用聚合酶链反应检测产蛋下降综合症病毒核酸的研究

根据对ＥＤＳ－ＤＮＡ重组质粒ｐＴＥＺＰ３和ｐＴＥＺＰ２８的核酸序列分析结果,设计了两对引物,它们均能从ＥＤＳ－ＤＮＡ上扩增出一个特异片段,其长度分别为２３８ｂｐ和２０９ｂｐ。经比较,ＰＣＲ比血球凝集试验至少灵敏２００倍,比核酸杂交试验灵敏千万倍,对１００份自然发病鸡的肛拭子,血液和软壳蛋样品的检测结果表明;ＰＣＲ的阳性出率远高于酸杂交试验,并用病毒分离方法证实了ＰＣＲ对野外病料的检出结果是可信的。     

人癌细胞内质网分子伴侣Grp94基因近3‘端的初步分析

采用ＰＣＲ及ＲＴ－ＰＣＲ方法结合核酸分子杂交技术,首镒确定了与Ｇｒｐ９４ｃＤＮＡ２２３１－２５００碱基片段对应的Ｇｒｐ９４基因序列上有内含子。含有内含子的扩增片段长约７０８ｂｐ。对三种癌细胞系进行了ＰＣＲ和ＲＴ－ＰＣＲ反应,电泳结果显示存在差异。     

二核苷酸重复多态性的非同位素检测及其在基因诊断中的应用

本文报道了一种检测二核苷酸重复多态性的简便的非同位素法,利用重复序列两侧的特异引物进行ＰＣＲ扩增,产生的等位片段在薄层变性聚丙烯酰胺凝胶电泳上分离,再用灵敏的银染法显色。该方法不需要标记ＰＣＲ产物,简便、快速,分辨率可达１ｂｐ,并可用多对引物同时进行多重ＰＣＲ分析。用此方法对ＤＭＤ家系成员ｄｙｓｔｒｏｐｈｉｎ基因的５＇－脑型外显子止游区和３＇－非翻译区的两个（ＣＡ）。位点进行了扩增片段长度多态性分     

直接逆转录原位PCR检测实验性汉坦病毒感染乳鼠脑组织中病毒RNA及其与原位分子杂交的比较

出生后２～３ｄ的昆明种乳鼠,经腹腔接种１００个半数致死量的陈株汉坦病毒,每只０．０５ｍｌ,于接种后１、２、４、６、８、１０、１２、１４ｄ处死动物,每个时间点３～６只不等,取其脑组织固定于４％的多聚甲醛中,石蜡包埋制备５μｍ的连续组织切片,每时间点取１～２例组织切片,用逆转录原位ＰＣＲ（ＲＴ－ＩＳＰＣＲ）方法检测组织中病毒Ｓ片段ＲＮＡ,组织脱蜡后,经ＤＮａｓｅ、蛋白酶Ｋ、消化等予处理,用汉坦病毒ＲＮＡＳ片段特异的一对引物,在组织切片上进行病毒ＲＮＡ的逆转录和ＰＣＲ过程,直接将ｄｉｇｏｘｉｇｅｎｉｎ－１１－ｄＵＴＰ掺入到扩增产物中,经过３０个ＰＣＲ循环后,用碱性磷酸酶标记的抗ｄｉｇｏｘｉｇｅｎｉｎ抗体免疫组化检测扩增产物,连续组织切片用ｄｉｇｏｘｉｇｅｎｉｎ标记的汉坦病毒Ｍ片段Ｇ２编码区ＲＴ－ＰＣＲ扩增产物的和Ｓ片段特异性探针进行原位分子杂交并与ＲＴ－ＩＳＰＣＲ结果进行比较,另外应用免疫组化检测该基因表达产物病毒核抗原（ＮＰ）,结果,ＲＴ－ＩＳＰＣＲ在病毒感染１ｄ的乳鼠脑组织中检测到病毒ＲＮＡ扩增产物,扩增产物定位于神经细胞胞浆内,而原位分子杂交和免疫组化检测阴性。在病毒感染２ｄ及２ｄ以后的乳鼠脑组织中ＲＴ－Ｉ     

