定的变化,环境中重金属汞离子进入林蛙体内含量的不同,可以促进或抑制其体内甲基化水平的变化,引起基因毒性作用。     

Distribution of tetrodotoxin in various organs of the starfish Astropecten polyacanthus

Tissues of various organs of the starfish Astropecten polyacanthus collected in the Hiroshima Prefecture from April 1985 to June 1986 were analyzed for lethal potency by the assay method for tetrodotoxin. The ovary showed the highest potency (47 to 1 450 MU g^-1), followed by the digestive organs (<10 to 960 MU g^-1) and the exoskeleton including spines and tube-feet (<10 to 170 MU g^-1). The pyloric caecum and testis were less toxic. Overall toxicity was remarkably higher in females (2 060±382 MU, mean±SE) than in males (1 106±214 MU).     

Acid and alkaline phosphatase activities in the clam Ruditapes philippinarum

Acid and alkaline phosphatase activities have been partially characterized in Ruditapes philippinarum (Adams and Reeve, 1850). Two activity peaks at pH=4.5 and pH 10.5 were detected in the gill, digestive gland, mantle, siphon and foot. Acid phosphatase activity was higher than that of alkaline phosphatase. The highest activity for both enzymes was observed in the digestive gland and, in decreasing order, the gill, foot, siphon and mantle. Alkaline phosphatase activity was similar in the mantle, siphon and foot. K _m values were determined for both enzymes in the gill and digestive gland. Hill coefficients were near 1, indicating no allosteric behaviour for either enzyme in the two organs. The optimum temperature was the same for acid phosphatase in both gill and digestive gland (50 °C), while for alkaline phosphatase it differed for these two organs (gill, 40 °C; digestive gland, 35 °C). The apparent activation energy was obtained from Arrhenius plots, and ranged from 8.61 kcal/mol for alkaline phosphatase in the gill, to 10.84 kcal/mol for acid phosphatase in the digestive gland. The effects of metals (1 mM conc) on both enzyme activities were assayed in vitro. Hg strongly inhibited the enzyme activities in the gill and digestive gland, probably because of its affinity for the sulphydryl group. Histochemically, acid phosphatase in the gill was located in a granular form throughout the gill cells, but was undetectable in the ciliate epithelium of the gill filaments. Alkaline phosphatase was located in the gill skeleton. Clam size and phosphatase activities were inversely related, probably reflecting a decrease in shell deposition with inereasing size. As a function of season, both enzymes were present in lowest amounts in winter, when undifferentiated sex cells were predominant in the germinative epithelium, and highest in summer, when ripe individuals of both sexes were more frequent.     

离体模型预测鱼体肝脏清除速率：鲑鱼肝细胞和肝脏S9组分的比较

将离体肝细胞和肝脏S9组分用于获取鱼类的体外生物转化数据可以优化模拟评估对化学物质的生物富集作用。然而涉及2种方式之间的直接对比的研究却几乎没有。本研究采用冷藏保存的鲑鱼肝细胞来测定对于6种多环芳烃(PAHs)的体外本征清除速率。我们运用测定结果推测体内本征清除速率，并将其作为输入值输入一种充分搅匀的肝脏模型中来预测肝清除速率。将事先由体外灌流肝脏测定的速率作为参考来评价预测结果。在2种竞争结合的假说前提下，由鲑鱼肝细胞测出的肝清除速率与实现的测定结果基本一致(6种多环芳烃中的5种都保持在2.1倍差异以下)。尽管多环芳烃的高代谢率是可能的原因之一，这些发现与之前由肝脏S9组分得出的结果相似。对苯并芘这一种化合物而言，由S9数据得出的体内本征清除速率是由肝细胞得出结果的10倍左右，这一结果可能是由细胞吸收速率造成的传播限制引起的。尽管苯并芘的结果差异较大，由任何一种体外测试方法得出的体内本征清除速率结果通常是一致的。这些结果显示离体肝细胞和肝脏S9组分2种系统均可用于优化鱼类的生物富集评估，尤其对于体外反应速率较高的情况。不同系统在化工领域的应用性是否相同则需要进一步的研究工作。
精选自Kellie A. Fay, Patrick N. Fitzsimmons, Alex D. Hoffman， John W. Nichols. Comparison of trout hepatocytes and liver S9 fractions as in vitro models for predicting hepatic clearance in fish. Environmental Toxicology and Chemistry: Volume 36, Issue 2, pages 463–471, July 2017. DOI: 10.1002/etc.3572
详情请见http://onlinelibrary.wiley.com/wol1/doi/10.1002/etc.3572/full
     

Combined effects of 2,3,7,8-tetrachlorodibenzo- p -dioxin and polychlorinated biphenyl congeners in rats

