Regulation of murine macrophage phagocytosis of sheep erythrocytes by T-2 toxin

The effect of a single oral dose of 4 mg of T-2 toxin/kg of body weight on in vivo phagocytosis of sheep RBC by peritoneal macrophages was evaluated in nonsensitized mice and in mice sensitized with sheep RBC. T-2 toxin treatment had no effect on the viability or phagocytic activity of resident peritoneal macrophages in nonsensitized mice. However, a significant (P less than 0.005) increase in phagocytic activity occurred in cells from mice treated with toxin and subsequently sensitized with sheep RBC. In contrast, phagocytosis of sheep RBC was significantly (P less than 0.05) suppressed in cells from mice treated with toxin after sensitization. Toxin treatment induced necrosis of lymphocytes and significant decreases in thymus and spleen weights. Seemingly, T-2 toxin, administered at a dose that caused marked lymphoid depletion, suppressed or enhanced in vivo macrophage phagocytic activity in antigenically sensitized mice, and enhancement or suppression of phagocytosis was a function of the time of toxin treatment in relation to antigenic stimulation.     

葡萄籽提取物原花青素对肉兔生长发育、血清酶活性及消化代谢的影响

本试验旨在研究葡萄籽提取物原花青素（Grape seed proanthocyanidin extracts,GSPE）对肉兔生长发育、血清酶活性及消化代谢的影响。采用单因子随机区组试验设计,选择128只60日龄、体质量相近的健康新西兰兔,随机分为4组（1个对照组和3个试验组）,每组32个重复,每个重复1只。对照组饲喂基础饲粮,3个试验组分别饲喂在基础饲粮中添加100、200、400mg/kg GSPE的试验饲粮。试验期为39d,其中预试期为6d,正试期为33d。正试期第10~15天收集试验兔排出的全部粪便和尿液。结果显示：4组试验兔死亡率和腹泻率分别为12.50%、6.25%、3.13%、3.13%和1.95%、1.52%、1.17%、0.59%;对照组试验兔日增重、日干物质进食量及血清碱性磷酸酶活性均显著（P〈0.05）或极显著（P〈0.01）低于200mg/kg组和400mg/kg组,而料重比及谷丙与谷草转氨酶活性均显著（P〈0.05）或极显著（P〈0.01）高于后者;对照组试验兔屠宰率显著（P〈0.05）或极显著（P〈0.01）低于其余3组,而400mg/kg组试验兔脾脏相对质量极显著（P〈0.01）高于其余3组;对照组试验兔十二指肠相对重量、相对长度及密度、空肠相对长度、盲肠相对质量、全肠道相对质量与相对长度及胃肠道相对质量均显著（P〈0.05）或极显著（P〈0.01）低于200mg/kg组和400mg/kg组,空肠相对质量、盲肠相对长度与密度、大肠相对长度及全肠道密度均显著（P〈0.05）或极显著（P〈0.01）低于400mg/kg组,且大肠相对质量与密度均显著（P〈0.05）或极显著（P〈0.01）低于其余3组;400mg/kg组试验兔饲粮干物质、有机物、粗纤维、钙与磷表观消化率、总能表观消化率与利用率及氮表观消化率均显著（P〈0.05）或极显著（P〈0.01）高于其余3组,氮利用率则显著（P〈0.05）高于对照组,而对照组试验兔饲粮粗脂肪表观消化率与消化能利用率均显著（P〈0.05）或极显著（P〈0.01）低于20     

Acute toxicological experiment of T-2 toxin in rabbits

Rabbits were treated with a single oral dose (1, 2, 4, 6, 8, 10 or 15 mg/kg body mass) of T-2 fusariotoxin. Doses of 4 mg or higher killed the animals in 24 to 48 h. As opposed to the controls, in the treated rabbits gross pathological and histopathological examinations revealed acute catarrhal gastroenteritis, necrosis of lymphoid cells of the gastrointestinal mucosa, centrolobular dystrophy of the liver, necrosis of cells of the mononuclear phagocyte system (MPS) in the liver, tubulonephrosis, focal dystrophy of the adrenal cortex, lymphocyte depletion involving both T- and B-cell-dependent zones of the lymphoid organs (spleen, lymph, ampulla ilei), and depletion and necrosis of the myelopoietic cell colonies of the bone marrow. Similar but milder changes were observed in surviving rabbits exsanguinated 48 h after treatment. In addition to the direct damage done to the digestive tract mucosa and liver, the toxin severely damaged the cells participating in humoral and cell-mediated immunity and in the local defence of the intestinal mucosa, and markedly impaired phagocytosis and granulocytopoiesis. In another experiment rabbits were given oral doses of 2 mg/kg body mass T-2 toxin daily for several days. One rabbit was killed by bleeding every day. In rabbits killed beyond day 7 there was subacute catarrhal gastritis, emaciation, and hypertrophy of the adrenal cortex.     

