基于转录组的疏花软紫草低拷贝核基因引物开发

基于高通量的转录组测序,为大量并快速的开发分子标记提供契机。本研究对紫草科植物疏花软紫草进行转录组测序,共得到92042086条reads,从疏花软紫草158446个Unigene中搜索到332个低拷贝核基因。为进行多态性验证,从中随机挑选30个设计引物,并对3个疏花软紫草种群共9个个体进行PCR扩增,结果发现其中16对引物能够扩增出单一稳定的目的条带,从中随机挑选7个片段进行群体测序并计算DNA多态性。结果表明,7对引物的多态性位点平均值为657,单倍型平均值为514,单倍型多态性 （HD） 在0389~0944之间,核苷酸多态性 （Pi） 为000148~001723。通过转录组测序技术开发的低拷贝核基因有较高的多态性,且可以有效地运用于群体遗传学和谱系地理学研究中。另外,这些低拷贝核基因能够被运用于软紫草属植物系统发育重建以及物种形成等研究工作中。     

不同植被恢复模式下呼伦贝尔沙地土壤反硝化细菌nirK基因组成结构和多样性研究

本研究选取呼伦贝尔沙地5种植被恢复模式(单播冰草、单播羊柴、单播柠条、冰草+柠条和冰草+柠条+羊柴+披碱草)为研究对象,以完全退化的沙地为对照,采用分子生物学技术分析了土壤反硝化细菌nirK基因组成结构和多样性,并探讨了与土壤理化因子的相关性。结果表明,土壤反硝化细菌nirK基因组成存在明显差异。单播羊柴模式土壤反硝化细菌nirK基因多样性指数最高,其次为单播冰草和单播柠条,而两种混播模式最低,这5种植被恢复模式均显著高于对照裸地。序列和系统发育分析结果表明,所获得的nirK基因片段与NCBI数据库中的nirK基因的相似度在81%99%之间,分别归属于苍白杆菌属、根瘤菌属及不可培养的细菌,其中与不可培养细菌相关的片段占到总数的50%以上。典范对应和相关分析结果表明,速效磷、pH、全氮、全磷和含水量对反硝化细菌的影响均达到显著水平,且5种理化因子间均具有极显著相关性,说明这5种理化因子相互关联,共同对反硝化细菌nirK基因组成变化起到决定作用。     

延黄牛ALDH1A1基因CDS序列克隆及其在各组织中的表达差异研究

为探索乙醛脱氢酶1A1(acetaldehyde dehydrogenase 1A1,ALDH1A1)基因功能,本试验以16月龄延黄牛母牛为研究对象,屠宰后采集心脏、肝脏、肺脏、肾脏、胃、十二指肠、皮下脂肪和背最长肌,提取总RNA。根据GenBank上公布的牛ALDH1A1基因mRNA序列(登录号:NM_174239.2),利用Oligo 7.0软件设计引物,应用RTPCR扩增ALDH1A1基因,将扩增产物连接pMD18-T载体进行克隆测序,获得延黄牛ALDH1A1基因完整CDS序列,应用生物信息学软件分析核苷酸序列及其蛋白结构。以延黄牛不同组织总RNA为模板,通过实时荧光定量PCR技术检测ALDH1A1基因在延黄牛各组织间的表达差异。结果显示,ALDH1A1基因CDS序列全长1 506bp,编码501个氨基酸;延黄牛ALDH1A1基因序列与野牛、牛的同源性最高(≥99.7%),与猫和豹的同源性分别为89.4%和89.6%,符合物种进化规律。ALDH1A1蛋白分子质量为54.805ku,理论等电点为7.16,亲水性较强,占86.4%,酸性氨基酸和碱性氨基酸分别占11.4%和12.2%,属于可溶性蛋白,但不是分泌性蛋白,无典型信号肽切割位点;存在31个氨基酸磷酸化位点(分值>0.5)。延黄牛ALDH1A1蛋白二级结构含有α-螺旋、延伸链、β-转角和无规则卷曲,分别占42.12%、16.17%、8.18%和33.53%,与该蛋白三级结构预测结果相同。实时荧光定量PCR结果表明,ALDH1A1基因在延黄牛肝脏、胃、皮下脂肪、十二指肠和肾脏组织中极显著表达(P<0.01);在背最长肌中显著表达(P<0.05)。本试验结果为进一步开展延黄牛ALDH1A1基因功能及肉质基因筛选研究提供了参考依据。     