The objective of this work was to evaluate potential interactions between 2,3,7,8-tetrachlorodibenzo-p-dioxin (TCDD) and polychlorinated biphenyls congeners (PCBs) in rats. Groups of five adult female rats were given 0, 2.5, 25, 250, or 1000?ng TCDD/kg body weight/day or TCDD in combination with a mixture of PCB congeners at a concentration of 2 or 20?µg?kg^?1 body weight/day by gavage for 28 days. After the 28-day treatment period, the rats were killed for the analysis of biochemical, liver enzyme activities, and hematological and pathological end points. Growth suppression, increased absolute and relative liver weights, and decreased thymic weight were observed in the 1000?ng TCDD group alone, or the groups receiving a mixture of 1000?ng TCDD and 2 and 20?µg PCBs. TCDD-increased liver and thymic weights were not altered by PCBs; however, growth suppression was more pronounced in animals receiving 1000?ng TCDD and 2?µg PCBs. Increased hepatic microsomal methoxy resorufin-O-demethylase and ethoxy resorufin-O-deethylase activities occurred in 250 and 1000?ng?kg^?1 TCDD-treated animals, which were antagonized by PCBs. Effects of 250?ng TCDD on serum cholesterol and liver uridine diphosphate glucuronosyl transferase activity were reduced by 20?µg PCBs. Treatment with 1000?ng TCDD increased serum albumin, decreased liver vitamin A, increased kidney vitamin A, and liver microsomal glutathione-S-transferase activity, which were not affected by PCBs. Decreased hemoglobin, platelet, packet cell volume, and red cell indices were observed in TCDD-treated rats, but no interactive effects were seen. Histopathological evaluation revealed that liver, thyroid, and thymus were the target organs, but the effects of co-exposure to PCBs and TCDD were variable. These results indicate that the mixture effects of PCBs and TCDD may be additive, synergistic, or antagonistic depending on the dose level and end points measured.     

Variations in carbohydrate metabolism during gonad maturation in female turbot (Scophthalmus maximus)

Several carbohydrate metabolism pathways were studied in four different tissues (liver, gonad, kidney and white muscle) of female turbot (Scophthalmus maximus) at three different stages of gonad maturation, i.e., previtellogenesis, early vitellogenesis and late vitellogenesis. During carbohydrate metabolism in the liver, the only major change noticed throughout vitellogenesis was increased glycolytic activity at early vitellogenesis. The major changes observed in the gonad during vitellogenesis were an increased use of exogenous glucose and increased gluconeogenesis, which were reflected in increased glucose levels throughout vitellogenesis accompanied by a small increase in glycogen levels. Changes observed in carbohydrate metabolism in the kidney pointed to increased gluconeogenesis during early vitellogenesis. Finally, during ovarian maturation, the muscle mobilized proteins whose constituent amino acids could have been used in other tissues either as substrates for gluconeogenesis or for protein synthesis. As an overall conclusion, changes in the carbohydrate metabolism of female turbot during maturation are quite marked in the gonad, kidney and white muscle, in contrast to other species, in which major changes have been previously reported to occur in the liver.     

大鼠不同脏器亚硫酸氧化酶活性及其与年龄的关系

为了探讨体内亚硫酸氧化酶的分布特点及随年龄的变化规律,以Wistar大鼠为实验材料,研究了不同月龄大鼠脏器中的亚硫酸氧化酶活性.以细胞色素C为电子受体,应用分光光度法测定了不同月龄(1、4、10个月)大鼠肝、肾、肺、脾、脑、胃及胸主动脉中亚硫酸氧化酶的活性.结果表明:1)亚硫酸氧化酶在大鼠全身主要脏器中普遍存在,且在不同脏器中该酶的活性不同,从强到弱的顺序基本表现为:肝、肾>胃>脑>胸主动脉血管>肺>脾;2)肝、肾、血管组织中亚硫酸氧化酶活性与大鼠年龄相关,肝脏亚硫酸氧化酶活性随年龄的增加而增加(Spearman,r=0.674,p<0.001),而肾脏和胸主动脉血管该酶活性随年龄的增加而减小(Spearman,r=-0.756,p<0.001;r=-0.629;p<0.05),其余脏器未见明显变化;3)亚硫酸氧化酶活性降低可能是一种机体衰老的生化标志物.     

Royal jelly inhibited N-acetylation and metabolism of 2-aminofluorene in human liver tumor cells (J5)

The present study was carried out to evaluate the question of whether or not royal jelly affects N-acetylation and metabolism of 2-aminofluorene (2-AF) in the human liver tumor cell line (J 5). N-acetylation and metabolism of 2-AF in intact J5 cells was determined by using high performance liquid chromatography for the amounts of acetylated and nonacetylated 2-AF and profile of 2-AF metabolism. The results indicated that royal jelly displayed a dose-dependent inhibition of N-acetylation of 2-AF in J5 cells. Royal jelly also decreased the profile of 2-AF metabolites in J5 cells. This report is the first demonstration which showed that royal jelly affects N-acetylation of 2-AF in human liver tumor cells (J5).     