Comparison of the effect of T-2 toxin with that of dexamethasone or cyclophosphamide on resistance to Babesia microti infection in mice

The effect of T-2 toxin on host resistance to acute and latent Babesia microti infections was evaluated in mice and was compared with the effects of the immunosuppressive drugs dexamethasone and cyclophosphamide. Mice with acute or latent B microti infection were treated with 2 mg of T-2 toxin/kg of body weight, 0.2 mg of dexamethasone/kg, or 30 mg of cyclophosphamide/kg daily for 5 days. Treatment with dexamethasone or cyclophosphamide caused significant (P less than 0.05) increases in Babesia parasitemia during acute infection and significantly (P less than 0.05) prolonged the duration of parasitemia during acute babesiosis. Treatment with T-2 toxin caused a transient significant (P less than 0.05) increase in Babesia parasitemia on day 10 after acute infection and numerical, though statistically nonsignificant, increases in the maximal level and duration of parasitemia during acute babesiosis. Significant (P less than 0.005) recrudescence of parasitemia was observed in the dexamethasone- and cyclophosphamide-treated mice with latent Babesia infection. Treatment with T-2 toxin did not cause recrudescence of parasitemia in mice with latent Babesia infection.     

Variations in serum sorbitol dehydrogenase, aspartate transaminase, and isoenzyme 5 of lactate dehydrogenase activities in horses given carbon tetrachloride

Seven horses were given 0.5 mg of carbon tetrachloride/kg of body weight via a nasogastric tube. Subsequent hepatocellular damage was monitored by serum enzyme determinations of sorbitol dehydrogenase, isoenzyme 5 of lactate dehydrogenase, and aspartate transaminase activities. Creatinine kinase activity was evaluated as an indicator of muscle cell damage. Sorbitol dehydrogenase, isoenzyme 5 of lactate dehydrogenase, and aspartate transaminase activities were significantly (P less than 0.05) increased by 24 hours after carbon tetrachloride administration. Isoenzyme 5 of lactate dehydrogenase and sorbitol dehydrogenase activities returned to baseline several days before aspartate transaminase activity returned to baseline. Creatine kinase activity remained unchanged.     

Pathologic, hematologic, and serologic changes in rabbits given T-2 mycotoxin orally and exposed to aerosols of Aspergillus fumigatus conidia

The influence of immunosuppression by T-2 mycotoxin on the fungal disease aspergillosis was investigated in rabbits. Four groups of rabbits (groups 1A, 1B, 3A, and 3B) were given 0.5 mg of T-2 toxin/kg of body weight/day, PO; in addition, rabbits of groups 3A and 3B were exposed to aerosols of Aspergillus fumigatus conidia from days 7 through 16. Rabbits of groups 2A and 2B were exposed to A fumigatus aerosols, but were not given T-2 toxin, and rabbits of group 0 served as controls. Two rabbits of group 1A, 1 rabbit of group 1B, and 1 rabbit of group 3A died before scheduled necropsy. Rabbits of groups 1A, 2A, and 3A were killed and necropsied on day 17, and the remaining rabbits (groups 0, 1B, 2B, and 3B) were killed and necropsied on day 28. Changes caused by T-2 toxin included leukopenia, marginal anemia, and increased number of and morphologic changes in nucleated erythrocytes by day 21, followed by a regenerative hematologic response. Serum alkaline phosphatase and sorbitol dehydrogenase activities and antibody response to A fumigatus (as measured by an indirect hemagglutination test) were decreased by T-2 toxin ingestion. Rabbits with aspergillosis had leukocytosis, increased PCV, and increased antibody response to A fumigatus. Histologic lesions consisting of centrilobular hepatocellular swelling, portal and periportal fibrosis, and lymphocyte necrosis and/or depletion within secondary lymphoid tissue were observed in most rabbits treated with T-2 toxin. Normal defense mechanisms against A fumigatus infection were compromised by T-2 treatment, as evidenced by the severity and extent of lung lesions, greater number of hyphal elements observed, and greater number of colonies of A fumigatus isolated from rabbits of groups 3A and 3B. There were no significant changes in group-0 rabbits.     