抗原捕获聚合酶链式反应（AC—PCR）直接分型检测单纯疱疹病毒

用抗单纯疱疹病毒（ＨＳＶ）型共同性ｇＣ和ｇＤ单克隆抗体（ＭｃＡｂ）,包被Ｅｐｐｅｎｄｏｒｆ管,捕捉ＨＳＶ,同时加入３个引物：一个是ＨＳＶ－１／ＨＳＶ－型共同性上游引物,另两个分别是ＨＳＶ－１和ＨＳＶ－２型特异性下游引物。借此建立了能直接分型检测ＨＳＶ的抗原捕获聚合酶链式反应（ＡＣ－ＰＣＲ）。ＨＳＶ－１的扩增产物为４７７ｂｐ,ＨＳＶ－２的为３９９ｂｐ,两型病毒经ＡＣ－ＰＣＲ扩增后产生分子量不同的ＤＮ     

水稻中编码甘油—3—磷酸转酰酶部分cDNA的克隆及序列分析

参照国外报道的几种双子叶植物的甘油－３－磷酸转酰酶的相对保守的氨基酸序列,设计并合成了一对简并引物,提取抗冷性强的水稻品种“丽梗２号”的ＲＮＡ,采用ＲＴ－ＰＣＲ技术,扩增出３１５ｂｐ的一般ｃＤＮＡ片段。扩增产物经纯化后直接克隆到ｐＧＥＭ－Ｔ载体系统中,经ＰＣＲ法鉴定,所得的重组质粒中含有３１５ｂｐ的片段。     

牛泡沫病毒（BSV）3026毒株的分离及分子生物学鉴定

从一头牛免疫缺陷病毒（ＢＩＶ）检测阳性３０２６号牛外周血中,分离到一株病毒,即３０２６病毒株。体外细胞增减和反转录分析证明,此病毒是一反转录病毒。可胎牛肺细胞中引起典型的泡沫样病变,形成合胞体,ＰＣＲ扩增和Ｓｏｕｔｈｅｍ杂交显示,此病毒的ＣＤＮＡ和ＰＣＲ产的均可与牛泡沫病毒（ＢＳＶ）阳性对照的ＨｉｒｔＤＮＡ杂交。３‘ＬＴＲ上游一段３３０ｂｐ的ＰＣＲ产物序理分析表明,３０２６毒株与ＢＳＶ阳性对照相比     

大熊猫SRY基因的PCR扩增和克隆

本文采用人ＳＲＹ基因的一对引物,通过ＰＣＲ扩增获得了雄性大熊猫ＳＲＹ基因片段。表明大熊猫存在与人ＳＲＹ基因同源的相应基因,将ＰＣＲ产物与载体ｐＵＣ－Ｅｃｏ－Ｔ连接后,用以转化ＪＭ１０９菌,经过与人ＳＲＹ基因探针菌落杂交筛选获得了大熊猫ＳＲＹ苈在克隆,命名为ｐＡＭＹ０．６,其插入片段为相应于人ＳＲＹ基因保守区在内的一段约６０９ｂｐＤＮＡ。此外,还制作和比较分析了人和大熊猫基因片段的限制酶图谱。     

一步法PCR检测大鼠肺支原体核酸的研究

一步法体外扩增结合Ｓｏｕｔｈｅｒｎ杂交检测Ｍ５３鼠肺支原体标准株,设计一对特异寡核苷酸引物及探针,合成、纯化、建立了特异、敏感、快速的检测手段。扩增产物经琼脂糖凝胶电泳鉴定,结果显示鼠肺支原体Ｍ５３株基因组ＤＮＡ７１０ｂｐ特异谱带。对５０只ＳＤ大鼠进行检测,结果ＰＣＲ方法检出率高于分离培养法,扩增产物行Ｓｏｕｔｈｅｒｎｂｌｏｔ杂交验证,采用碱性磷酸酶标记寡核苷酸探针,可与膜上特异靶ＤＮＡ序列杂交,而阴性对照无杂交信号。特异性实验检出１０ｐｇ的ＤＮＡ。充分说明一步法ＰＣＲ,具有高度、特异、灵敏、快速等优势,适应与大、小鼠监测中应用。     

