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1.
应用PCR技术扩增出HBV DNA C基因片段并与pAT153质粒重组,转化到E.coli RRI中,经体内扩增,提纯,用光生物系标记,制备了C基因的重组质粒探针。该探检测灵敏度在Southern印迹中达1pg,在点印迹中为5pg。用此探针以Southern印迹方式配合PCR技术检测乙肝病人血清中的HBV DNA,在53例PCR产物电泳检测阴性的样品中,Southern杂交又检出18例阳性。 相似文献
2.
制备CVB3结构蛋白和非结构蛋白重组质粒DNA疫苗时,采用RT-PCR从CVB感染的HeLa细胞中扩增VP1、VP2、2A和3D基因,重组入真核表达质粒pcDNA3中,构建pcDNA3/VP2、pcDNA3/VP1、pcDNA3/2A和pcDNA3/3D重组质粒,经酶切和测下实扩增的序列并将各重组质粒体外转染真核细胞COS-7,用RT-PCR检测mRNA的转录,用Western-blot检测表达产物。结果4种重组质粒酶切出相应大小的目的片段,经测序证实为CVB3相应序列,Western-blot证实能够在体外真核细胞中表达。本文成功构建CVB3结构与非结构蛋白的重组质粒DNA疫苗,为进一步研究其免疫效果奠定了基础。 相似文献
3.
用PCR扩增和克隆马立克氏病病毒糖蛋白D基因 总被引:2,自引:0,他引:2
用PCR技术,从GA株马立克氏病病毒(MDV)感染的成纤维细胞(GEF)基因组DNA中扩增出MDV糖蛋白D(gD)抗原基因片段的约1300bp编码序列,将该pcR扩增的产物于EcoRI和Kpnl位点克隆到pUC18质粒载体中,在以digoxigenin(dig)标记的gDPCR产物作为探针,进行原位杂交初步筛选到阳性重组质粒克隆,再根据酶切分析筛选到含MDVgD基因的重组质粒p18MgD。将p18MgD质粒DNA用dig标记后,在Southernblot中,该探针能识别MDV基因组DNA的BamHI-A克隆中的A片段DNA。酶切位点分析表明,该gD克隆也和已发表的MDV的RBIB株gD一样,不含有EcoRⅠ、HindⅢ、PstⅠ、SmaⅠ、pvuⅡ等酶切位点。证明该重组质粒是MDVgD克隆。 相似文献
4.
应用PCR技术定向克隆了细小病毒H-1的非结构蛋白(NS)部分基因片段。自行设计并合成了PCR引物△P3和△P4,在两个引物中分别引入两个突变碱基,使扩增后的DNA片段的两端含有限制性核酸内切酶HindⅢ或BamHI的酶切位点,经双酿切法把该DNA片段重组到pUC118质粒中。对插入片段的DNA序列测定和分析结果证实该片段为H-1NS-1基因序列。以此重组质粒为探针,采用分子杂交的方法,分别测定了H-1及MVMDNA在细胞内的复制水平。这一基因的克隆为制备H-1的质量监测、H-1及MVMNS-1蛋白抑瘤作用机理及其在肿瘤细胞及正常组织中的转录表达等研究奠定了基础。 相似文献
5.
本文利用HBV DNA基因组preC和C区的一套引物,以PCR法检测了26例健康正常人血清和95例免疫标志各异、临床症状不同的乙肝或可疑乙肝患者的血清,前者无1例检出HBV DNA,后者共检出的66例血 清存在HBV DNA。该方法特异性强,适用于检测任一亚型的HBV DNA,一轮PCR最低可检出0.1pg的HBV DNA。 相似文献
6.
HBV-DNA的PCR二步法扩增及其快速检测方勤,吴云涛,蔡宜权(中国科学院武汉病毒研究所,武汉430071)关键词HBV-DNA,二步温控PCR,Southern杂交,生物素寡聚核苷酸杂交乙型肝炎是危害人类健康的主要疾病之一,其病原常用的检测方法多... 相似文献
7.