Enhanced resistance to listeriosis induced in mice by preinoculation treatment with T-2 mycotoxin

The effect of T-2 toxin on cell-mediated resistance to bacterial infection was evaluated in mice challenge exposed with Listeria monocytogenes. Mice were treated orally on days -5, -4, -3, -2, -1, +1, and +3 with 2.0, 1.0, 0.5, or 0 mg of T-2 toxin/kg of body weight and were exposed to 10(6) (LD100) or 10(5) (LD50) L monocytogenes by intraperitoneal injection on day 0. Necrosis and depletion of lymphocytes in the thymus and spleen, decrease in thymus weight, reductions in the number of circulating total leukocytes and lymphocytes, and necrotizing gastroenteritis occurred in the toxin-treated mice. Although the cytotoxic effect of T-2 toxin on lymphoid tissue was marked, enhanced resistance to Listeria infection was revealed by significant (P less than 0.01) decreases in mortality caused by listeriosis in the toxin-treated mice. Mortality decreased from 100% to 64% in the mice exposed to 10(6) Listeria and from 50% to 20% in the mice exposed to 10(5) Listeria. Percentage of mortality after Listeria challenge exposure was dependent on the T-2 toxin dose and was progressively decreased in the mice given 0.5, 1.0, or 2.0 mg of toxin/kg.     

Effect of fusarium T-2 toxin on hematological and biochemical parameters in the rabbit.

The single intravenous administration of purified T-2 toxin to rabbits to 0.5 mg per kg body weight produced a decrease in hematocrit, while blood cell count, and serum alkaline phosphatase activity. The plasma clotting time, as measured by the activated partial thromboplastin time assay, was prolonged after intravenous T-2 toxin administration. In contrast, the administration of T-2 toxin to rabbits at 2.0 mg per kg body weight by gastric intubation produced oral lesions, diarrhea and anorexia in the animals but did not cause significant alteration in hematological and biochemical parameters. The results suggest that the rabbit may be a suitable model for further examination of the biochemical mechanisms involved in the cytotoxic action of T-2 toxin.     

Immunotoxic effects of T-2 mycotoxin on cell-mediated resistance to Listeria monocytogenes infection

The effect of T-2 toxin on cell-mediated resistance to bacterial infection was evaluated in mice exposed to Listeria monocytogenes. Mice were inoculated with 4.0 X 10(5) (LD50) or 4.0 X 10(4) (nonlethal) L. monocytogenes on day 0 and treated orally on days 0, 1, 2, and 3 with 2.0, 1.0, or 0 mg/kg T-2 toxin. Toxin induced suppression of resistance was indicated by the rapid growth of Listeria in the spleen and by significant (P less than 0.005) increases in mortality due to listeriosis. Necrosis and depletion of lymphoid tissue, lymphopenia, and a marked decrease in the influx of lymphocytes and macrophages into Listeria elicited peritoneal exudates and at sites of infection in the liver and spleen occurred in the toxin treated mice. The immunotoxic effect of T-2 toxin on cell-mediated resistance to listeriosis was dosage dependent and attributed to toxin induced lymphoid depletion and the failure of surviving lymphocytes and mononuclear cells to clear the host of infection.     

Experimental T-2 toxicosis in sheep.

Lambs received T-2 toxin at a rate of 0.6 or 0.3 mg/kg body weight per day in a protein reduced diet for 21 days to study the immunological and pathological effects of T-2 toxin in sheep. Blood was collected before T-2 treatment and on days 7, 14 and 21 of the trial for hematological and biochemical examination and for the separation of peripheral blood lymphocytes for the mitogen assay. Myeloid:erythroid ratios were determined from sternal bone marrow samples taken a day before T-2 treatment began, on day 12 and at death (day 22). Lambs treated with 0.6 mg/kg body weight of T-2 toxin daily were leukopenic on day 7 and lymphopenic on days 7 and 14. Also, on day 7, the mitogenic responses of these lambs to the B-cell mitogen, lipopolysaccharide, were significantly depressed and prothrombin times were prolonged. At necropsy, lymphoid atrophy of mesenteric lymph nodes and spleens was most marked in lambs treated with 0.6 mg/kg body weight of T-2 toxin per day. To the authors' knowledge, this is the first report of leukopenia, lymphopenia and lymphoid depletion in ruminants fed T-2 toxin.     

