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目的:建立从转基因作物中快速提取DNA的方法.方法 :采用Chelex-100法提取抗草甘膦大豆和非转基因大豆、转基因抗虫玉米Bt176和非转基因玉米中的DNA,使用PCR扩增大豆和玉米的内源基因(Lectin,zSSⅡb)及外源特异性序列(CaMV35S,Bt176)评价提取核酸的质量.结果 :Chelex-100法能够快速在1h之内从大豆和玉米中提取DNA,所提取的DNA可以直接用于PCR扩增反应,PCR扩增产物电泳条带清晰,转基因抗草甘膦大豆样品和转基因抗虫玉米Bt176检测均出现强阳性结果.结论 :Chelex-100法提取DNA可以作为转基因检测的模板,该方法具有经济、简便、快速的特点,适合于转基因检测工作. 相似文献
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改良Chelex-100法快速提取转基因农产品DNA 总被引:1,自引:0,他引:1
旨在建立一种从转基因农产品中快速提取DNA的方法.分别采用改良Chelex-100法和常规CTAB法提取转基因大豆GTS40-3-2基因组DNA,测其浓度和纯度,PCR扩增其内源基因(Lectin)、启动子(CaMV35S)和品系特异性序列,对两种方法进行比较和评价,并研究两种方法提取的DNA在-20℃下保存一个月内的检测效果,以及改良Chelex-100法在玉米、小麦和水稻等其他转基因农产品的应用效果.结果表明,改良Chelex-100法能够快速在1.5h之内从样品中提取DNA,所提取的DNA直接用于PCR扩增反应,产物电泳条带清晰明亮.两种方法提取的DNA在-20℃下保存一个月内的检测效果未见明显差别.该方法在玉米、小麦和水稻等转基因农产品的应用效果稳定.因此,改良Chelex-100法提取的DNA可以作为PCR扩增模板用于转基因农产品检测.该方法具有经济、简便、快速、安全的特点,适合转基因农产品大规模筛选和鉴别. 相似文献
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为探讨指甲游离缘核DNA分型的可行性, 采集无关个体指甲游离缘样本10份, 分别以不同消化体系, 采用有机法、Chelex-100法,有机法结合Chelex-100法等3种方法提取指甲游离缘核DNA, AmpFlSTR IdentifierTM试剂盒复合扩增, ABI PRISM 3130自动遗传分析仪检测分析。结果显示:与对照血样比较,有机法结合Chelex-100法提取的样本核DNA均获得满意的STR分型, 有机法提取的样本核DNA可以进行STR分型, 但部分样本图谱峰值不均衡, Chelex-100法提取的样本核DNA不能分型或出现较多等位基因缺失。提示指甲游离缘可以进行成功地核DNA的分型, 有机法和有机法结合Chelex-100法提取的DNA质量都可成功检测, 其中以有机法结合Chelex-100法提取DNA的检测成功率最高。 相似文献
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《基因组学与应用生物学》2018,(10)
为明确内蒙古西部地区放线菌的多样性,为未来该地区放线菌资源的开发利用及生态系统的稳定性提供一定的理论基础。本研究从内蒙古西部地区采集土壤样品,提取土壤样品的总DNA,通过巢式PCR扩增放线菌16S rRNA基因片段,利用DGGE (denaturing gradinent gel electrophoresis)技术进行分析,切胶回收,再利用不带GC夹子的引物进行扩增,将PCR产物送往公司测序后对16S rRNA基因序列进行比对,分析内蒙古西部地区放线菌的多样性及其与土壤理化性质之间的相关性。对内蒙古西部地区放线菌多样性分析发现,内蒙古西部地区土壤放线菌的多样性较为丰富,丰富度指数处于10~28之间,其中,棕钙土的丰富度最高,栗褐土的最低;同一地区相同类型土壤中草地的放线菌数量比耕地丰富。放线菌的多样性与有效磷的含量呈显著正相关。经过16S rRNA基因序列比对共得到了7个属的放线菌,包括Saccharopolyspora (糖多孢菌属)、Thermomonospora (高温单孢菌属)、Streptomyces (链霉菌属)、Iamiaceae (酸微菌属)、Corynebacterium (棒杆菌属)、Timonella、Pseudonocardia (假诺卡氏菌属)。通过研究得出内蒙古西部地区的放线菌资源较为丰富,作为应用于抗细菌、抗真菌和抗肿瘤的新型药物中的重要微生物资源,具有进一步研究的价值,继而推动内蒙古西部地区放线菌资源的开发与利用。 相似文献
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目的利用mtDNA 12S rRNA基因序列测定法对西藏自治区森林公安局送检的三件毛发物证进行种属鉴定,并探讨该方法在无毛囊毛发样本鉴定中的应用价值。方法用酚/氯仿法从毛发样本中提取出基因组总DNA,再用一通用引物通过PCR技术扩增mtDNA上12S rRNA基因的部分片段并进行序列测定。测序结果在GenBank上进行BLAST搜索,再利用DNAMAN软件进行同源性分析。结果1号样和3号样扩增产物序列与藏原羚的线粒体DNA的12S rRNA基因序列的部分片段的同源性均高达99%;2号样的序列与盘羊的线粒体DNA的12S rRNA基因序列的部分片段的同源性高达98%。结论1号和3号样为藏原羚,2号样为盘羊。本研究所用方法在野生动物案件的样本鉴定中有极高的应用价值。 相似文献
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Vázquez-Novelle MD Pazos AJ Abad M Sánchez JL Pérez-Parallé ML 《FEMS microbiology letters》2005,243(1):279-283