广西片形吸虫中间宿主—小土窝螺线粒体rrnL基因遗传多态性研究

为研究广西小土窝螺不同地理株线粒体大亚基（large subunit ribosomal rRNA,rrnL）基因的遗传多态性,对广西大片吸虫6个流行地区96个小土窝螺样品的rrnL基因进行PCR扩增,通过单链构象多态性（single strand conformation polymorphism,SSCP）技术筛选出具有代表性的样品进行克隆、测序,并用DNAStar 5.0及MEGA 4.0软件加以比对分析。结果显示,6个地区小土窝螺rrnL基因PCR扩增长度约500 bp,在长度为273 bp的序列中检测到15个变异位点,占核苷酸总数的5.49%。百色、南宁和桂林3个地区相同地理株间存在较大的遗传差异。种系发育分析表明,线粒体rrnL基因在一定程度上不是研究小土窝螺种群遗传变异的良好分子标记。本研究为阐明片形吸虫中间宿主—小土窝螺的种群遗传关系提供了基础数据。     

链孢粘帚霉寄生核盘菌菌核差异表达基因的筛选及分析

为克隆和研究链孢粘帚霉Gliocladium catenulatum寄生核盘菌菌核的相关基因,应用抑制消减杂交技术构建了cDNA消减文库并进行了筛选。通过PCR技术从文库中共筛选到1315个阳性克隆,克隆中插入片段大小主要集中于300～600bp之间。随机挑取120个克隆,经测序和同源性分析,获得60条有效序列,其中部分序列所编码的血红素加氧酶、核糖体蛋白L11、细胞色素P450及热激蛋白等均参与机体对胁迫条件的应答反应。11条序列在NCBI数据库中未找到显著匹配的序列,可能为新基因片段。分别将寄生于核盘菌菌核上的粘帚霉cDNA和粘帚霉与核盘菌纯培养的cDNA混合物经RasⅠ酶切后进行标记作为探针,利用反向Northern杂交技术验证了所选取的25条序列全部为差异表达基因片段。     

苏云金芽孢杆菌cry基因在大肠杆菌中表达产物和生物活性

研究了几种Bt cry基因于大肠杆菌(Escherichia coli)中表达产物在pH 10.0的50mmol/L碳酸钠和20mmol/L乙醇胺溶解液中的溶解性 ,发现同样的Cry蛋白在碳酸钠中的溶解度大于乙醇胺。通过胰蛋白酶消化 ,明确Cry1Ca7、Cry1Ia8酶解产物为 38kD多肽 ;Cry1Ie1、Cry1Cb2、Cry2Ab4酶解产物为 41kD多肽 ;Cry1Ac酶解产物为60kD多肽。采用FPLC层析方法对 6种原毒素及其酶解后得到的毒素多肽进行了分离纯化 ,比较了原毒素和毒素的杀虫活性的差异。其结果表明 ,Cry1Ac的原毒素和毒素对棉铃虫初孵幼虫的校正死亡率均为 100% ,Cry2Ab4的原毒素的毒力高于其酶解毒素。     

马生长激素(GH)基因的PCR-SSCP研究

选取4个蒙古马地方品种、1个国内培育品种和1个国外引人品种共281匹马，采用PCR—SSCP技术，检测了GH基因5’侧翼区、第1内含子、第2外显子和第5外显子4个位点的遗传多态性。结果显示：仅第5外显子出现多态性，表现出AA、BB和AB3种基因型，其余位点未检测到多态。群体遗传学分析结果表明：除纯血马外，其余品种都是等位基因A为优势基因；Hardy-Weinberg平衡检验显示，乌审马、乌珠穆沁马、巴尔虎马处于平衡状态，锡尼河马、三河马、纯血马处于非平衡状态；各品种马的多态信息含量均为中度多态（0．25〈PIC〈0．5）。本研究为今后马的分子育种奠定一定基础。     