PCR和生物素探针对HFRSV的检测和分型的探讨

分析比较肾综合征出血热病毒（ＨＦＲＳＶ）７６／１１８株和Ｒ＿（２２）株的核苷酸序列,根据引物设计原则及检测分型的目的,设计并合成了３对引物。１对引物取于两毒株间的高同源区段,作为共同引物和外引物;另两对引物取于两毒株间的低同源区段,分别作为野鼠型引物、家鼠型引物和内引物。建立了ＤＮＡ聚合酶链反应（ＰＣＲ）和ＮｅｓｔＰＣＲ方法,并用ＮｃｓｔＰＣＲ合成了两种型特异的生物素探针。ＰＣＲ检测７６／１１８、Ａ＿９、陈、Ｒ＿２、Ｒ＿２２５个毒株,用外引物时均扩增出１条约３００ｂｐ的条带;用内引物的野鼠型引物时,除Ｒ＿（２２）株之外,其余４株均扩增出１条约７０ｂｐ的条带。斑点杂交试验证实了ＰＣＲ检测分型的准确性。ＮｅｓｔＰＣＲ和生物素探针斑点杂交试验可以测出１－１０ｂｇ的目的ｃＤＮＡ。     

Real time PCR hybridization for the rapid and specific identification of Francisella tularensis

Tularemia is highly infectious and fatal zoonotic disease caused by Gram negative bacteria Francisella tularensis. The necessity to undergo medical treatment in early phase of illness in humans and possibility of making use of bacterial aerosol by terrorists in an attack create an urgent need to implement a rapid and effective method which enables to identify the agent. In our study two primers FopA F/R and hybridization probes FopA S1/S2 designed from fopA gene sequence, were tested for their potential applicability to identify F. tularensis. In this research 50 strains of F. tularensis were used and the test gave positive results. Reaction specificity was confirmed by using of non-Francisella tularensis bacterial species. The results obtained in the real-time PCR reaction with primers Tul4 F/R and hybridization probes Tul4 S1/S2, designed from tul4 gene, were comparable to the results from previous experiment with fopA - primers set. Investigation of fopA and tul4 primers and hybridization probes properties revealed characteristic Tm (melting temperature) value of the products--61 degrees C and 60 degrees C, respectively. Detection sensitivity was remarkably higher when fopA primers set was used 1 fg/microl, and for tul4 primers set, minimal detectable concentration is 10 fg/microl.     

Detection of diverse new Francisella-like bacteria in environmental samples

Following detection of putative Francisella species in aerosol samples from Houston, Texas, we surveyed soil and water samples from the area for the agent of tularemia, Francisella tularensis, and related species. The initial survey used 16S rRNA gene primers to detect Francisella species and related organisms by PCR amplification of DNA extracts from environmental samples. This analysis indicated that sequences related to Francisella were present in one water and seven soil samples. This is the first report of the detection of Francisella-related species in soil samples by DNA-based methods. Cloning and sequencing of PCR products indicated the presence of a wide variety of Francisella-related species. Sequences from two soil samples were 99.9% similar to previously reported sequences from F. tularensis isolates and may represent new subspecies. Additional analyses with primer sets developed for detection and differentiation of F. tularensis subspecies support the finding of very close relatives to known F. tularensis strains in some samples. While the pathogenicity of these organisms is unknown, they have the potential to be detected in F. tularensis-specific assays. Similarly, a potential new subspecies of Francisella philomiragia was identified. The majority of sequences obtained, while more similar to those of Francisella than to any other genus, were phylogenetically distinct from known species and formed several new clades potentially representing new species or genera. The results of this study revise our understanding of the diversity and distribution of Francisella and have implications for tularemia epidemiology and our ability to detect bioterrorist activities.     

应用TaqMan荧光定量PCR检测土拉弗朗西斯菌

目的：利用Roche LightCycler实时定量PCR系统建立一种快速、灵敏、特异的检测土拉弗朗西斯菌的方法。方法：基于TaqMan荧光探针实时定量PCR技术,选择土拉弗朗西斯菌染色体上的特异序列[醇醛酮还原酶（AKR）和外膜蛋白FopA基因]作为检测靶序列,建立土拉弗朗西斯菌实时定量PCR检测方法;评价该检测方法的特异性和灵敏性;采用克隆菌株污染环境土壤来模拟实际样品,评价该检测方法在快速检测与现场检测等实际应用中的表现。结果：优化筛选基因组中的FT-AKR和FT-fopA片段作为检测靶序列,所建立的土拉弗朗西斯菌实时定量PCR检测方法检测克隆菌株质粒的灵敏度均为10个拷贝/每个反应体系;以其他非土拉弗朗西斯菌为模板未出现非特异扩增;模拟环境土壤样品检测灵敏度2个引物对分别为440和960CFU/g土壤;盲测实验结果显示对于灵敏度范围内的阳性样本均能正确识别,并能正确检测出不同浓度的阳性样本。以FT-fopA片段为靶序列的扩增效率不及基于FT-AKR引物对的扩增。结论：基于FT-AKR片段的引物对扩增效率高,检测土拉弗朗西斯菌具有特异、灵敏的特点,对临床诊断、环境污染监测、防治生物突发事件等具有重要意义。     