The aim of this study was to evaluate the ability of a nested PCR system to detect Salmonella senftenberg in raw oysters. The specific primers of the PCR were derived from the invA gene sequence, essential for Salmonella invasiveness into epithelial cells. First, for the extraction of DNA, four methods (guanidine isothiocyanate, E.Z.N.A. Mollusc Kit, Chelex-100, and lysis with detergents) were compared. A nested PCR method combined with 3.5 h pre-enrichment in buffered peptone water (BPW) and DNA extraction by the resin Chelex-100 is proposed for the detection of S. senftenberg in oyster samples. The detection limit of the method is less than 0.1 CFU/ml (<1 CFU/g of oyster). This procedure is shown to be an excellent tool for the sensitive detection of S. senftenberg from naturally contaminated oysters, with results being obtained within 8 h. 相似文献
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利用16S rRNA基因RFLP、16S rRNA基因序列分析以及16S-23S rRNA IGS PCR RFLP技术对分离自我国南北大豆产区的慢生大豆根瘤菌进行了群体遗传多样性和系统发育研究。16S rRNA基因PCR RFLP分析以及16S rRNA基因序列分析结果表明:所有供试慢生大豆根瘤菌可分为B.japonicum和B.elkanii两个类群,其中属于B.japonicum的为优势种群,占供试菌株的91%,属于B.elkanii的仅占9%,多样性水平较低。16S-23S rRNA IGS PCRRFLP研究结果表明:属于B.japonicum的慢生根瘤菌具有较丰富的遗传多样性,在69%的相似性水平上可分为群Ⅰ和群Ⅱ两大类群。群I的菌株以分离自黑龙江和河北等北部区域的菌株为代表,群Ⅱ的菌株以分离自广西和江苏等南部地域的菌株为代表,反映出明显的地域特征。两群菌株在系统发育上均与USDA6、USDA110和USDA122等B.japonicum的模式或代表菌株有差异。 相似文献
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Application of rpoB sequence similarity analysis, REP-PCR and BOX-PCR for the differentiation of species within the genus Geobacillus 总被引:1,自引:0,他引:1
Meintanis C Chalkou KI Kormas KA Lymperopoulou DS Katsifas EA Hatzinikolaou DG Karagouni AD 《Letters in applied microbiology》2008,46(3):395-401
Aim: To investigate the applicability of rpoB gene, which encodes the β subunit of RNA polymerase, to be used as an alternative to 16S rRNA for sequence similarity analysis in the thermophilic genus Geobacillus. Rapid and reproducible repetitive extragenic palindromic fingerprinting techniques (REP‐ and BOX‐polymerase chain reaction) were also used. Methods and Results: rpoB DNA (458 bp) were amplified from 21 Geobacillus‐ and Bacillus type strains, producing different BOX‐ and REP‐PCR profiles, in addition to 11 thermophilic isolates of Geobacillus and Bacillus species from a Santorini volcano habitat. The sequences and the phylogenetic tree of rpoB were compared with those obtained from 16S rRNA gene analysis. The results demonstrated between 90–100% (16S rRNA) and 74–100% (rpoB) similarity among examined