抗附红细胞体有效药物的筛选

以PCR检测附红细胞体呈现阳性，且镜检染虫率达909／5以上的猪血样为研究对象，选择几种附红细胞体敏感的药物(血虫净，附红净，庆大霉素，博士914，土霉素，三毒清，红弓链914，附红120，红弓链克，乌金土霉素)和对支原体敏感的恩诺沙星，对立克次氏体敏感的红霉素，采用两种方法进行体外药效试验。附红净对附红细胞体的作用效果最明显，而庆大霉素对附红细胞体基本无效，其他药物对附红细胞体也有一定杀灭效果。     

微卫星与金华猪生长性状关系的研究

采用微卫星标记多重扩增结合荧光标记检测技术,对152头金华猪种群的30个微卫星位点的不同基因型与生长发育性状的关系进行了初步分析和显著性检测。结果显示SW 2476、SW 0215、SW 24等3个微卫星位点不同基因型间的出生重差异显著;SW 902、S0143、SW 0215、S0228、SW 24等5个微卫星位点不同基因型间的60日龄重差异显著;S0178、S0218、S0255、S0155、SW 951等5个微卫星位点不同基因型的4月龄重差异显著;而S0217微卫星位点的不同基因型的6月龄重差异显著。     

新城疫病毒F基因的真核表达及其免疫原性检测

为了探讨F基因在DNA免疫防制新城疫(ND)中的免疫原性,将NDV Z株F基因插入到真核表达载体pcDNA3.1/V5-H is-TOPO中,构建了真核表达质粒pcDNA NDV ZF。在脂质体作用下将pcDNA NDV ZF转染CEF细胞,用间接免疫荧光试验检测,在CEF细胞中可见有大量F蛋白表达。将重组质粒以100μg/只的剂量肌注免疫SPF雏鸡,经间接ELISA试验检测二免前后的血清,结果证明,pcDNA NDV ZF基因可在SPF鸡体内诱导相应抗体的产生,具有特定的免疫原性。     

猪附红细胞体感染对仔猪猪瘟免疫效果的影响

为探讨猪附红细胞体对仔猪猪瘟免疫效果的影响,本试验利用猪瘟抗体检测ELISA试剂盒,对已注射猪瘟疫苗的69头感染猪附红细胞体的仔猪和31头无猪附红细胞体感染的健康仔猪进行了猪瘟抗体检测。结果表明,感染猪附红细胞体仔猪的猪瘟抗体水平低下,其猪瘟疫苗整体免疫合格率(49·2%)明显低于健康仔猪(93·5%),且显性感染仔猪的免疫合格率(41·6%)明显低于隐性感染仔猪(53·5%)。说明猪附红细胞体严重干扰了猪瘟疫苗的免疫效果,且干扰程度与猪附红细胞体的感染程度呈正相关。     