饲粮营养水平对妊娠及泌乳獭兔繁殖性能、血清生化指标及生殖激素的影响

本文旨在探讨饲粮营养［消化能（ＤＥ）＋粗蛋白质（ＣＰ）］水平对妊娠及泌乳獭兔繁殖性能、血清生化指标及生殖激素的影响。选用平均体重为（４．７３±０．４２）ｋｇ的经产母獭兔 １００只,随机分成 ５组（每组 ２０个重复,每个重复 １只）,分别饲喂 １０．５ＭＪ／ｋｇＤＥ＋１８％ ＣＰ、１０．５ＭＪ／ｋｇＤＥ＋１６％ ＣＰ、１０．０ＭＪ／ｋｇＤＥ＋１７％ ＣＰ、９．５ＭＪ／ｋｇＤＥ＋１８％ ＣＰ、９．５ＭＪ／ｋｇＤＥ＋１６％ ＣＰ的试验饲粮。试验从母兔配种开始至仔兔 ４５日龄结束。结果表明：饲粮营养水平除显著影响断奶窝重（Ｐ＝０．０３６５）外,对妊娠及泌乳獭兔其他繁殖性能指标无显著影响（Ｐ＞０．０５）;饲粮营养水平显著影响妊娠獭兔血清谷草转氨酶活性（Ｐ＝０．０４３９）以及胆固醇（Ｐ＝０．０４７８）、高密度脂蛋白胆固醇（Ｐ＝０．０２５６）、低密度脂蛋白胆固醇含量（Ｐ＝０．０２４８）;妊娠獭兔血清生殖激素未受饲粮营养水平的影响（Ｐ＞０．０５）;饲粮营养水平显著影响泌乳獭兔血清总蛋白（Ｐ＝０．０３６９）、尿素氮（Ｐ＝０．０４７３）、胆固醇含量（Ｐ＝０．０２３２）;除血清促黄体生成素外,泌乳獭兔血清其他生殖激素均未受饲粮营养水平的影响（Ｐ＞０．０５）。由此得出,饲粮ＣＰ水平在 １６％ ～１８％、ＤＥ水平在 ９．５～１０．５ＭＪ／ｋｇ范围内变动时,饲粮营养水平对妊娠及泌乳獭兔繁殖性能、血清生殖激素基本无影响,但会影响部分血清生化指标。     

Effects of treatment of growing swine with aflatoxin and T-2 toxin

Effects of dietary aflatoxin (AF) and T-2 toxin, singly and in combination, were evaluated in growing crossbred (Yorkshire x Landrace x Hampshire) pigs. The experimental design consisted of 4 treatment groups of 6 barrows each fed diets containing 0 mg of AF and T-2/kg of feed (controls; group 1), 2.5 mg of AF/kg of feed (group 2), 10 mg of T-2/kg of feed (group 3), or 2.5 mg of AF plus 10 mg of T-2/kg of feed (AF + T-2; group 4) ad libitum for 28 days (7 to 11 weeks of age). Production performance, and serum biochemical, and hematologic evaluations were made weekly. Body weight and body weight gain were depressed by all toxin treatments, but the effect of AF and T-2 toxin in combination was less than additive. Liver and kidney weights, as a percentage of body weight, were increased by AF treatment, and heart weight, as a percentage of body weight, was increased by T-2 treatment. Treatment with T-2 toxin induced necrotizing contact dermatitis on the snout, buccal commissures, and prepuce. Consumption of AF resulted in increased serum activities of alkaline phosphatase, aspartate transaminase, cholinesterase, and gamma-glutamyltransferase, and decreased serum concentrations of urea nitrogen, cholesterol, albumin, total protein, calcium, potassium, magnesium, and phosphorus. Consumption of T-2 toxin resulted in increased serum triglyceride concentration and decreased serum iron concentration. Treatment with AF induced lower serum unsaturated iron-binding capacity and high RBC count, PCV, hemoglobin concentration, WBC count, and prothrombin time.(ABSTRACT TRUNCATED AT 250 WORDS)     