从我国内蒙古地区流行的犬细小病毒病病犬的肠溶物中分离提纯犬细小病毒(CPV)。提取病毒基因组DNA,并以此DNA为模板,采用人工合成的引物进行PCR扩增,PCR产物经BamHI、SacI双酶切后,克隆于pUC19质粒的BamHI/SacI位点。重组质粒pUCVP2经PCR鉴定、限制酶切分析和序列分析,结果表明:获得了犬细小病毒内蒙株(CPV-IM)VP2基因的全长克隆,VP2基因全长1755nt, 相似文献
8.
以p53cDNA为探针,用Southern印迹法对人胃癌细胞系BGC823进行了检测,发现该细胞中p53基因存在异常,将可在真核细胞表达的重组野生型P53质粒pC53-SN3和突变型p53质粒pC53-SCX3,用指质体介导法,分别导入BCG823细胞,获得了较长时间受G418的多个阳性克隆。Southern抑迹法证实阳性克隆细胞中有外源性p53基因存在。 相似文献
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10.
介绍了一种从人血清中同步扩增和检测HBV-DNA和HCV-RNA的方法。HCV-RNA反转录成cDNA,这种cDNA和从HBV中抽提出的DNA一起,用根据HBV、HCV保守区序列设计的特异引物进行同步PCR扩增,这种方法对于检测HBV和HCV重复感染很有用处 相似文献
11.
化学发光Southern blot法检测HBV体外复制及其应用于药物对HBV的抑制分析 总被引:1,自引:0,他引:1
目的:建立化学发光Southern blot检测细胞内HBV DNA的方法,同时检测3种不同靶点抗乙肝药物的体外作用。方法:用地高辛标记HBV探针,优化杂交条件,检测来自HepG2及HepG2.2.15 HBV DNA复制中间体;利用建立的化学发光Southern blot检测HBV DNA的方法检测经拉米夫定、Bay41-4109、α-Galcer以不同药物浓度处理的HepG2.2.15HBV DNA复制中间体的水平。结果:(1)标记的HBV探针的检测灵敏度为0.1pg,杂交系统的检测灵敏度为1pg,可检测到HepG2.2.15细胞内的HBV DNA特异性信号;(2)以该法检测胞内HBV DNA可见3种药物都有明显的抑制作用,其半数有效量(IC50)分别为1.53μmol/L、0.41μmol/L、0.01μmol/L。结论:胞质HBV DNA的水平能准确地反映不同靶点抗HBV药物的抗病毒效果,建议在观察药物特别是中药抗病毒研究中采用。 相似文献
12.
异羟基洋地黄毒甙元(Digoxigenin)标记的探针在乙型肝炎病毒核酸杂交中的应用 总被引:1,自引:0,他引:1
应用异羟基洋地黄毒甙元标记的探针,检测了人和鸭的血清及肝脏中的乙型肝炎病毒核酸,并与~(32)P标记的同位素探针做了比较。结果证明,该探针的特异性和敏感性与同位素探针一致(0.2pg)。它可用于各种核酸杂交试验,如打点杂交、Southern和Northern转印杂交试验等。恰当地从标本中提取待测核酸,是应用该探针的重要条件。 相似文献
13.
The aim of this study was to develop Prevotella intermedia-specific PCR primers based on the P. intermedia-specific DNA probe. The P. intermedia-specific DNA probe was screened by inverted dot blot hybridization and confirmed by Southern blot hybridization. The nucleotide sequences of the species-specific DNA probes were determined using a chain termination method. Southern blot analysis showed that the DNA probe, Pig27, detected only the genomic DNA of P. intermedia strains. PCR showed that the PCR primers, Pin-F1/Pin-R1, had species-specificity for P. intermedia. The detection limits of the PCR primer sets were 0.4 pg of the purified genomic DNA of P. intermedia ATCC 49046. These results suggest that the PCR primers, Pin-F1/Pin-R1, could be useful in the detection of P. intermedia as well as in the development of a PCR kit in epidemiological studies related to periodontal diseases. 相似文献
14.