Comparison of three different PCR methods for detection of Brucella spp in human blood samples

In the diagnosis of human brucellosis, PCR could be a more sensitive technique than blood cultures and more specific than conventional serological tests. We compared three different PCR methods for the detection of Brucella spp. and we studied whether human genomic DNA affect the sensitivity of three primer pairs for the detection of Brucella DNA in a peripheral-blood PCR assay. These three pairs of primers amplified three different fragments included in: (i). a gene encoding a 31-kDa Brucella abortus antigen (primers B4/B5), (ii). a sequence 16S rRNA of B. abortus (primers F4/R2), and (iii). a gene encoding an outer membrane protein (omp-2) (primers JPF/JPR). The three primers assayed showed a difference in sensitivity for detecting purified Brucella DNA, ranging between 8 fg and 20 pg. However, the sensitivity of the primers F4/R2 and B4/B5 was affected by the presence of human DNA while the primers JPF/JPR were not. Therefore, although the sensitivity of PCR using primers F4/R2 is affected by human DNA, they are still the most sensitive and they could provide a useful tool for the diagnosis of human brucellosis.     

金标银染免疫渗滤法检测土拉弗朗西斯菌

目的:建立金标银染免疫渗滤法检测土拉弗朗西斯菌(土拉菌)的方法,评价其灵敏度、特异性、重复性及其应用。方法:以小鼠抗土拉菌脂多糖单克隆抗体作为捕获抗体包被硝酸纤维素膜、兔抗土拉菌多克隆抗体作为检测抗体标记胶体金,通过金标银染技术放大检测信号,建立金标银染免疫渗滤法检测土拉弗朗西斯菌体系;评价该方法的灵敏度、特异性和重复性;以经荧光定量PCR定量的土拉弗朗西斯菌为检测对象,比较金标银染免疫渗滤法和免疫层析法。结果:金标银染免疫渗滤法检测土拉弗朗西斯菌的最小检出量为1.0×103 CFU/mL,灵敏度高于免疫层析法;检测大肠杆菌、炭疽芽孢杆菌、布鲁菌和鼠疫耶尔森菌的结果均为阴性;密封保存的检测卡80 d内重复性良好,100 d后反应强度略有降低。结论:金标银染免疫渗滤法检测土拉弗朗西斯菌敏感性高、特异性强、重复性好,且方便快捷,不需要仪器设备,可作为快速检测土拉弗朗西斯菌的首选方法。     

Paired-end sequence mapping detects extensive genomic rearrangement and translocation during divergence of Francisella tularensis subsp. tularensis and Francisella tularensis subsp. holarctica populations

Comparative genome hybridization of the Francisella tularensis subsp. tularensis and F. tularensis subsp. holarctica populations have shown that genome content is highly conserved, with relatively few genes in the F. tularensis subsp. tularensis genome being absent in other F. tularensis subspecies. To determine if organization of the genome differs between global populations of F. tularensis subsp. tularensis and F. tularensis subsp. holarctica, we have used paired-end sequence mapping (PESM) to identify regions of the genome where synteny is broken. The PESM approach compares the physical distances between paired-end sequencing reads of a library of a wild-type reference F. tularensis subsp. holarctica strain to the predicted lengths between the reads based on map coordinates of two different F. tularensis genome sequences. A total of 17 different continuous regions were identified in the F. tularensis subsp. holarctica genome (CR(holar)(c)(tica)) which are noncontiguous in the F. tularensis subsp. tularensis genome. Six of the 17 different CR(holarctica) are positioned as adjacent pairs in the F. tularensis subsp. tularensis genome sequence but are translocated in F. tularensis subsp. holarctica, implying that their arrangements are ancestral in F. tularensis subsp. tularensis and derived in F. tularensis subsp. holarctica. PCR analysis of the CR(holarctica) in 88 additional F. tularensis subsp. tularensis and F. tularensis subsp. holarctica isolates showed that the arrangements of the CR(holarctica) are highly conserved, particularly in F. tularensis subsp. holarctica, consistent with the hypothesis that global populations of F. tularensis subsp. holarctica have recently experienced a periodic selection event or they have emerged from a recent clonal expansion. Two unique F. tularensis subsp. tularensis-like strains were also observed which likely are derived from evolutionary intermediates and may represent a new taxonomic unit.     

