饲喂不同浓度黄曲霉毒素B1饲料对花鳗鲡幼鱼生长、抗氧化能力和毒素积累的影响

以含不同浓度黄曲霉毒素B₁(AFB₁) (0、10、100和1000 μg/kg饲料)的4种饲料饲喂平均初始体重为(6.41±0.10) g的花鳗鲡(Anguilla marmorata)幼鱼56d, 探讨AFB₁对花鳗鲡幼鱼生长性能、抗氧化能力、肝脏组织结构及鱼体肌肉中的毒素积累的影响。结果表明, 各实验组幼鱼均未表现出行为及体色的异常。1000 μg/kg毒素组幼鱼的存活率、终末体重、摄食率、特定生长率和饲料效率显著低于对照组, 10 μg/kg毒素组和100 μg/kg毒素组与对照组无显著差异。10 μg/kg毒素组幼鱼肝脏超氧化物歧化酶(SOD)、过氧化氢酶(CAT)、谷胱甘肽过氧化物酶(GSH-Px)、谷胱甘肽S转移酶(GST)活性和丙二醛(MDA)含量与对照组无显著差异。饲料AFB₁含量≥100 μg/kg显著影响花鳗鲡幼鱼肝脏的超氧化物歧化酶(SOD)、谷胱甘肽过氧化物酶(GSH-Px)和谷胱甘肽转移酶(GST)活性。对照组和10 μg/kg毒素组幼鱼肝脏组织学观察未发现明显病理变化。1000 μg/kg毒素组幼鱼的肝脏细胞表现出严重的空泡化。随着饲料AFB₁水平的升高, 幼鱼肝脏和肌肉中AFB₁积累量均显著升高。1000 μg/kg毒素组幼鱼肝脏和肌肉中AFB₁积累量分别为17.75和5.98 μg/kg, 均超过FDA食品安全限定标准(5 μg/kg)。由此可见, 饲料中AFB₁≤10 μg/kg对花鳗鲡幼鱼是相对安全的浓度。     

饲喂不同浓度黄曲霉毒素B1饲料对草鱼幼鱼生长和毒素积累的影响

以含不同浓度黄曲霉毒素B₁(AFB₁)(0、10、20、100、1000和5000 μg/kg饲料)的6种等氮等能(32.96%蛋白质, 14.55 kJ/g能量)配合饲料饲喂平均初始体质量为(2.90±0.16) g草鱼(Ctenopharyngodon idellus)幼鱼84d, 探讨AFB₁对草鱼幼鱼生长、肝胰脏和肾脏组织结构以及鱼体肌肉中的毒素积累的影响。实验分为6个实验组, 每组3个平行。结果表明, 在整个实验过程中各实验组幼鱼的行为均未表现出异常, 各组幼鱼的存活率、终末体重、摄食率、特定生长率、饲料效率、肝体比、脏体比均无显著差异。饲料AFB₁水平对草鱼幼鱼血清谷丙转氨酶(ALT)、谷草转氨酶(AST)、碱性磷酸酶(AKP)、超氧化物岐化酶(SOD)和谷胱甘肽过氧化物酶(GSH-Px)活性均无显著影响。各毒素组和对照组肝胰脏、肾脏组织学观察中未发现病理变化。摄食AFB₁≤1000 μg/kg的草鱼幼鱼肌肉中未检测出AFB₁残留, 仅在5000 μg/kg实验组中检测出肌肉中含有(1.21±0.18) μg/kg的AFB₁, 低于FDA食品安全限定标准。由此可见, 草鱼幼鱼至少可耐受AFB₁含量达5000 μg/kg饲料(实测值: 4979.2 μg/kg饲料) 84d。     