精氨酸在体内和体外试验中对鲤鱼免疫力的影响

本试验采用体外和体内2种方法来研究精氨酸(Arg)对鲤鱼免疫力的影响。体外试验中,在培养基中分别添加0、0.5、1.0、1.5和2.0mmol/L的Arg,将肾脏白细胞培养不同的时间段后测定增殖指数、呼吸爆发活力、吞噬活力和杀菌率。体内试验中,将平均体重37g的鲤鱼随机分为5组,每组3个重复,每个重复10条,分别体内注射0、25、50、100和200 mg/kg鱼体重的Arg,商业饲料投喂2周,进行肾脏白细胞增殖指数、呼吸爆发活力和吞噬活力的测定,以及血清和肝胰脏一氧化氮(NO)含量、一氧化氮合成酶(NOS)活性及血清白蛋白(ALB)含量的测定。体外试验结果表明:添加Arg能够提高肾脏白细胞的增殖指数、呼吸爆发活力、吞噬活力和杀菌率。培养12和24h后,1.0、1.5和2.0mmol/L Arg组肾脏白细胞增殖指数显著高于0mmol/L Arg组(P0.05);培养6、12和24h后,1.0mmol/L Arg组肾脏白细胞呼吸爆发活力显著高于0mmol/L Arg组(P0.05);培养12和24h后,1.0、1.5和2.0mmol/L Arg组肾脏白细胞吞噬活力显著高于0mmol/L Arg组(P0.05);培养18h后,1.0、1.5和2.0 mmol/L Arg组肾脏白细胞杀菌率显著高于0 mmol/L Arg组(P0.05)。体内试验结果表明:50、100和200 mg/kg Arg组肾脏白细胞呼吸爆发活力、吞噬活力和增殖指数显著高于0mg/kg Arg组(P0.05);100和200mg/kg Arg组血清ALB和NO含量显著高于0 mg/kg Arg组(P0.05),50、100和200mg/kg Arg组血清NOS活性显著高于0mg/kg Arg组(P0.05);50、100和200mg/kg Arg组肝胰脏NO含量显著高于0mg/kg Arg组(P0.05),25和50mg/kg Arg组肝胰脏NOS活性显著高于0mg/kg Arg组(P0.05)。由此可见,Arg提高了鲤鱼肾脏白细胞的免疫力,体外试验表明Arg的适宜浓度为1.0mmol/L。正常摄食情况下,Arg在鲤鱼体内注射适宜浓度为50~100mg/kg。     

饲粮中核黄素添加水平对生长獭兔肉品质、毛囊发育和免疫性能的影响

本试验旨在研究饲粮中核黄素添加水平对生长獭兔肉品质、毛囊发育和免疫性能的影响。选择体重相近的3月龄獭兔160只,随机分为4组,每组40个重复,每个重复1只兔。各组分别饲喂在基础饲粮中添加0(对照)、3、6和12 mg/kg核黄素的饲粮。预试期7 d,正试期53 d。结果表明:与对照组相比,饲粮中添加6、12 mg/kg核黄素显著降低了獭兔肌肉的滴水损失(P0.05),饲粮中添加3、6、12 mg/kg核黄素显著提高了獭兔皮肤中总毛囊密度(P0.05),饲粮中添加3、6 mg/kg核黄素显著提高了獭兔皮肤中初级毛囊密度(P0.05),饲粮中添加6、12 mg/kg核黄素显著提高了獭兔皮肤中次级毛囊密度(P0.05),饲粮中添加3、6 mg/kg核黄素显著降低了獭兔皮肤中次级毛囊密度/初级毛囊密度(P0.05)。饲粮中核黄素添加水平对獭兔的胸腺重、胸腺指数及血清免疫球蛋白G、免疫球蛋白A、白细胞介素-2含量影响显著(P0.05),且均随着饲粮中核黄素添加水平的升高呈先增加后降低的趋势,并均在6 mg/kg添加组中达到最大值,显著高于对照组(P0.05)。由此可见,3~5月龄生长獭兔饲粮中核黄素适宜添加水平为6 mg/kg(实际测定饲粮中核黄素水平为8.35 mg/kg)。     

Effect of sodium bicarbonate infusion on serum osmolality, electrolyte concentrations, and blood gas tensions in cats.