Parasite DNA amplified by PCR from blood of 73 chagasic children and adults of two endemic areas of Chile were studied by Southern blot and/or dot blot hybridization analysis with a panel of three minicircle probes corresponding to the parasite genotypes (clonets 19, 33 and 39). The hybridization pattern of the PCR positive samples identified clonets 39, 19/20, and 32/33 with frequencies of 0.84, 0.32 and 0.26, respectively. A total of 31 samples corresponded to mixed infections. The most frequently found mixtures were: clonets 39 and 19/20 (14 cases), followed by clonets 39 and 32/33 (8 cases), clonets 39, 32/33 and 19/20 (8 cases), and clonets 32/33 and 19/20 (1 case). Amplified DNA from 9 cases showed no hybridization signal with none of the three studied probes indicating that other genotypes different to the ones mentioned are circulating in humans, but that the clonets used as probes are the most prevalent ones in terms of transmission in the endemic areas studied. A biological characterization of 34 T. cruzi populations isolated from the xenodiagnosis of the patients was performed on an experimental murine model. The biochemical characterization of the parasite populations by molecular karyotype determined that the most frequent parasite isolated from patients belongs to clonet 39. 相似文献
15.
Identification of Aeromonas hydrophila hybridization group 1 by PCR assays. 总被引:5,自引:0,他引:5 
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下载免费PDF全文 A Cascn J Anguita C Hernanz M Snchez M Fernndez G Naharro 《Applied microbiology》1996,62(4):1167-1170
Synthetic oligonucleotide primers of 24 and 23 bases were used in a PCR assay to amplify a sequence of the lip gene, which encodes a thermostable extracellular lipase of Aeromonas hydrophila. A DNA fragment of approximately 760 bp was amplified from both sources, i.e., lysed A. hydrophila cells and isolated DNA. The amplified sequence was detected in ethidium bromide-stained agarose gels or by Southern blot analysis with an internal HindIII-BamHI 356-bp fragment as a hybridization probe. With A. hydrophila cells, the sensitivity of the PCR assay was < 10 CFU, and with the isolated target, the lower detection limit was 0.89 pg of DNA. Primer specificity for A. hydrophila was determined by the PCR assay with cells of 50 strains of bacteria, including most of the 14 currently recognized DNA hybridization groups of Aeromonas spp. as well as other human and environmental Aeromonas isolates. Detection of A. hydrophila by PCR amplification of DNA has great potential for rapid identification of this bacterium because it has proved to be highly specific. 相似文献
16.
We have established a method for amplifying and obtaining large quantities of chromosome-specific DNA by linker/adaptor ligation and polymerase chain reaction (PCR). Small quantities of DNA isolated from flow cytometry-sorted chromosomes 17 and 21 were digested with MboI, ligated to a linker/adaptor, and then subjected to 35 cycles of PCR. Using this procedure, 20 micrograms of chromosome-specific DNA can be obtained. Southern blot analysis using several DNA probes previously localized to chromosomes 17 and 21 indicated that these gene sequences were present in the amplified chromosome-specific DNA. A small quantity of the chromosome-specific DNA obtained from the first round of PCR amplification was used to amplify DNA for a second, third, and fourth round of PCR (30 cycles), and specific DNA sequences were still detectable. Fluorescence in situ hybridization using these chromosome-specific DNA probes clearly indicated the hybridization signals to the designated chromosomes. We showed that PCR-amplified chromosome 17-specific DNA can be used to detect nonrandom chromosomal translocation of t(15;17) in acute promyelocytic leukemia by fluorescence in situ hybridization. 相似文献
17.