饲喂不同浓度黄曲霉毒素B1饲料对异育银鲫成鱼的生长和毒素积累的影响

以含不同浓度黄曲霉毒素B1(AFB1)的配合饲料饲喂异育银鲫(Carassius auratus gibelio)成鱼56d,研究异育银鲫成鱼[(122.3±0.7)g]生长、生理反应、肝脏组织学变化、卵巢发育以及鱼体各组织中的AFB1的毒素积累状况。实验分为5个实验组,不同实验组饲料中AFB1含量分别为0、5、20、50、500μg/kg饲料(实测值分别为2.59、4.12、12.39、46.23、454.07μg/kg饲料),每个处理3个平行。在整个实验过程中各实验组均未表现出外部形态和行为异常,各组存活率均达到100%。各实验组异育银鲫成鱼终末体重、摄食率(FR)、特定生长率(SGR)和饲料效率(FE)均无显著差异。饲料AFB1水平对异育银鲫血清总胆固醇(TC)含量、血清谷丙转氨酶(GPT)、谷草转氨酶(GOT)和碱性磷酸酶(AKP)活性均无显著影响。各毒素组血清超氧化物岐化酶(SOD)活性与对照无显著差异。各毒素组肝脏和卵巢均未见明显的组织学病理变化。肌肉和性腺中的AFB1积累量低于FDA食品安全限定标准(5μg/kg)。肝胰脏中的AFB1积累和饲料中的AFB1水平呈对数关系。饲喂AFB1≥50μg/kg饲料使异育银鲫成鱼肝脏AFB1积累超过安全限量标准。结果表明,异育银鲫成鱼至少可耐受AFB1含量达500μg/kg饲料(实测值:454.07μg/kg饲料)56d。     

日本沼虾MT基因克隆、组织差异性表达及与饲料铜、锌含量的相关性

为了更全面理解日本沼虾(Macrobrachium nipponense)的铜/锌营养生理作用,研究利用RACE技术从日本沼虾肝胰腺中克隆获得一金属硫蛋白基因cDNA全长(mn-MT),并对该基因分子特征、组织表达谱和饲料铜/锌水平对其表达的影响进行分析。结果显示:(1)mn-MT cDNA全长665 bp,含编码59个氨基酸的180 bp的开放阅读框,预测该多肽的理论分子量为6.085 kD,等电点为7.73。该蛋白中半胱氨酸含量最高(30.5%),其次是赖氨酸(16.95%)和丝氨酸(10.17%)。相似性分析显示mn-MT氨基酸序列与美洲海螯虾、斑节对虾和中华绒螯蟹MT的相似性分别达到78%、75%和75%。(2)qRT-PCR分析显示, mn-MT mRNA在肝胰腺、血细胞、鳃、胃、卵巢、肠和肌肉中都有表达,其中肝胰腺中表达量最高。(3)用4组铜添加量分别为0、20、40及160 mg/kg的饲料和3组锌添加水平分别为0、35和210 mg/kg的饲料饲喂初重为(0.1010.002) g日本沼虾56d后,分析各组虾肝胰腺的mn-MT mRNA表达。mn-MT mRNA表达随饲料铜水平的提高而升高,到40 mg/kg组达到最高(P0.05),而后开始下降;饲料中高锌(210 mg/kg)显著提高mn-MT表达(P0.05), 0和35 mg/kg组间差异不显著(P0.05)。结果表明饲料中铜/锌均可影响mn-MT表达,且呈现不同的剂量依赖效应。       

急性低氧/复氧胁迫对克氏原螯虾抗氧化-能量代谢的影响

为研究低氧/复氧胁迫对克氏原螯虾(Procambarus clarkii)抗氧化及能量代谢的影响,将克氏原螯虾暴露于(1.0±0.1) mg/L急性低氧胁迫和后续(6.8±0.2) mg/L复氧环境中,于低氧胁迫1h、6h及复氧1h、12h分别采集肝胰腺、鳃和血淋巴,研究低氧/复氧胁迫下克氏原螯虾抗氧化-能量代谢酶的活力变化,分析鳃和肝胰腺组织的超微结构改变。在低氧胁迫下,肝胰腺和血淋巴中SOD酶活力显著下降(P<0.05);复氧以后,肝胰腺、血淋巴及鳃组织中SOD酶活力均出现了显著上升(P<0.05)。SOD酶活力变化可能与复氧过程中超氧阴离子自由基的过量产生有关。在复氧12h后,血淋巴和鳃组织中MDA含量均出现了显著性增加(P<0.01),提示机体细胞在复氧胁迫下产生了脂质过氧化。在低氧胁迫下,肝胰腺、鳃和血淋巴中ACP、AKP酶活力显著上升(P<0.05);在复氧12h后,肝胰腺和鳃组织中ACP酶活力显著降低(P<0.01)。显示低氧/复氧胁迫影响了机体的非特异性免疫应答。在急性低氧胁迫下,肝胰腺、血淋巴与鳃组织中的LDH含量和总ATPase活力均显...     