The effects of single IV injections of sodium bicarbonate (0.5 mEq/kg of body weight, 1 mEq/kg, 2 mEq/kg, and 4 mEq/kg) on serum osmolality, serum sodium, chloride, and potassium concentrations, and venous blood gas tensions in 6 healthy cats were monitored for 180 minutes. Serum osmolality increased and remained significantly (P less than 0.05) increased for 120 minutes in cats given 4 mEq of sodium bicarbonate/kg. Serum sodium was increased significantly (P less than 0.05) for 30 minutes in cats given 4 mEq of sodium bicarbonate/kg. Serum sodium decreased and remained significantly (P less than 0.05) decreased for 120 minutes in cats given 1 g of 20% mannitol/kg, and serum osmolality was significantly (P less than 0.05) decreased at 30 and 60 minutes. Serum chloride decreased significantly (P less than 0.05) for 10 minutes in cats given 1 mEq of sodium bicarbonate/kg, and was significantly decreased for 30 minutes in cats given 2 mEq and 4 mEq of sodium bicarbonate/kg. Serum chloride decreased and remained significantly (P less than 0.05) decreased for 30 minutes in cats given 1 g of 20% mannitol/kg. Serum sodium and serum osmolality did not change significantly (P less than 0.05) in cats given 4 ml of 0.9% sodium chloride/kg. Serum potassium decreased significantly (P less than 0.05) for 10 minutes in cats given 1 mEq of sodium bicarbonate/kg, and for 120 minutes in cats given 2 mEq/kg or 4 mEq/kg. There was a significantly (P less than 0.05) greater decrease in serum potassium that lasted for 30 minutes after given sodium bicarbonate at the dosage of 4 mEq/kg, compared with other dosages given.(ABSTRACT TRUNCATED AT 250 WORDS)     

Hematologic and serum biochemical effects of long-term administration of anti-inflammatory doses of prednisone in dogs.

Results of routine hematologic and serum biochemical analyses from 12 healthy adult male dogs that were given prednisone (0.55 mg/kg of body weight, PO, q 12 h) for 35 days were compared with those of a control group of 6 dogs that were given gelatin capsules. Analyses were performed at 2-week intervals during and after prednisone administration. Lymphocyte and eosinophil counts were significantly (P less than 0.005) decreased after 2 and 4 weeks of prednisone treatment, compared with controls. Two weeks after treatment, eosinophil counts in prednisone-treated dogs were similar to those of control dogs, whereas lymphocyte counts remained low 4 weeks after treatment in treated dogs (1,869 +/- 145 cells/microliters), compared with that in control dogs (3,662 +/- 548 cells/microliters). Neutrophil and monocyte counts did not significantly change during glucocorticoid administration. Mean platelet volume significantly (P less than 0.001) decreased after 4 weeks of prednisone treatment, but returned to pretreatment values by 2 weeks after treatment. Four weeks of prednisone treatment did not cause significant increased activity in serum alanine transaminase, total alkaline phosphatase or the steroid-induced isoenzyme of alkaline phosphatase. Significant increases in serum albumin (P less than 0.001) and total protein (P less than 0.05) concentrations were detected after 4 weeks of treatment, but mean values were not significantly different from those of controls 2 weeks after treatment ended. Results of our study indicate that eosinophil and lymphocyte counts are the most sensitive indicators of long-term glucocorticoid administration at anti-inflammatory dosages of 1.1 mg/kg daily.     

Evaluation of lasalocid as a coccidiostat in calves: titration, efficacy, and comparison with monensin and decoquinate