Identification of Francisella tularensis in natural water samples by PCR

Abstract Francisella tularensis , the causative agent of the epizootic disease tularemia in mammals, can be isolated from mud and water. To study the spread and persistence of Francisella tularensis in water, different strategies for pre-treatment of natural water samples prior to identification of the bacterium by polymerase chain reaction (PCR) were evaluated. A method for handling of samples taken from natural waters was developed. Applied on natural water samples amended with F. tularensis , the method rendered identification by PCR reproducible and it resulted in an amplified Francisella -specific product in all samples from natural waters tested. In addition, by employing primers targeting conserved regions of the 16S rDNA the presence of bacteria was demonstrated in all samples investigated. The results presented will, in combination with other techniques that allow identification, improve studies on the epizootiology and epidemiology of the genus Francisella .     

土拉弗朗西斯菌检测研究进展

土拉弗朗西斯菌（Francisella tularensis）是土拉菌病（Tularemia）的致病菌,是最具传染性的致病菌之一,在自然界中已发现一百种以上的动物感染此菌。因其传播途径多样,易扩散、毒性强而被美国疾病控制预防中心列入A类生物恐怖制剂。土拉菌病是一种人畜共患病,致死率高,及时、准确的检测土拉菌对于土拉菌病患者及时治疗和防止扩散具有重要的意义。土拉菌检测方法很多,如菌培养,微凝集实验、酶联免疫吸附、快速检测试纸条、生物传感器、PCR、核酸杂交检测、质谱分析、基因芯片等。但到目前为止还没有一种成熟的用于土拉菌检测方法,其主要原因在于土拉菌致病性强,且不易分离培养。本文综述了土拉菌细菌学、免疫学、分子生物学方法检测的最新研究进展。     

Identification of Francisella species and discrimination of type A and type B strains of F. tularensis by 16S rRNA analysis.

Tularemia is a zoonotic disease, occurring throughout the Northern Hemisphere. The causative agent, the bacterium Francisella tularensis, is represented by two main types. Type A is found in North America, whereas type B is mainly found in Asia and Europe and to a minor extent in North America. No routine technique for rapid diagnosis of tularemia has been generally applied. We have partially sequenced 16S rRNAs of two F. tularensis strains, as well as the closely related Francisella novicida. Of 550 nucleotides analyzed, only one difference in 16S rRNA primary sequence was found. This 16S rRNA analysis enabled the construction of oligonucleotides to be used as genus- and type-specific probes. Such probes were utilized for the establishment of a method for rapid and selective detection of the organism. This method allowed identification of Francisella spp. at the level of genus and also discrimination of type A and type B strains of F. tularensis. The analysis also permitted the detection of F. tularensis in spleen tissue from mice infected with the bacterium. The results presented will enable studies on the epizootiology and epidemiology of Francisella spp.     

Development and comparison of two assay formats for parallel detection of four biothreat pathogens by using suspension microarrays

Microarrays provide a powerful analytical tool for the simultaneous detection of multiple pathogens. We developed diagnostic suspension microarrays for sensitive and specific detection of the biothreat pathogens Bacillus anthracis, Yersinia pestis, Francisella tularensis and Coxiella burnetii. Two assay chemistries for amplification and labeling were developed, one method using direct hybridization and the other using target-specific primer extension, combined with hybridization to universal arrays. Asymmetric PCR products for both assay chemistries were produced by using a multiplex asymmetric PCR amplifying 16 DNA signatures (16-plex). The performances of both assay chemistries were compared and their advantages and disadvantages are discussed. The developed microarrays detected multiple signature sequences and an internal control which made it possible to confidently identify the targeted pathogens and assess their virulence potential. The microarrays were highly specific and detected various strains of the targeted pathogens. Detection limits for the different pathogen signatures were similar or slightly higher compared to real-time PCR. Probit analysis showed that even a few genomic copies could be detected with 95% confidence. The microarrays detected DNA from different pathogens mixed in different ratios and from spiked or naturally contaminated samples. The assays that were developed have a potential for application in surveillance and diagnostics.