《Research in virology》1991,142(5):373-379
Serum hepatitis B virus DNA (HBV DNA) is now the most important and reliable marker for monitoring viral replication. Quantitative detection of HBV DNA in serum is based on a commercial standardized solution hybridization assay (Genostics). In this work, we studied the sensitivity and specificity of this method, in comparison with the polymerase chain reaction (PCR) technique, for low-value HBV DNA serum samples. Fifty-four patients with or without HBV serological markers were divided into 4 groups according to their HBV DNA values.Genomic amplication was found to affect 2 conserved regions of the viral genome, the S and C regions. Samples with an HBV DNA concentration equal to or greater than 1.5 pg/ml were considered positive in the “Genostics” test. A total of 38% of patients considered negative in the quantitative assay (< 1.5 pg/ml) were found to be positive for HBV DNA in serum after PCR. Only 26% of patients with an HBV DNA concentration of between 1.5 and 10 pg/ml in the Genostics test had PCR-detectable viral DNA in serum. Some 56% of patients with HBV DNA values between 10 and 20 pg/ml were found to be positive after amplification. All patients whose HBV DNA values were above 20 pg/ml had PCR-detectable viral DNA in serum.Our PCR results suggest that the positive limit level of the Genostics test has to be re-evaluated. Indeed, for low values of HBV DNA (under 20 pg/ml and especially under 10 pg/ml), it is not possible to conclude about the positivity from the quantitative assay, and results have to be estimated according to the clinical and serological status of the patients. Moreover, PCR can be falsely negative because of methodological problems.Nevertheless, this study confirms that PCR does enable detection of the viral genome in HBV-seronegative patients and in “old” and “cured” HBV-infection marker carriers. 相似文献
18.
A simple method to create a chromosome-specific DNA librqary of rice,including microdissection,amplification,charterization and cloning,is described.Rice chromosome 4 from a metaphase cell has been isolated and amplified by the Linker Adapter PCR (LA-PCR).The PCR products were labeled as probes with DIG-11-dUTP using the random priming method.Southern blot analysis with rice genomic DNA and specific RFLP markers demonstrated that the PCR products were derived from rice chromosome 4.A large library comprising over 100,000 recombinant plasmid microclones from rice chromosome 4 was constructed.Colony hybridization showed that 58% of the clones contained single or low-copy sequences and 42% contained repetitive sequences.The size of inserts generated by PCR ranged from 140bp to 500bp.This method will facilitate cloning of the specific chromosome DNA markers and important genes of rice. 相似文献
19.
Manca N Viani I Perandin F Piccolo G Calderaro A Galati L Ricci L Dettori G Turano A Chezzi C 《The new microbiologica》2000,23(3):339-346
The present study evaluates the sensitivity, specificity and usefulness of a PCR method with Southern blot hybridization to detect malaria parasites in blood samples from subjects with a suspect clinical diagnosis of malaria imported to Italy. Plasmodia were detected by PCR using a genus-specific primer-set corresponding to the sequences common to P. falciparum, P. vivax, P. malariae and P. ovale, as described by Arai (Arai et al., Nucleosides Nucleotides, 1994, 13, 1363-1364) and Kimura (Kimura et al., Journal of Clinical Microbiology, 1995, 33, 2342-2346). In addition, four distinct tandemly repetitive species-specific probes, described by Kawai (Kawai et al., Analytical Biochimestry, 1993, 209, 63-69), were synthesized to specifically detect the four malaria parasites species by Southern blot hybridization. Fifteen blood samples from 12 patients (7 with malaria) were tested and the genus-specific PCR method showed a sensitivity of 100% and a specificity of 100%, when compared to microscopy, in detecting malaria parasites in the tested blood samples. Fourteen samples (nine were positive and five negative by PCR) were confirmed by Southern blot, whereas only one P. vivax positive sample was not hybridized with the species-specific probes. We conclude that this PCR method with Southern blot hybridization may be useful in detecting malaria parasites in patients with malaria imported to Italy. 相似文献