Toxicological and ecological implications of biotransformation enzymes in the tropical teleost Chaetodon capistratus

Hepatic cytochromes P450 (phase I monooxygenases) and glutathione transferases (phase II conjugating enzymes) were investigated in Chaetodon capistratus (Linnaeus) collected in Florida and Belize in June and December 1991, respectively. These biotransformation enzymes play major roles in the detoxification of xenobiotics by converting lipophilic chemicals to more hydrophilic, readily excretable metabolites. Content of total microsomal P450 (0.501 to 0.821 nmol mg^-1 microsomal protein) and rates of NADPH-cytochrome c (P450) reductase (270.7 to 330.2 nmol min^-1 mg^-1 microsomal protein) and glutathione transferase (2.81 to 3.12 g min^-1 mg^-1 cytosolic protein) in these fish were greater than in most untreated fish species, i.e., fish that have not been exposed to PAHs (polycyclic aromatic hydrocarbons) or PCBs (polycyclic biphenyls). Ethoxyresorufin O-deethylase (EROD) rates (0.029 to 0.171 nmol min^-1 mg^-1) were also comparable to those in most untreated marine fish. Immunoblot analysis with monoclonal antibody (MAb) 1-12-3 to scup P450E (the EROD catalyst and a teleost representative of the PAH-inducible CYP1A gene subfamily) showed slight amounts of cross-reacting protein in C. capistratus liver microsomes. Hepatic CYP1A content and EROD activity did not differ significantly between fish collected in Florida and Belize, suggesting that the two sites differed little in contamination by CYP1A inducers. Immunochemical analyses with polyclonal antibodies to scup P450B (a teleost representative of the CYP2B subfamily) and human CYP3A4 cross-reacted strongly with C. capistratus hepatic proteins. The CYP2B and CYP3A subfamilies in mammals are believed to have partially evolved in response to toxic dietary allelochemicals. C. capistratus regularly feeds on terpenoid-rich gorgonian corals, suggesting that biotransformation enzymes may be involved in the metabolism of dietary allelochemicals as well as anthropogenic xenobiotics in this species.     

Sulfide tolerance and detoxification in shallow-water marine fishes

Hydrogen sulfide is a potent inhibitor of aerobic respiration. Sulfide is produced in sediments, and many species of fish live in association with the bottom. Tolerance tests, enzyme assays, and chromatography of sulfur compounds in thirteen species of shallow-water marine fishes (collected in San Diego, California, USA in 1987–1988) indicate adaptations to sulfide that vary with habitat and lifestyle. Tidal-marsh inhabitants, like Gillichthys mirabilis and Fundulus parvipinnis, have higher tolerance to sulfide (96 h LC₅₀ at 525 to 700 M) relative to outer-bay and open-coast inhabitants (surviving <12 h at much lower concentrations). The cytochrome c oxidase of all species shows high activity and susceptibility to sulfide poisoning, with 50% inhibition at 30 to 500 nM in various tissues. The two marsh species are able to survive at sulfide concentrations already inhibitory to their cytochrome c oxidase and fatal to other species. All species detoxify sulfide by oxidizing it to thiosulfate. All have sulfide-oxidizing activity in the blood, spleen, kidney, liver and gills, which correlates significantly with heme content. Thiosulfate appears in the tissues of sulfide-exposed fish and builds up to high concentrations (up to 2 mM) with stronger and longer exposure. Unexposed fish contain little or no thiosulfate. Sulfide is barely detectable in the tissues, even in high-sulfide exposure tests. We suggest that fish blood, in having high sulfide-oxidizing activity and no cytochrome c oxidase, can act as a short-term first line of defense against sulfide, and thus minimize the amount that reaches the vital organs. The results of this study indicate that sulfide is a significant environmental factor influencing the ecological distribution of marine fishes.     

脱氧雪腐镰刀菌烯醇、黄曲霉毒素B_1和玉米赤霉烯酮对秀丽隐杆线虫的联合毒性研究

脱氧雪腐镰刀菌烯醇(DON)、黄曲霉毒素B_1(AFB_1)和玉米赤霉烯酮(ZEN)是最为常见的粮食真菌毒素,易共存于谷物产品和动物饲料中,而目前对其联合毒性的研究较少,且研究结果并不完全一致。为探究DON、AFB_1和ZEN的联合毒性作用,本论文以秀丽隐杆线虫(C.elegans)为模型,分别评估了毒素混合物AFB_1+DON、AFB_1+ZEN、DON+ZEN和AFB_1+DON+ZEN对C.elegans的生长发育(体长)和生殖能力(产卵量)的毒性作用,并用Chou-Talalay模型来判定毒素混合物的相互作用类型。研究表明,AFB_1、DON和ZEN单独染毒C.elegans时,其毒作用强弱为AFB_1ZENDON。联合染毒时,AFB_1+DON对C.elegans产生协同作用,而DON+ZEN则产生拮抗作用;AFB_1+ZEN对体长(24 h)和产卵量的毒作用随着暴露浓度的增加,由弱拮抗变为协同作用,而在毒素暴露48 h后,对线虫的生长发育呈协同作用;AFB_1+DON+ZEN除在EC50-24 h和EC75-24 h时对体长产生明显的毒性增强作用外,其他普遍表现出拮抗作用。由此表明,DON、AFB_1和ZEN对C.elegans的联合毒性作用与剂量和时间相关。