bacteria. Conclusion: BOX‐ and REP‐PCR can be applied for molecular typing within Geobacillus genus. rpoB sequence similarity analysis permits a more accurate discrimination of the species within the Geobacillus genus than the more commonly used 16S rRNA. Significance and Impact of the Study: The obtained results suggested that rpoB sequence similarity analysis is a powerful tool for discrimination between species within the ecologically and industrially important strains of Geobacillus genus. 相似文献
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新疆艾比湖嗜盐菌的细菌视紫红质和16S rRNA基因序列的研究 总被引:1,自引:0,他引:1
为了研究分析嗜盐古生菌物种与细菌视紫红质(BR)蛋白基因资源,从40份土壤、湖水及淤泥样品中分离出148株嗜盐菌,对其中6株菌采用聚合酶链式反应(PCR)方法对其编码螺旋C至螺旋G的蛋白基因片段和16SrRNA基因进行了扩增,并测定了基因的核苷酸序列。与已报道的相应片段进行对比,ABDH10,ABDH1I和ABDH40中的螺旋C至螺旋G的蛋白与其他菌株差异显著。基于16SrRNA序列的同源性比较以及系统发育学研究表明,ABDH10和ABDH40是Natronorubrum属下的新成员和Natrinema属下的新成员,ABDH40的16SrRNA序列已登录到GenBank,其序列号为AY989910。ABDH11中的螺旋C至螺旋G的蛋白与其他菌株差异显著。 相似文献
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目的建立鼠棒状杆菌PCR检测方法并应用于临床样本检测。方法用脑心浸出液培养基复苏、培养鼠棒状杆菌(corynebacteriumkutscheri,C.kutscheri)并提取基因组DNA作模板;根据GenBank中C.kutsche6的16S基因序列设计合成引物,建立鼠棒状杆菌PCR检测方法并进行敏感性和特异性的评价;人工感染昆明鼠,建立小鼠棒状杆菌感染模型,采集肝脏和肾脏,提取DNA进行检测。结果成功建立了鼠棒状杆菌PCR检测方法,该方法可检测到100个阳性质粒;对小鼠沙门氏菌、肺炎链球菌和巴氏杆菌无交叉反应;全部8个人工感染样本全部检测为阳性。结论建立的鼠棒状杆菌PCR检测方法灵敏度高、特异性好,可作为鼠棒状杆菌感染的快速检测方法。 相似文献
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Sequence analysis of 16S rRNA genes amplified from two ribosomal RNA gene clusters of Bifidobacterium bifidum 总被引:3,自引:0,他引:3
Jung-Hoon Yoon Dong Koo Yim Michael Goodfellow Yong-Ha Park 《Antonie van Leeuwenhoek》1999,75(4):329-333
Two rRNA gene clusters were detected in the genome of Bifidobacterium bifidum KCTC 3202T using Southern blot analysis. To analyse the sequences of the 16S rRNA genes from rrnA and rrnB, 16S rDNAs were amplified by PCR using DNA fragments purified from gel slices containing each of the rRNA gene clusters. The amplified 16S rDNAs from rrnA and rrnB were cloned into vectors and three clones of each gene sequenced. The resultant sequences were confirmed by direct sequencing of the 16S rDNAs from rrnA and rrnB. Sequence differences were not found between rrnA and rrnB in 1488 bp of the 16S rRNA genes. 相似文献
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目的:对从新疆实验动物研究中心饲养的封闭群灰仓鼠体内分离到的1株鞭毛虫进行形态学鉴定及基因鉴定。方法取灰仓鼠回盲部内容物进行直接涂片和常规姬姆萨染色后镜检观察,提取虫体总DNA,PCR扩增该鞭毛虫的16S rRNA基因,测序后与国外已报道的鞭毛虫进行核酸同源性分析,并应用MEGA5.22软件绘制系统发育进化树。结果形态学观察表明分离到的鞭毛虫为鼠三毛滴虫。测序后核酸同源性分析表明鼠三毛滴虫新疆灰仓鼠分离株16S rRNA序列与国外已报道的三毛滴虫高度同源。系统发育进化树表明鼠三毛滴虫新疆灰仓鼠分离株序列与已报道的鼠三毛滴虫16S rRNA(序列号AY886846.1)位于同一进化分支,与其他相关三毛滴虫亲缘关系较远。结论形态学鉴定和16 S rRNA基因分析表明,此次从新疆实验动物研究中心饲养的封闭群灰仓鼠体内分离到的鞭毛虫为鼠三毛滴虫。 相似文献