饲料中添加合成虾青素对中华绒螯蟹成体雌蟹性腺发育、色泽和抗氧化能力的影响

采用在基础饲料中分别添加0、130和260 mg/kg的合成虾青素配制成3种粗蛋白和粗脂肪含量分别为42%和16%的等氮等脂的中华绒螯蟹(Eriocheir sinensis)育肥饲料(分别记为饲料1、2和3), 以中华绒螯蟹商业育肥饲料作为饲料4, 分别投喂4组雌蟹(每个饲料组3个重复水槽, 每个水槽中12只蟹), 进行为期60d的室内养殖实验, 以探讨添加合成虾青素对中华绒螯蟹成体雌蟹性腺发育、色泽及抗氧化能力的影响。结果显示: (1)实验进行到30d和60d, 在饲料中添加虾青素对雌体肝胰腺指数(HSI)和性腺指数(GSI)均无显著影响(P>0.05)。(2)性腺、肝胰腺和头胸甲中的总类胡萝卜素含量和红度值(a值)均以饲料3组最高, 性腺亮度值(L值)和黄度值(b值)以饲料1组最高(P<0.05); 饲料2组头胸甲的b值最高, 饲料1组最低(P<0.05)。(3) 饲料1组中华绒螯蟹血清过氧化物酶(POD)活性显著高于其他组, 饲料4组的过氧化氢酶(CAT)、谷胱甘肽还原酶(GR)、乳酸脱氢酶(LDH)、总抗氧化能力(T-AOC)、丙二醛(MDA)和乳酸(LD)含量最高(P<0.05); 肝胰腺中的SOD、T-AOC、GSH-Px和GR活性均以饲料1组最高, 饲料2组最低(P<0.05)。(4) 饲料2组血清酸性磷酸酶(ACP)活性和血蓝蛋白(Hc)含量显著高于其他组, 其余各组间差异不显著。血清中的碱性磷酸酶(ALP)和γ-谷氨酰转移酶(γ-GT)活性和一氧化氮(NO)含量均以饲料4组最高(P<0.05), 肝胰腺中的ACP、ALP和γ-GT活性以饲料1组最高。综上, 在育肥饲料中添加合成虾青素对成体雌蟹性腺发育无显著影响, 但可显著提高头胸甲、肝胰腺和卵巢中的类胡萝卜素总量、色泽和抗氧化能力, 建议雌蟹育肥饲料中合成虾青素的含量为90 mg/kg左右。     

稻虾田黄鳝的食物组成及其对克氏原螯虾捕食强度研究

文章研究了稻田黄鳝(Monopterus albus)天然饵料生物资源、稻田黄鳝对克氏原螯虾(Procambarus clarkii)捕食选择及不同投喂策略下黄鳝对克氏原螯虾的捕食强度,旨在为构建与优化稻-虾-鳝综合种养模式提供依据。结果表明,稻田中黄鳝天然饵料生物种类丰富,达16种(属);克氏原螯虾是黄鳝最喜猎物,其次为米虾,再次为蚯蚓和水生寡毛类;稻田黄鳝自然生长期间,其胃和肠前端食物团中,克氏原螯虾重量百分比均显著高于其他猎物,其中8月份占比最大,达93.90%, 4月份占比最小,为76.85%;当克氏原螯虾为唯一食物时,每尾大规格成鳝(≥200 g)日均捕食量为(1.63±0.065) g;当克氏原螯虾、米虾和蚯蚓作为食物时,黄鳝主要捕食克氏原螯虾且不捕食蚯蚓,对三者的选择指数分别为0.066、–0.266和–1;若以克氏原螯虾、鱼糜-饲料为食物时,黄鳝主要摄食鱼糜-饲料,极少捕食克氏原螯虾,对两者的选择指数分别为–0.846和0.591。     

