狂犬病病毒SRV9克隆株核蛋白基因的克隆、表达与特性分析

根据已发表的狂犬病病毒核蛋白基因序列，设计并合成了一对引物，从SAD株驯化的SRV9。蚀斑株中提取病毒RNA，通过RT-PCR扩增出核蛋白的全长cDNA序列，测序结果显示，其序列与国外报道的SAD母源株序列一致。将核蛋白的cDNA克隆至原核表达载体pET-28b( )中，转化大肠杆菌BL21（DE3）plyss，于30℃1mmol/LIPTG条件下诱导表达，大肠杆菌菌体裂解产物经SDS-PAGE分析，在分子量约为56kDa处出现一新的蛋白带。和预期的目的蛋白分子量相符，Western-blotting检测表明，表达产物能与狂犬病病毒阳性血清发生特异性反应，出现单一反应带，扫描分析显示，表达产物占菌体总蛋白的23%，包涵体分离，纯化后，纯度达89%，上述结果为核蛋白在狂犬病基因免疫和免疫检测中的进一步应用奠定了基础。     

大骨鸡中MSTN基因表达规律性的研究

本实验以大骨鸡为试材,采用RT-PCR法检测了MSTN基因在大骨鸡不同器官、不同时间的表达情况,结果表明MSTN基因在骨骼肌中表达水平较高,在心肌、肾脏、脑、肠、舌中也有微量表达,但在肺、肝脏中未检测出MSTNmRNA,而且在14日龄时表达水平明显低于35日龄和56日龄,而且在孵化后一周时胸肌中MSTN基因的表达水平达到最低。     

柑橘裂皮病类病毒的一步RT-PCR法检测及其在甜橙体内的分布

柑橘裂皮病是由柑橘裂皮病类病毒(Citrusexocortisviroid,CEVd)引起的一种重要的柑橘病害。分别采用快速微量核酸提取法和SDS-KAc抽提法在表现症状的Etrog香橼中提取核酸,采用一步RT-PCR法对CEVd进行检测,结果显示SDS-KAc法可以消除带毒样品中非特异性条带。从嫁接接毒的铜水72-1锦橙植株的接穗部取嫩叶、老叶、皮,从砧木部茎杆上取老皮以及根皮分别提取总核酸进行RT-PCR检测,分析CEVd在甜橙体内的分布情况。初步检测结果表明在接穗的嫩叶、老叶、皮,砧木部茎杆的老皮和根皮上都可以检测到CEVd,以接穗部叶和皮检出稳定性高。     

摄入不同能量的围产期乳牛肝低密度脂蛋白受体mRNA丰度的比较

将30头健康、经产、处于围产期的黑白花乳牛随机分为3组，每组10头。从产前28d开始，低能量组乳牛饲喂《中国奶牛饲养标准（2000）》减少20％日粮（能量摄入80％），对照组乳牛饲喂《标准》日粮（能量摄入100％），高能量组乳牛饲喂《标准》增加20％日粮（能量摄入120％），产后各组乳牛均饲喂标准日粮。至产后第56d结束试验；采用内对照RT-PCR方法检测摄入不同能量的围产期乳牛肝活体组织低密度脂蛋白受体（LDLR）mRNA丰度。结果，不同能量组乳牛肝LDLR mRNA丰度产前至产后均呈现先升高后降低的趋势。100％和120％能量组肝LDLR mRNA丰度在产后14d达最大值，且产后均高于产前（产后56d除外，P〈0．01或P〈0．05）；而80％能量组产后1d即达到最大值，产前14d至产后14d，LDLR mRNA相对表达量显著高于100％和120％能量组；产后28～56d，120％能量组显著高于80％和100％能量组（P〈0．01）。表明围产期乳牛能量摄入水平对肝LDLR mRNA丰度有显著影响。     

Detection of Colletotrichum coccodes from soil and potato tubers by conventional and quantitative real-time PCR

Colletotrichum coccodes is the causal agent of the potato blemish disease black dot. Two PCR primer sets were designed to sequences of the ribosomal internal transcribed spacer (ITS1 and ITS2) regions for use in a nested PCR. The genus-specific outer primers (Cc1F1/Cc2R1) were designed to regions common to Colletotrichum spp., and the species-specific nested primers (Cc1NF1/Cc2NR1) were designed to sequences unique to C . coccodes . The primer sets amplified single products of 447 bp (Cc1F1/Cc2R1) and 349 bp (Cc1NF1/Cc2NR1) with DNA extracted from 33 European and North American isolates of C. coccodes. The specificity of primers Cc1NF1/Cc2NR1 was confirmed by the absence of amplified product with DNA of other species representing the six phylogenetic groups of the genus Colletotrichum and 46 other eukaryotic and prokaryotic plant pathogenic species. A rapid procedure for the direct extraction of DNA from soil and potato tubers was used to verify the PCR assay for detecting C. coccodes in environmental samples. The limit of sensitivity of PCR for the specific detection of C. coccodes when inoculum was added to soils was 3·0 spores per g, or the equivalent of 0·06 microsclerotia per g soil, the lowest level of inoculum tested. Colletotrichum coccodes was also detected by PCR in naturally infested soil and from both potato peel and peel extract from infected and apparently healthy tubers. Specific primers and a TaqMan fluorogenic probe were designed to perform quantitative real-time (TaqMan) PCR to obtain the same levels of sensitivity for detection of C. coccodes in soil and tubers during a first-round PCR as with conventional nested PCR and gel electrophoresis. This rapid and quantitative PCR diagnostic assay allows an accurate estimation of tuber and soil contamination by C. coccodes .     

RT—PCR检测南方菜豆花叶病毒

根据南方菜豆花叶病毒（ＳＢＭＶ）两株系Ｂ和Ｃ的核酸序列设计两对引物，利用ＲＴ－ＰＣＲ可以特异地区分纯化的和０．２ｇ病叶中的两株系，ＲＴ－ＰＣＲ检测ＳＢＭＶ－Ｂ的灵敏度为１０ｐｇ。     

检测猪流行性腹泻病毒的R-PCR方法的建立

根据猪流行性腹泻病毒 (PEDV)的N基因自行设计和合成了一对可扩增长度为 641bp目的片段的引物 ,成功地建立了检测的猪流行性腹泻病毒的RT PCR方法。对猪轮状病毒 (PRV)、猪传染性胃肠炎病毒 (TGEV)的RT PCR检测结果均呈阴性。对PEDV JS株的RT PCR产物的序列分析表明 ,与CV777株的同源性为 97 3 %。