盐碱胁迫下黑麦草生长及离子微区分布特征

盐碱生境通过离子毒害和渗透胁迫等抑制植物的生长发育。离子微区分布调控主要通过调整盐分在不同部位的分布来减轻Na⁺等高浓度离子对重要组织器官的毒害作用,是盐碱胁迫下植物生存的重要策略之一。为探究黑麦草在盐碱胁迫下的离子微区分布特征,本研究通过水培法,采用不同盐碱浓度(0、50、100、200 mmol·L^-1)培养液处理黑麦草植株,考察其生长、离子吸收、运输选择性和微区分布变化,揭示黑麦草对盐碱胁迫的适应机制。结果表明:1) 盐碱胁迫下,植株的相对含水率、叶绿素含量逐渐降低,电解质外渗率显著升高;当盐碱浓度大于100 mmol·L^-1时,根长、株高和生物量均显著降低,即黑麦草的耐盐阈值是100~200 mmol·L^-1;2) 盐碱浓度为50 mmol·L^-1时,植株根中K⁺/Na⁺较空白升高了48.3%,Ca²⁺/Na⁺升高了54.1%,说明黑麦草根部可通过增强K⁺、Ca²⁺的吸收来维持细胞渗透压并缓解高浓度Na⁺的毒性;3) 在50~200 mmol·L^-1的盐碱浓度下,黑麦草叶片中可溶性组分及细胞壁中Na⁺的相对含量较对照显著增加,但细胞器内Na⁺的相对含量降低,说明叶部将Na⁺富集在液泡和细胞壁中,以减少Na⁺对细胞器的毒害作用;4) 叶片微观结构的SEM电镜图片显示,盐碱胁迫下叶片表皮增厚、导管数量减少和孔径缩小。综上所述,盐碱胁迫下黑麦草不同器官的适应机理不同,根部主要通过强化K⁺、Ca²⁺的吸收,降低对Na⁺的吸收,并将Na⁺区隔化在液泡中以降低离子毒害和维持渗透调节,而叶片主要通过将Na⁺区隔在液泡及细胞壁中,以及微观结构的变化来保护细胞器免受离子毒害。本研究可为黑麦草的耐盐碱适应机制及其在盐碱土上的种植提供理论依据。     

发酵花生秧对番鸭生产性能、屠宰性能、血清生化指标及鸭粪常规成分的影响

本研究旨在探究发酵花生秧的营养价值及其对番鸭生产性能、屠宰性能、生化指标及鸭粪污染指标的影响,探讨利用发酵花生秧进行番鸭节粮养殖的可行性。选取15日龄的公番鸭360只,随机分为4组,每组6个重复,每个重复15只。对照组饲喂基础日粮,试验Ⅰ组饲喂90%基础日粮+10%发酵花生秧,试验Ⅱ组饲喂85%基础日粮+15%发酵花生秧,试验Ⅲ组饲喂80%基础日粮+20%发酵花生秧,预饲期7 d,正式试验期48 d,测定并计算各组番鸭的生产性能、屠宰性能及各脏器指数,同时采集各组番鸭的血清、肌肉及新鲜粪样,测定血清生化指标及鸭粪常规成分的变化情况。结果表明,①与未发酵的花生秧相比,发酵后的花生秧粗蛋白质、钙水平分别上升31.82%（P<0.01）、97.40%（P<0.01）;粗纤维、磷及水分含量分别下降2.35%（P<0.05）、20.69%（P<0.05）、53.23%（P<0.01）,营养价值得到提升。②与对照组相比,试验Ⅰ、Ⅱ组料重比分别下降6.51%（P<0.01）、6.84%（P<0.01）;试验Ⅰ、Ⅱ、Ⅲ组的腿肌率分别上升20.50%（P<0.05）、25.55%（P<0.05）、9.27%（P>0.05）;肝脏指数分别上升9.90%（P>0.05）、12.23%（P<0.05）、3.18%（P>0.05）;肌胃指数分别上升17.70%（P<0.05）、30.82%（P<0.05）、36.66%（P<0.05）;腺胃指数分别上升1.37%（P>0.05）、32.99%（P<0.05）、36.43%（P<0.05）;③发酵花生秧可影响番鸭血清中TP、ALB、GLB、A/G、ALT、AST、AST/ALT、UREA、UA、CRE含量;与对照组相比,试验Ⅰ、Ⅱ、Ⅲ组鸭粪中的总氮、磷、钾、水分含量均呈下降趋势。综上,10%、20%发酵花生秧饲料能显著提高番鸭的生产性能,明显降低增重成本,对番鸭的产肉性能无明显影响,但可能对其肝脏功能、肾脏功能、免疫功能有一定的影响。     