植物蛋白替代鱼粉对克氏原螯虾生长和繁殖的影响

为了探究复合植物性蛋白(豆粕﹕菜粕=1﹕1)替代鱼粉对克氏原螯虾(Procambarus clarkii)生长以及繁殖性能的影响, 实验以豆粕和菜粕为植物性蛋白源配制了6组不同替代水平的等氮等能的饲料并选取其中替代水平较高的3组添加蛋氨酸和赖氨酸, 进行为期10周的养殖实验。实验结果表明: 随着饲料中植物蛋白水平的提高, 克氏原螯虾增重率和绝对繁殖力均显著下降(P<0.05)。与对照组相比, 添加适量的植物性蛋白(33.8%)能显著提高克氏原螯虾的生长性能的同时对其绝对繁殖力和性腺指数无明显影响(P<0.05)。此外, 在饲料中添加高水平的植物蛋白抑制克氏原螯虾的生长并且降低其繁殖能力, 而在饲料中补充赖氨酸和蛋氨酸可以很好地改善这一状况。另外, 尽管每组饲料的处理方式不同, 但是克氏原螯虾性腺指数与绝对繁殖力变化一致。     

基于纳米金和辣根过氧化物酶双标记抗体的黄曲霉毒素B1高灵敏检测方法的建立及应用

黄曲霉毒素B₁（aflatoxin B₁,AFB₁）在自然界普遍存在,可污染多种粮食作物和饲料,给动物和人类健康造成严重威胁。为建立AFB₁高灵敏度的快速检测方法,本研究通过采用纳米金颗粒（Au nanoparticles,AuNPs）和辣根过氧化物酶（horseradish peroxidase,HRP）双标记AFB₁单克隆抗体,建立新型酶联免疫检测方法（HRP-AuNPs IC-ELISA）,检测下限（IC₁₀）为0.017ng/mL,检测区间（IC₂₀-IC₈₀）为0.026-0.376ng/mL,半数抑制率（IC₅₀）为0.099ng/mL,与黄曲霉毒素B₂、G₁、G₂ 和M₁ 的交叉反应率分别为2.7%、9.3%、2.1%和5.3%,与赭曲霉毒素A、伏马毒素B₁、桔青霉素、展青霉毒素和玉米赤霉烯酮几乎不存在交叉反应。在玉米和面粉样本中的加标回收率可达88.93-103.55%,与LC-MS/MS同时对天然样本中AFB₁ 含量进行检测,结果表明,两种方法相关性良好。本研究建立的HRP-AuNPs IC-ELISA耗时短且灵敏度高,可用于实际样本中AFB₁ 的快速定量检测与分析,也为其他霉菌毒素的精准检测技术开发提供参考。     

两种绿藻辅助饲喂对克氏原螯虾生理活性的影响

以克氏原螯虾为研究对象, 测定了在正常投喂人工颗粒饲料的基础上辅助添加小球藻、刚毛藻饲喂克氏原螯虾的生理活性。结果表明: 试验期间添加小球藻(1.0×106-1.0×107 cells·L-1)、刚毛藻(0.06-0.08 g·L-1)对克氏原螯虾的生长与存活率均无显著影响(P >0.05), 但肌肉超氧化物歧化酶(SOD)和肝胰脏酸性磷酸酶(ACP)的活性显著降低(P <0.05); 机体的血细胞密度显著增加(P <0.05), 外骨骼和肌肉中虾青素的含量极显著增加(P <0.01); 单独添加刚毛藻肌肉虾青素含量也显著提高(P <0.05), 血清、肝胰脏和肌肉碱性磷酸酶(AKP)的活性极显著提高(P <0.01), 肝胰脏酸性磷酸酶的活性极显著降低(P <0.01)。摄食小球藻和刚毛藻对于克氏原螯虾的抗逆活性和免疫能力具有促进作用, 养殖水体中适度添加小球藻和刚毛藻有助于克氏原螯虾的健康与活力。     