猪圆环病毒2型灭活疫苗中病毒抗原含量实时荧光定量PCR检测方法的建立

依据GenBank公布的猪圆环病毒2型Cap基因序列,在保守区域设计特异性引物和TaqMan探针,优化反应体系,建立评价猪圆环病毒2型灭活疫苗中病毒含量的实时荧光定量PCR检测方法,对方法的特异性、敏感性和重复性进行试验,并验证灭活剂用量和灭活时间对检测结果的影响。结果显示：该方法只对猪圆环病毒2型基因有特异性扩增,其他3种对照病毒基因的扩增结果均为阴性;检测灵敏度达到10^2.0 TCID₅₀/mL,比普通PCR方法高100倍;方法的重复性好,对同一样品进行10次检测,变异系数为2.28%;不同灭活剂用量和灭活时间对结果的影响较小,不会因各厂家使用的灭活剂用量和灭活时间不同,影响疫苗对比实验的公平性。该研究成功建立了一种评价猪圆环病毒2型灭活疫苗中病毒含量的实时荧光定量PCR检测方法,用于猪圆环病毒2型灭活疫苗样品中病毒抗原含量的定量,其结果可以反映不同猪圆环病毒2型灭活疫苗样品中抗原含量差异,为研究猪圆环病毒2型灭活疫苗病毒抗原含量评估方法提供了新的思路。     

Comparison Analysis of Immune Related Gene of Orf Virus in Sheep and Camels

The purpose of this study was to investigate the variation of Orf virus (ORFV) immune related genes after infection with different species.The ORFV genomes of sheep and camel were extracted and named ORFV-Y and ORFV-LT,respectively.Based on ORFV genome sequence published in GenBank (accession No.:KF234407.1),three pairs of specific primers were designed and synthesized to amplify the B2L,F1L and VIR gene fragments of ORFV-Y and ORFV-LT,respectively,and the amplified fragments were cloned into pMD19-T vector,transformed into E.coli DH5α competent cells.The recombinant plasmid was identified,and positive clones were selected for sequencing,DNAStar software was used to analyze the homology,amino acid sequence and phylogenetic tree of 13 ORFV genome sequences published on NCBI.The results showed that the nucleotide homology of B2L,F1L and VIR genes were 92.8% to 99.2%,95.7% to 99.5% and 77.6% to 100%,respectively.After comparing the amino acid sequence between the two genomes and the reference sequence,it was found that there were obvious differences in the immune related genes between the two genomes,and F1L gene had some rules to follow.The phylogenetic analysis of B2L,F1L and VIR genes showed that ORFV-Y was closely related to the Chinese Fujian goat strain,while ORFV-LT was far from the reference strains,and was a separate branch.The results showed that ORFV had obvious difference in immune related genes between sheep and camels,it provided a reference basis for further research on the changes of ORFV gene sequences in different species and the development of vaccines for different species in the future.     

Polymorphism of IGFBP2 Gene and Its Association with Meat Quality Traits in Pigs

This study was aimed to analyze the genetic variation of insulin-like growth factor binding protein 2 (IGFBP2) gene effect on meat quality traits in pigs. A pair of primer was designed,which based on DNA sequence of IGFBP2 gene (GenBank accession No.:BV727778). The genetic polymorphism of IGFBP2 gene was detected by PCR-RFLP in Sujiang pig, Jiangquhai pig and Landrace pig, and the association between IGFBP2 gene polymorphism and meat quality traits in three pig breeds was analyzed. The results showed that three genotypes (AA, AB and BB) were detected. The Chi-square test results showed that the genotype distribution of three pig breeds was in Hardy-Weinberg equilibrium (P > 0.05). The polymorphism information content (PIC) were moderately polymorphic in three pig breeds. According to the association analysis of different genotypes, significant difference was found in color value, intramuscular fat content and marbling, the color value (except for Jianquhai pig) and intramuscular fat content of AA genotype were significantly higher than AB and BB genotypes (P < 0.05), the marbling of AA and AB genotypes was significantly higher than BB genotype (P < 0.05). In conclusion,the polymorphism of IGFBP2 gene intron 3 had significant effects on meat quality traits, and was candidate gene for the potential impact on meat quality traits of pigs.