乙烯对匍匐翦股颖ISR抗病反应中AsA-GSH循环及胼胝质沉积的影响

以匍匐翦股颖品种“Penn-A4”为试验材料,侵染立枯丝核菌后,经丁二醇(BDO)诱导产生系统抗性(ISR),喷施不同浓度的乙烯合成抑制剂氯化钴(CoCl₂)和促进剂1-氨基环丙烷羧酸(ACC)后,检测抗坏血酸-谷胱甘肽(AsA-GSH)循环中抗坏血酸(AsA)和还原型谷胱甘肽(GSH)含量及相关酶活性的变化,并观察匍匐翦股颖ISR反应中胼胝质沉积的变化。结果表明,乙烯抑制剂处理下,匍匐翦股颖幼苗中AsA含量较低,抗坏血酸过氧化物酶(APX)活性下降,大量GSH被催化还原为氧化型谷胱甘肽(GSSG),GSSG大量积累,同时谷胱甘肽还原酶(GR)活性较低,GSSG经GR少量还原为GSH。乙烯促进剂处理下,AsA含量较高,APX活性升高,GSSG在高活性GR作用下催化还原为GSH,使得GSH大量积累。因此在匍匐翦股颖ISR抗病反应中,高浓度乙烯促进AsA和GSH的大量积累,它们不仅参与了活性氧的代谢平衡,同时也作为信号分子在ISR抗病反应中起着重要作用。匍匐翦股颖感染褐斑病后,胼胝质主要沉积在厚壁细胞、韧皮部、木质部和表皮组织,其中厚壁细胞胼胝质沉积最多,表皮组织沉积最少。此外,胼胝质沉积面积在不同乙烯信号分子处理间存在差异,但随着处理时间的延长差异不显著。一定浓度的乙烯对ISR反应中胼胝质的沉积具有一定的影响,随着处理时间的延长显著增加,在100 μmol·L^-1ACC处理5 d后,胼胝质沉积总面积仅为9.916 mm²,处理10 d后升至最高,为38.396 mm²,但在病害侵染后期,胼胝质数量减少,在100 μmol·L^-1ACC处理15 d后,胼胝质沉积总面积降至20.052 mm²,反映了乙烯信号分子对胼胝质沉积的影响是一种短期效应,短期内可提高匍匐翦股颖植株抗病性,具有信号分子的短时效特点。研究结果为探清匍匐翦股颖ISR抗病响应中ET信号分子如何调控抗病生理特性提供了理论基础。     

日粮中添加牛至油对河西绒山羊育肥性能的影响研究

牛至精油对家畜生产性能和免疫力的提高有重要的影响。通过在日粮中添加牛至精油育肥河西绒山羊,研究其对河西绒山羊生长性能、屠宰性能及胴体品质的影响。对照组饲喂基础日粮,试验组在饲喂的基础日粮中分别添加4和7 g宜生饲宝(含牛至精油的添加剂),4和7 g宜生饲宝中牛至精油的含量分别为52和91 mg。对照组和试验组均为同月龄、同体重的河西绒山羊羯羊,试验组和对照组均设3个重复,每个重复5只羊。育肥期为90 d,每30 d为1个阶段。试验结果表明:育肥全期,对照组、4 g组和7 g组河西绒山羊平均日增重分别为96.30、172.22和169.82 g·d^-1,4 g组和7 g组分别显著高于对照组(P<0.05),4 g组和7 g组无显著差异(P>0.05);屠宰性状,胴体重对照组、4 g组和7 g组分别为20.24、24.18和23.90 kg,无显著差异(P>0.05),屠宰率对照组、4 g组和7 g组分别为48.86%、51.21%和51.56%,4 g组和7 g组分别显著高于对照组(P<0.05),4 g组和7 g组无显著差异(P>0.05),胴体净肉重对照组、4 g组和7 g组分别为12.90、16.27和15.99 kg,4 g组和7 g组分别显著高于对照组(P<0.05),4 g组和7 g组无显著差异(P>0.05);肉质性状,大理石纹4 g组和7 g组分别显著高于对照组(P<0.05),4 g组和7 g组无显著差异(P>0.05),pH、熟肉率、失水率、嫩度、蒸煮损失对照组、4 g组、7 g组间均无显著差异(P>0.05)。日粮中添加牛至油可以显著提高河西绒山羊的育肥性能,本试验日粮中添加4 g宜生饲宝(含牛至精油52 mg)效果最佳。     

低温胁迫对狗牙根生理及基因表达的影响

以耐寒性差异较大的杂交狗牙根品种运动百慕大、天堂419和普通狗牙根品种保定狗牙根为试验材料,分析了昼夜温度为适温(30 ℃/25 ℃)、亚适温(18 ℃/12 ℃)、冷害(8 ℃/4 ℃)和冻害(4 ℃/-4 ℃)4种温度处理下,低温对狗牙根生长速率和草坪质量、MDA含量、叶绿素荧光(F_v/F_m)、光合作用(P_n、G_s、C_i、T_r)、H₂O₂和O2·-含量、抗氧化酶活性(SOD、POD、CAT、APX)、抗氧化酶及耐寒相关基因(CBF1、COR、LEA)表达的影响。结果表明,随着温度的降低,狗牙根草坪质量、生长速率、F_v/F_m和光合作用显著下降,但在耐寒性强的运动百慕大中下降幅度较小;低温下叶片MDA和H₂O₂含量及O2·-产生速率显著升高,其中在耐寒性弱的保定狗牙根中升高程度更大;狗牙根叶片抗氧化酶活性及抗氧化酶基因的表达水平随着处理温度的下降而显著升高,其中在运动百慕大中更为明显;狗牙根CBF1、COR和LEA基因表达量随着温度的下降而显著升高,尤其是在耐寒狗牙根运动百慕大中更为显著。低温诱导的抗氧化酶和耐寒相关基因上调表达,增强了细胞内的抗氧化防御,有助于狗牙根植株维持较高的光合作用和细胞膜稳定性,延缓叶片的衰老,从而提高了狗牙根的抗寒能力。     