Effects of oral administration of aflatoxin B1 and fumonisin B1 in rabbits (Oryctolagus cuniculus)

The effects of prolonged oral administration (21 days) of fumonisin B₁ (FB₁) and aflatoxin B₁ (AFB₁) were studied in male New Zealand rabbits by clinical, pathological, biochemical and sphingolipid analyses. Twenty-four animals were randomly divided into the following four experimental groups: (A) 0 mg FB₁ + 0 μg AFB₁/(kg body weight (bw) day) (control); (B) 0 mg FB₁ + 30 μg AFB₁/(kg bw day); (C) 1.5 mg FB₁/(kg bw day) + 30 μg AFB₁/(kg bw day); (D) 1.5 mg FB₁/(kg bw day) + 0 μg AFB₁. Animals from group B and principally from group C presented clinical signs of intoxication. Rabbits from group C presented a lower body weight gain than controls. Differences were observed between intoxicated rabbits and controls with respect to absolute and relative liver and kidney weight, hepatic function, serum urea and creatinine levels and Sa/So ratio. The most frequent hepatic and renal injuries were vacuolar degeneration of the liver and kidney as shown by the histopathological and serum biochemical results. Combined administration of AFB₁ and FB₁ resulted in synergistic toxic effects both in the liver and in the kidney, but hepatic injuries were more marked.     

Indirect competitive immunoassay for detection of aflatoxin B1 in corn and nut products using the array biosensor

Because of the potential health risks of aflatoxin B₁ (AFB₁), it is essential to monitor the level of this mycotoxin in a variety of foods. An indirect competitive immunoassay has been developed using the NRL array biosensor, offering rapid, sensitive detection and quantification of AFB₁ in buffer, corn and nut products. AFB₁-spiked foods were extracted with methanol and Cy5-anti-AFB₁ added to the resulting sample. The extracted sample/antibody mix was passed over a waveguide surface patterned with immobilized AFB₁. The resulting fluorescence signal decreased as the concentration of AFB₁ in the sample increased. The limit of detection for AFB₁ in buffer, 0.3 ng/ml, was found to increase to between 1.5 and 5.1 ng/g and 0.6 and 1.4 ng/g when measured in various corn and nut products, respectively.     

南昌市空气PM2.5和PM10的时空动态及其影响因素

PM_2.5和PM₁₀已成为我国大部分城市空气的首要污染物.本文通过分析南昌市2013—2015年的空气PM_2.5和PM₁₀质量浓度、气象因素、交通流量的监测数据,探讨了空气颗粒物污染的时空动态规律以及气象、交通对颗粒物浓度变化的影响.结果表明: 2013、2014、2015年,南昌市PM_2.5浓度(70.92 μg·m^-3＞53.70 μg·m^-3＞43.65 μg·m^-3)、PM₁₀浓度(119.72 μg·m^-3＞86.11 μg·m^-3＞73.32 μg·m^-3)逐年降低,并呈现出夏季低(PM_2.5和PM₁₀平均浓度分别为36.74、69.20 μg·m^-3)、冬季高(PM_2.5和PM₁₀平均浓度分别为74.29、111.64 μg·m^-3)的季节动态和由城市中心向郊区递减的城乡梯度变化; PM_2.5/PM₁₀值(0.595＞0.584＞0.557)逐年降低,并且表现出城市中心高、城市边缘低的空间分布格局;PM_2.5、PM₁₀浓度受到多种气象因素的影响,与气压、温度、相对湿度、风速、降水量、日照时数显著相关,各种气象因子对PM_2.5、PM₁₀浓度的影响存在差异;车流量会显著提高周边PM_2.5浓度,但对PM₁₀浓度影响不明显.     

