云南不同烟区片烟醇化过程色度及主要化学成分变化特征研究

研究云南不同烟区片烟醇化过程中外观颜色以及内在化学物质变化差异,为云南烟区醇化片烟的使用提供理论依据。取云南3个产区片烟进行醇化,对比分析其在醇化过程中的颜色以及内在化学物质变化差异。不同产区片烟在醇化过程中色差值L、b与总糖、总氮、烟碱呈现逐渐下降趋势,云南文山片烟色差值L、色差值b、总糖、总氮下降幅度大于云南保山与云南大理;还原糖与质体色素降解产物先上升后下降,云南大理峰值出现时间晚于云南保山与云南文山;色度值R、苯丙氨酸降解产物、西柏烷类降解产物、棕色化产物逐渐上升,不同产区变化幅度表现为云南文山>云南保山>云南大理。云南文山片烟在醇化过程中,片烟的外观颜色与内在化学物质变化幅度更大,达到最佳醇化期所需时间少于云南大理与云南保山。     

广西芒果树叶片苔藓发生情况调查及药剂筛选试验

对广西芒果树叶片苔藓的发生情况及防治药剂进行了初步研究?调查了广西芒果主产区的南宁市(武鸣区?兴宁区)和百色市(田东县?田阳县?田林县和右江区)?在南宁市开展4种药剂的18种不同浓度或者配比组合的药剂筛选试验?结果表明, 南宁市芒果树叶片平均发病率达到88.5%, 右江区发病率为81.7%, 其后依次为田东县?田林县和田阳县, 发病率分别为56.1%?54.8%和34.2%?通过不同药剂及其不同配比药效试验, 80%乙蒜素乳油的防效极显著优于46%氢氧化铜水分散粒剂?32%唑酮·乙蒜素乳油和70%甲基硫菌灵可湿性粉剂?80%乙蒜素乳油500倍液?1 000倍液和1 500倍液的防效分别为93.37%?85.82%和51.85%?综上, 芒果树叶片苔藓已在广西全区普遍发生, 南宁市和右江区受害严重, 推荐使用80%乙蒜素乳油1 000倍液防治?     

水牛SND1基因克隆及生物信息学分析

试验旨在利用电子克隆法对水牛SND1（staphylococcal nuclease and tudor domain containing 1）基因进行克隆和序列分析，为探究该基因对水牛泌乳性能的作用机制奠定基础。以奶牛SND1基因（GenBank登录号：NM_205784.1）作为种子序列，利用Primer Premier 5.0设计3对引物，以水牛基因组DNA为模板，PCR扩增水牛SND1基因mRNA序列，扩增获得序列连接pMD18-T载体，通过测序拼接获得水牛SND1基因mRNA全序列，并对其进行生物信息学分析。结果显示，水牛SND1基因完整编码序列长为3 503 bp，包含长为2 733 bp CDS序列，编码910个氨基酸，蛋白分子式为C₄₅₂₃H₇₁₈₃N₁₂₈₁O₁₃₅₄S₂₆，分子质量为102.01 ku，理论等电点（pI）为6.74，不稳定系数为42.07，平均亲水性为-0.419，属可溶酸性蛋白。二级结构以α-螺旋和无规则卷曲为主，其中α-螺旋占37.80%，无规则卷曲占34.18%。结合Protfun 2.2在线软件对SND1的功能进行预测分析表明，该蛋白在嘌呤和嘧啶、中央中间代谢、能量代谢、氨基酸生物合成发挥功能的可能性分别为0.449、0.401、0.303和0.262。SND1基因编码区序列与黄牛、绵羊、山羊、猪、马、人的同源性分别为98.7%、97.8%、97.8%、93.8%、93.1%和91.7%，物种之间同源性较高，系统进化情况与其亲缘关系远近一致。利用SMART在线软件预测蛋白结构域，结果显示，水牛SND1蛋白包含有4个SN区域，说明SND1基因编码区在进化过程中较为保守。     

基于生态经济学理论的林下套种模式研究

在分析生态经济学理论基础上论述了林下经济的生态经济学理论基础,并介绍了几种主要的林下经济模式,对几种模式的相关试验研究结果表明:合适的林下经济模式不仅可以有效地带来可观的经济效益,而且可以提高林下土壤肥力以及改良土壤物理性质,从而实现生态经济学的核心内涵—生态效益与经济效益双丰收。     