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PCR-generated artefact from 16S rRNA gene-specific primers 总被引:2,自引:0,他引:2
Artefacts consisting of concatenated oligonucleotide primer sequences were generated during sub-optimally performing polymerase chain reaction amplification of bacterial 16S rRNA genes using a commonly employed primer pair. These artefacts were observed during amplification for terminal restriction fragment length polymorphism analyses of complex microbial communities, and after amplification from DNA from a microbial culture. Similar repetitive motifs were found in gene sequences deposited in GenBank. The artefact can be avoided by using different primers for the amplification reaction. 相似文献
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新疆塔里木盆地可培养嗜盐放线菌系统发育多样性 总被引:3,自引:0,他引:3
应用纯培养手段和基于16S rRNA基因序列的系统发育分析,对从塔里木盆地高盐环境土壤样品中分离的18株可培养嗜盐放线菌多样性进行了研究.实验结果表明,18株嗜盐放线菌可3个(GlycomycetaceaePseudonocardineae和Nocardiopsaceae),在有效发表的5个属的嗜盐放线菌中有4个属的嗜盐放线菌被分离到.多数菌株属于Actinopolyspora属(38.9%),Nocardiopsis属(27.8%)和Streptomonospora属(22.2%),是塔里木盆地高盐环境中嗜盐放线菌的优势类群.这些分离菌株中,菌株YIM 92370与最近种的相似性为92%,在Glycomycetaceae科内形成一个独立的分支,极有可能代表Glycomycetaceae科的一个新属.研究结果表明塔里木盆地高盐环境中存在有较为丰富的嗜盐放线菌系统发育多样性,并且潜藏着新类型的放线菌资源. 相似文献
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Nested PCR for detection of mutans streptococci in dental plaque 总被引:1,自引:0,他引:1
Sato T Matsuyama J Kumagai T Mayanagi G Yamaura M Washio J Takahashi N 《Letters in applied microbiology》2003,37(1):66-69
AIMS: Mutans streptococci such as Streptococcus mutans and Streptococcus sobrinus have been implicated in human dental caries. In an attempt to develop a rapid and sensitive method for detecting Strep. mutans and Strep. sobrinus in dental plaque, a nested PCR amplification based on the 16S rRNA gene was employed. METHODS AND RESULTS: A universal set of PCR primers for bacterial 16S rRNA gene was introduced for the first PCR, and then two sets of primers specific for the 16S rRNA gene sequences of either Strep. mutans or Strep. sobrinus were used for the second PCR. Eighteen plaque samples were analyzed, and a nested PCR was shown to be more sensitive for detecting Strep. mutans and Strep. sobrinus than direct PCR. CONCLUSIONS, SIGNIFICANCE AND IMPACT OF THE STUDY: The 16S rRNA gene-based nested PCR method is a rapid and sensitive method for the detection of mutans streptococci, and may also be suitable for carrying out large-scale studies on the cariogenicity of mutans streptococci. 相似文献