家蚕品种“明丰×春玉”改良系农村饲养初报

家蚕品种"明丰×春玉"抗Bm NPV改良系在农村试养中,表现出蔟中不利气候条件下结茧率偏低的现象。针对存在的问题,对品种特性进行进一步改良。改良品种的农村试养对比结果表明,改良系抗病毒病性状优良,各项经济性状优于对照品种。     

Effect of Luteolin on Blood Indexes,Liver and Kidney in Mice with Acute Mercury Poisoning

To study the effect of luteolin on blood indexes,liver and kidney in mice with acute mercury poisoning,28 mice were randomly divided into four groups:Control group (intraperitoneal injection 0.9% saline),luteolin group (lavage 100 mg/kg luteolin),mercuric chloride group (intraperitoneal injection 4 mg/kg mercury chloride) and mercury chloride+luteolin group (intraperitoneal injection 4 mg/kg mercuric chloride,lavage 100 mg/kg luteolin).The activities of ALT in serum,AST,CREA and BUN contents,blood WBC,RBC,HGB content and GSH and MDA contents of liver tissue were detected.Morphological changes of liver and kidney tissues were observed.The results showed that compared with the control group,the activities of ALT and AST of mercuric chloride group were extremely significantly increased (P < 0.01),serum CREA,BUN,blood WBC and liver tissue MDA contents were significantly increased (P < 0.05) while blood RBC,HGB and liver tissue GSH contents were significantly decreased (P < 0.05).Liver,kidney pathological changes were obviously.Compared with mercuric chloride group,the activities of ALT,AST in serum,CREA,BUN,blood WBC and liver tissue MDA contents of mercuric chloride+luteolin group were significantly decreased (P < 0.05),while blood RBC,HGB and liver tissue GSH contents were significantly elevated (P < 0.05).Liver,kidney pathological changes were attenuated obviously.The poisoning were characterized by inflammation and the occurrence of anemia when acute mercury poisoning occurred,liver and kidney showed different degrees of injury in mice.Luteolin could reduce the toxic effects of acute mercury poisoning on blood,liver and kidney.     

Effect of Human Menopausal Gonadotropin,17β-estradiol and Epidermal Growth Factor on the Quality of in vitro Maturation Bovine Oocytes

For optimizing in vitro maturation system of bovine oocytes,we firstly examined the influence of four different hormonal regimes(FSH+LH,HMG,FSH+LH+E₂ and HMG+E₂) on oocyte maturation rates.Then we studied the effects of epidermal growth factor (EGF) in the above defined medium on bovine oocyte maturation,in vitro development and quality of parthenogenetic embryos.The cell apoptotic index of parthenogenetic blastocysts was detected by TUNEL.No significant difference was observed in maturation rates in four groups supplemented with different hormones.However,human menopausal gonadotropin (HMG) provided steady maturation results in replicates.Maturation of oocytes was promoted by supplementation with 17β-estradiol (E₂).Combination of HMG and E₂ gave rise to steady and efficient mature results.The presence of EGF at 30 ng/mL concentration significantly increased maturation rate and blastocyst rate and reduced apoptotic cells in parthenogenetic blastocysts.Therefore,the optimal oocyte maturation solution could be supplemented with 0.075 IU/mL HMG,1 μg/mL E₂ and 30 ng/mL EGF.