猪日本脑炎病毒RT-PCR检测方法的建立

设计了1对引物,利用RT-PCR技术检测乙型脑炎病毒(JEV)。从GenBank中查出收录的31株猪乙型脑炎病毒E基因的已知序列,用DNA star软件对这31株猪乙型脑炎病毒E基因进行同源性分析,以确定扩增的靶序列。以这段靶区域为模板,利用Primer 5软件设计了1对引物,用减毒株SA14-14-2建立了检测乙脑病毒的RT-PCR方法,经敏感性,特异性试验测定,证明该方法敏感,特异;该法可检出样品稀释至256倍的鼠脑毒,相当于0.06个TCID50,对4株河北地区JEV分离株进行检测,结果所设计引物对4株病毒均能扩增出预期的片段。     

影响仔猪胃肠道发育的因素

仔猪胃肠发育的情况直接影响了营养物质的消化、吸收及利用,及时找到影响其发育的因素对仔猪的营养管理是非常有意义的。目前发现的诸多因素中,生长因子及营养物质对其发育起到促进作用,而抗营养因子往往对其发育不利。本文从生长因子、营养物质到抗营养因子角度出发,分析了它们对仔猪肠道发育影响,为今后合理配制仔猪饲养阶段的日粮提供依据。     

猪胎及仔猪消化道发育的研究进展

猪消化道发育的情况直接影响了营养物质的消化吸收与利用,因而找出其发育规律能更好的指导仔猪的饲养管理。本文综述了猪从胚胎到断奶以后消化道组织器官、消化腺分泌、肠道吸收能力的发育情况,为合理配制仔猪日粮及饲养管理等方面提供依据。     

Trinexapac-ethyl、Prohexad ione-Ca在草坪化学控制中的应用研究

为探明Trinexapac-ethyl和Prohexadione-Ca用于草坪化学控制的可行性,研究了其对高羊茅(Festuca arundinacea)生长发育的影响。结果显示:使用剂量高于0.095 kg/hm²时,Trinexapac-ethyl对高羊茅具有明显的矮化作用,在0.36kg/hm²剂量下Prohexadione-Ca的抑制率可达95.2%;Trinexapac-ethyl和Prohexadione-Ca都能使植株新增鲜重显著降低,但对新增干重影响很小,Trinexapac-ethyl对植株新增干重无影响;在施用Trinexapac-ethyl的情况下,随着留茬高度的增加新增株高减少,合理留茬高度为4-6cm;Trinexapac-ethyl和Prohexadione-Ca可以有效降低株高,从而减少草坪修剪次数。     

Cloning,Expression and Bioinformatics Analysis of Enterococcus faecalis from Northeast Black Bear

In order to detect Enterococcus faecalis endocarditis antigen (EfaA) of bear that was used to disclose the infected Northeast Black bear immediately, a pair of PCR primers was synthesized by EfaA gene of Enterococcus faecalis that was recorded in GenBank (accession number:U03756.1) and the target fragment was 689 bp. The PCR product was cloned by pMD19-T vector, then was transferred to Escherichia coli DH5α competent cells and the positive clones were filtered. Recombinant plasmid (pMD19-T-EfaA) was extracted. Identification of PCR and digestion, sequencing, the structure prediction of proteins were operated. The results showed that EfaA gene was cloned successfully, and the gene homology with ATCC 29212 was 100.0%. pMD19-T-EfaA was constructed successfully, structure of proteins was predicted. This study provided theoretical basis for diagnostic methods of Enterococcus faecalis and laid basis for prevention and control of Northeast Black bear disease.     

Pathogen Analysis of Bovine Respiratory Disease Complex

To investigate the pathogen of bovine respiratory disease complex (BRDC) of a dairy farm in Guangxi, a strain of Mycoplasma and a strain of gram-negative pathogenic bacterium were isolated and identified by the means of field surveys, clinic observation, pathological examination, isolation studies and so on.Treatments were taken according to drug sensitivity test results.The Mycoplasma strain, growing on PPLO medium, formed typical "fried egg" colonies.A 448 bp of oppF fragment was amplified by PCR from the strain and had 98.4% nucleotide identity with Mycoplasma bovis reference isolate PG5 of USA.The biochemical features of the gram-negative bacterial isolate were same with Serratia marcescens.The PCR amplified 16S rDNA of the gram-negative pathogenic bacterium strain was 1 400 bp.It shared 99.0% nucleotide identity with other Serratia marcescens reference strains obtained from GenBank.Animal experiment showed that the gram-negative pathogenic bacterium isolate could cause the mice to die.The drug sensitivity tests showed all isolates were sensitive to spectinomycin, azithromycin, amikacin, gentamicin and neomycin.It was effective to treat with dexamethasone and spectinomycin.Pathogen analysis and drug treatment showed that the BRDC was caused by Mycoplasma bovis and Serratia marcescens.     

猪圆环病毒2型山东分离株全基因组的克隆与序列分析

根据猪圆环病毒2型(PCV-2)全基因组序列,设计一对特异性引物,从疑似断奶仔猪多系统衰竭综合征(PMWS)病料中扩增出PCV-2基因组DNA,将基因片段克隆于pMD18-T载体,筛选获得含有相应片段的阳性重组质粒pMD18-T-PCV-2。对筛选出的阳性质粒进行测序。结果表明,PCV山东株的全基因组为1 767 bp,与国内外毒株核苷酸同源性高达99.6%。