Effect of Salvia miltiorrhiza on aflatoxin B1-induced oxidative stress in cultured rat hepatocytes

Recent findings have suggested that oxidative damage might contribute to the cytotoxicity and carcinogenicity of aflatoxin B₁ (AFB₁). Salvia miltiorrhiza (Sm), a herbal plant that has been used extensively in traditional Chinese medicine for treating cardiovascular and liver diseases, is believed to have some antioxidative capabilities. In this study, the protective effect of Sm against AFB₁-induced cytotoxicity was investigated in cultured primary rat hepatocytes. AFB₁-induced cytotoxicity and lipid peroxidation (LPO) were estimated by determination of lactate dehydrogenase (LDH) leakage and thiobarbituric acid reactive substances (TBARS) formation, respectively. Intracellular reactive oxygen species (ROS) formation was measured using a fluorescent probe 2',7'-dichlorofluorescein diacetate (DCFH-DA). In addition, changes of intracellular glutathione (GSH) content were also studied. Results showed that Sm was able to suppress the LDH leakage induced by AFB₁ in a dose-dependent manner. A dose-dependent inhibitory effect of Sm on AFB₁-induced LPO was also found in hepatocytes treated with Sm. It was further observed that Sm produced an inhibitory effect on ROS formation caused by AFB₁. Concomitantly, the GSH content in Sm-treated groups increased substantially compared to those without Sm treatment. These findings suggest that Sm can inhibit the cytotoxicity of AFB₁ through decreasing ROS formation, inhibiting LPO and preventing GSH depletion. The major component of the aqueous extract of Sm was identified by using high performance liquid chromatography (HPLC), proton magnetic resonance (¹H-NMR) and mass spectrum (MS). Analytical results suggested that D(+)β3,4-dihydroxyphenol lactic acid (DA) is the main compound of the aqueous extract of Sm.     

Potentiation of bradykinin-induced vascular permeability increase by prostaglandin E2 and arachidonic acid in rabbit skin

The activity of prostaglandins (PG) in producing vascular permeability was quantitated by dye extraction method in skin of anaesthetized rabbits. PGE₁ and PGE₂ (0.01–10 μg) produced increase in vascular permeability. Activity was approximately equal to that of histamine (Hist) and 1/20 of that of bradykinin (BK) on a weight basis. The activity of PGF₁ and PGF₂ was only 1/20 of that of PGE₁ or PGE₂.

In spite of the relatively low potency of PGE₁ and PGE₂ in the rabbit, near threshold doses (0.1 or 1 μg) of PGE₂ could potentiate permeability responses to bradykinin (0.1 μg) by 10 or 100-fold, respectively. Equivalent doses (0.1 or 1 μg) of histamine could not potentiate the bradykinin responses. Arachidonic acid (AA) at 1 μg, produced a 10-fold potentiation in the permeability response to bradykinin (0.1 μg). Pretreatment of the rabbits with indomethacin (20 mg/kg, i.p.) reduced the responses of BK (0.1 μg) + AA (1 μg) down to a similar magnitude of those seen with bradykinin alone. However, indomethacin did not block responses to either, BK alone, BK + PGE₂, or BK + Hist. Various doses (1, 10, 100 and 300 μg) of arachidonic acid alone also produced increase in cutaneous vascular permeability, although its potency was only 1/3–1/8 of that of PGE₂. This activity of arachidonic acid was attributed in part to its bioconversion to PGE₂, since its activity was significantly reduced by the prostaglandin antagonist, diphloretin phosphate (DPP) (60 mg/kg, i.v.) and by indomethacin (20 mg/kg, i.p.), which blocks conversion of arachidonic acid to prostaglandins. Arachidonic acid may owe some of its permeability increaseing effects to histamine release, since its effects were also reduced by the anti-histamine, pyrilamine (2.5 mg/kg, i.v.).