Two experiments were conducted to evaluate lasalocid as a coccidiostat in Holstein calves and to compare lasalocid with monensin and decoquinate. In experiment 1, calves in 3 groups (6 calves/group) were each inoculated with 500,000 sporulated oocysts, 88% of which were Eimeria bovis and 12% were E zuernii. Calves in each group were given lasalocid-medicated feed at 0.50 (group 3), 0.75 (group 4), or 1 mg/kg (group 5) of body weight/day for 45 days. Two control groups (6 calves/group) were also evaluated; calves in control group 2 were inoculated and nontreated, and calves in control group 1 were noninoculated and nontreated. At 0.50, 0.75, or 1 mg/kg/day, lasalocid was equally effective in preventing induced coccidiosis (E bovis and E zuernii) in calves. Compared with inoculated nontreated controls, treated calves had significantly (P less than 0.05) fewer oocysts in feces and had fewer clinical signs of coccidiosis from days 16 to 30 after inoculation. Experiment 2 was conducted to compare the effectiveness of monensin, lasalocid, and decoquinate for the prevention of experimentally induced coccidiosis. Calves (n = 48) were allotted into 4 groups (12 calves/group); each was inoculated orally with 275,000 sporulated oocysts, predominantly E bovis and E zuernii, and each was given nonmedicated feed (group 6) or feed medicated with 33 mg of lasalocid (group 7), decoquinate (group 8), or monensin (group 9)/kg of feed for 46 days. Calves given medicated rations had significantly (P less than 0.05) fewer oocysts in their feces and fewer clinical signs of coccidiosis than did calves given nonmedicated rations.(ABSTRACT TRUNCATED AT 250 WORDS)     

Adverse effects of gentamicin in scarlet macaws and galahs

The adverse effects of administration of gentamicin (5 mg/kg of body weight, IM, q 12 h) for 7 days were studied in healthy scarlet macaws (Ara macao) and galahs (Eolophus roseicapillus; cockatoos). Polydipsia and polyuria developed in each species, but were greater and persisted longer in the cockatoos. Peak water intake in the cockatoos more than quadrupled, and remained increased for 23 days after cessation of gentamicin administration. Plasma aspartate transaminase activity increased significantly (P less than 0.05) after treatment in the macaws, and plasma aspartate transaminase and lactate dehydrogenase activities increased in the cockatoos. Single IM administration of gentamicin (5 mg/kg) resulted in mean (+/- SEM) plasma concentration of 20.6 (+/- 1.85) micrograms/ml at 0.5 hour for either species of birds. There were no significant differences between mean plasma gentamicin concentrations for cockatoos and macaws at any time after drug administration, except at 12 hours, when values for cockatoos were significantly (P less than 0.05) greater than those for macaws. The elimination half-life for gentamicin after IM administration of 5 and 10 mg/kg was 1.17 and 1.07 hours, respectively, for macaws and 1.23 and 1.44 hours, respectively, for cockatoos. Correlation between drug disposition and adverse side effects could not be detected.     

乳酸锌对断奶肉兔生长性能、肠道发育和血清生化指标的影响

本试验旨在研究饲粮中添加乳酸锌对断奶肉兔生长性能、肠道发育和血清生化指标的影响.选择28日龄同期断奶新西兰兔420只,随机分为5组:对照组(饲喂基础饲粮,饲粮中添加硫酸锌形式的锌0 mg/kg)、硫酸锌组(在基础饲粮中添加硫酸锌形式的锌80 mg/kg)以及3个乳酸锌组(在基础饲粮中分别添加乳酸锌形式的锌20、40、8...     

Prevention of coccidiosis in domestic dogs and captive coyotes (Canis latrans) with sulfadimethoxine-ormetoprim combination

Sulfadimethoxine-ormetoprim combination was evaluated as a coccidiostat against experimentally induced coccidiosis in young dogs and coyotes (Canis latrans). The animals were experimentally inoculated with 50,000 or 100,000 sporulated oocysts of Isospora ohiohensis (98%) and Isospora canis (2%). In experiment 1, daily treatment for 13 to 23 days with a combination of 27.5 mg of sulfadimethoxine/kg of body weight (BW) and 5.5 mg of ormetoprim/kg of BW admixed to the feed resulted in no significant (P greater than 0.05) difference in fecal oocyst counts between treated and nontreated groups of dogs or coyotes. In experiment 2, treatment with a combination of 55 mg of sulfadimethoxine/kg of BW and 11 mg of ormetoprim/kg of BW for 23 days was 99.8% effective against Isospora spp infections in dogs. Significantly (P less than 0.05) fewer oocysts were present in feces of treated dogs than were present in feces of nontreated dogs from first passage of oocysts at day 4 to the end of the patent period at days 19 to 21. After the 2nd week of treatment, BW of treated dogs were significantly greater (P less than 0.05) than BW of nontreated dogs. Evidence of drug toxicity was not observed clinically or by serum chemical analyses.