草果AtNCED基因克隆、表达和植物表达载体构建

9-顺式环氧类胡萝卜素双加氧酶(9-cis-epoxycarotenoid dioxygenase, NCED)是ABA生物合成的限速酶。诸多研究表明NCED基因表达量的变化与ABA含量显著相关,在种子休眠过程中发挥重要作用。为探究草果AtNCED基因的序列特征和功能,本研究以草果(Amomum tsaoko Crevost et Lemarie)种子转录组为基础,采用RT-PCR技术克隆了一个AtNCED基因。该基因全长2 372 bp,包含一个1 830 bp的开放阅读框(open reading frame, ORF),编码610个氨基酸。生物信息学分析显示,AtNCED基因编码的蛋白在N-末端包含典型的叶绿体转运肽序列,在催化结构域含有4个高度保守的组氨酸残基。AtNCED蛋白与芭蕉科马来西亚蕉同源性较高,与其他单子叶植物处在同一进化分支。实时荧光定量PCR分析结果表明,AtNCED基因表达量随着层积时间的增加逐渐下降,该基因可能正向调控种子休眠,在草果种子休眠诱导与维持中发挥重要作用。进一步地,利用同源重组方法,成功构建了pBI121-AtNCED过表达载体,并转化至农杆菌EHA105。该研究结果为弄清ABA激素信号在种子休眠中的调控作用提供了帮助。     

寨卡病毒SYBR GreenⅠreal-time PCR方法的建立及应用

为建立一种针对寨卡病毒的快速诊断方法,本研究根据寨卡病毒的3’端保守基因序列,设计合成1对引物,建立了检测寨卡病毒的荧光定量PCR方法。结果显示:所建立的检测方法的Ct值与标准品在1.41×10^1~1.41×10^10^ copies/μL具有良好的线性关系,相关性为1,斜率为-3.502;灵敏性结果显示,该方法的检测限度为1.41×10^1 copies/μL,是普通PCR的10000倍;特异性结果显示,对CHIKV、DENV和JEV无特异性扩增,特异性强;重复性试验结果显示,组内和组间变异系数均小于1%,重复性好。本研究建立的SYBR Green I real-time PCR检测方法,可用于寨卡病毒感染的快速诊断。     

“互联网+农业”模式下食用菌的营销策略

在"互联网+农业"融合发展背景下,食用菌企业需要借助互联网,构建市场主导、数字驱动的全新营销战略,助力产品营销。以"互联网+农业"模式为研究视角,分析食用菌产品营销现状,提出发挥技术优势、挖掘用户需求和建设优质平台等营销建议,以助力食用菌产品市场营销与效益转化。     

Isolation,Identification and Analysis of Serotype and Antibiotic Susceptibility of Pathogenic Salmonella from Chickens

To investigate the situations of predominant strain and antibiotic resistance of pathogenic Salmonella from chickens in Guangxi Zhuang Autonomous region, Salmonella was pre-enriched and isolated from tissues of clinical suspected chickens, and the Salmonella isolates were identified by biochemical test using ID 32E System for the identification of Enterobacteriaceae of VITEK System ATB Expression, serotypes were determined by slid agglutination test, antibiotic susceptibility was analyzed by ATB VET Susceptibility Test Strip of Enterobacteriaceae antibiotics.The results showed that 34 Salmonella strains were obtained from 310 clinical samples, of which 1 strain belonged to A serogroup, 1 to C2 serogroup, 15 to B serogroup, 14 to D serogroup and 3 to untyped serogroup, and S.typhimurium of B serogroup and S.pullorum of D serogroup were the predominant serotypes.All Salmonella isolates were sensitive to meropenem, imipenem, spectinomycine and apramycine, and the resistance rates to chloramphenicol, kanamycine and gentamicine were less than 10%, and the resistance rates to amoxicillin, streptomycine, flumequine, oxolinique, sulfamethizol, tetracycline and nitrofurantoine ranged between 50% and 90%, while the resistance rates to penicilline, oxacilline, fusidique, rifampicine and metronidazole reached to 100%.The results indicated that the serotype distribution of pathogenic Salmonella from chickens exhibited regional characteristics, and S.typhimurium and S.pullorum were the predominant serotypes in Guangxi Zhuang Autonomous region, and antibiotic resistance of Salmonella isolates was very serious which should be highly concerned.     

广西猪瘟病毒E0和E2基因的克隆及序列分析

通过分析目前广西猪瘟病毒(CSFV)的E0和E2基因特征,为了解广西地区CSFV的分子流行病学、遗传变异及综合防控提供科学依据。试验采用RT-PCR方法,对阳性猪瘟样品进行CSFV的E0及E2基因的扩增,经克隆、测序后,利用DNAStar软件对序列进行比对分析,同时绘制系统遗传进化树。结果表明,从阳性猪瘟样品中成功扩增CSFV的E0及E2基因。序列比对分析发现,GX2毒株与参考毒株的E0基因核苷酸同源性在83.1%~94.1%,其推导氨基酸同源性在85.9%~99.6%;与参考毒株的E2基因核苷酸同源性为81.7%~93.7%,其推导氨基酸同源性为89.0%~97.0%;E0与E2基因均属于基因Ⅱ群。氨基酸变异位点分析表明,E0蛋白的RNase活性区域氨基酸基序位点没有发生变异;E2蛋白中15个位点上的半胱氨酸均未发生变异,但单抗识别位点S734R发生变异。遗传进化分析显示测定的GX2毒株与近年来广西CSFV流行毒株的变异趋势相似,与中国传统疫苗株HCLV、经典强毒株Shimen的同源性较低,亲缘关系较远,与广西近年来的流行毒株GXWZ02株的同源性较高,亲缘关系较近。     

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.