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目的建立检测博尔纳病病毒(BDV)RNA的原位PCR方法。方法首先设计BDV特异性引物以及检测BDV-RNA的原位PCR扩增系统.然后对BDV持续感染细胞(BDV/OL)和正常细胞(OL细胞)爬片进行原位PCR扩增,进而分别用DNA酶或RNA酶消化处理BDV/OL细胞爬片后,再进行原位PCR扩增。结果经原位PCR扩增后.约60%~70%的BDV持续感染细胞核中出现了阳性反应信号,但正常细胞无信号出现,并且病毒感染细胞中的阳性信号在RNA酶消化作用下消失,但不受DNA酶作用的影响。结论该研究建立的PCR检测方法具有BDV和RNA特异性,可以应用于检测相关动物或神经精神疾病患者的脑组织中BDV-RNA,为进一步证明BDV的致病性奠定基础。 相似文献
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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� 相似文献
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本文选取Wistar大鼠作为实验对象,从微生态学角度初步探索了大鼠口腔菌群的测定技术。文中探讨了大鼠活体取菌方法,初步确立口腔优势菌属,摸索出以纸片法取菌滴种培养基的最佳稀释度及四种口腔优势菌定量检测结果,为开展口腔微生态学的研究提供一定参考。 相似文献
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目的建立检测博尔纳病病毒(BDV)RNA的3′RACE(rapid amplification of cDNA ends)方法。方法根据已知的BDV p40基因序列设计上游引物sp1;提取BDV(H1766株)持续感染OL细胞的总RNA,用引物sp1和oligo dT进行3′RACE扩增,将PCR产物克隆到pGEM-T载体并转化到大肠埃希菌中,制备阳性菌落的目的质粒,进行序列测定和同源性比对;同时对检测BDV RNA的3′RACE方法的特异性和敏感性进行分析。结果建立了检测BDV RNA的3′RACE技术;所获得的BDV p40基因的3′末端扩增产物的核苷酸序列与已知BDV(H1766株)p40基因的核苷酸序列同源性为100%;本方法对BDV RNA(mRNA)具有特异性,但对BDV p40基因重组质粒无扩增结果;并且可以检测到0.04 ng以上含量的BDV感染细胞的总RNA。结论检测BDV RNA的3′RACE技术可以排除实验室污染造成的BDV基因扩增的假阳性,并可用于进一步分析BDV基因序列的特点以及评价BDV相关基因的表达情况。 相似文献
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博尔纳病病毒及其分子生物学研究进展 总被引:1,自引:0,他引:1
博尔纳病病毒(Borna disease virus,BDV)是一种嗜神经病毒,它能引起动物的进行性脑脊髓灰质炎(博尔纳疾病[1,2]。) 相似文献
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目的分析博尔纳病病毒(Borna disease virus,BDV)H1766株对BALB/c小鼠的感染性。方法选择病毒滴度为2.0×107FFU/ml的BDV病毒液分别对新生和成年BALB/c小鼠进行脑内接种,并用相同病毒液对原代培养的新生BALB/c小鼠脑细胞进行接种。经过一定时间的病毒作用后分别提取总RNA,采用巢式RT-PCR方法检测BDV-p40基因,并通过免疫组化方法检测脑内接种脑组织中BDV-P40蛋白。结果脑内接种病毒的小鼠脑组织中可以检测到BDV-p40基因和BDV-P40蛋白,培养的小鼠脑细胞中可以检测到BDV-p40基因。结论BDVH1766株可以感染新生和成年的BALB/c小鼠。 相似文献
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PDGF在大鼠断层供皮区创面愈合过程中表达变化的研究 总被引:2,自引:0,他引:2
实验研究已经证明Platelet-derivedgrowthfactor(PDGF)能够促进各种类型的伤口愈合,然而在伤口愈合过程中内源性PDGF表达变化的研究却少有报道,为探讨PDGF对伤口愈合的影响,我们应用原位杂交、斑点杂交技术观察了内源性PDGF在大鼠创面愈合过程中的表达变化,结果发现:在创面愈合过程中,肉芽组织中的成纤维细胞,毛细血管内皮细胞及创缘真皮内的毛囊上皮细胞均能表达PDGF-BB基因,在伤后6天,组织修复的高峰期,PDGF-BB基因表达达到最强,伤后12天,伤口完全上皮化,PDGF的基因表达也恢复正常,说明PDGF的基因表达和伤口愈合时间有密切的关系。提示PDGF在创面愈合过程中可能起着重要的调控作用。 相似文献
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侧脑室接种隐球菌感染大鼠模型的脑组织含水量变化研究 总被引:1,自引:0,他引:1
目的探讨隐球菌中枢神经系统感染大鼠模型的脑组织含水量变化。方法侧脑室接种隐球菌构建中枢神经系统隐球菌感染的大鼠模型,大鼠随机分为实验组和对照组,实验组大鼠侧脑室注射隐球菌菌悬液,对照组大鼠侧脑室注射生理盐水。两组分别采用干湿重法于6h、12h、24h、48h、72h动态检测大鼠脑组织含水量的变化。结果大鼠隐球菌中枢神经系统感染后,脑组织含水量于6h开始明显升高,12h到达高峰,后逐渐下降,但仍明显高于对照组;与对照组差异有统计学意义。结论隐球菌中枢神经系统感染后的大鼠脑组织含水量与对照组差异明显。 相似文献
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本实验采用地高辛标记前胰岛素寡核苷酸探针原位杂交组织化学技术,研究了Wistar大鼠胰腺组织胰岛素基因的表达。实验用Wistar大鼠5只,胰腺经4%多聚甲醛灌注固定,并在同一固定液中后固定24h,常规石蜡包埋切片。结果表明,经前胰岛素寡核苷酸探针杂交的胰腺切片中,胰岛B细胞呈蓝色。杂交反应物位于B细胞的细胞质和部分核仁中,胞核无色。胰岛其它细胞及胰腺外分泌部腺泡细胞无杂交反应物。对照切片中均无阳性信号出现。结果表明地高辛标记寡核苷酸探针不仅具备非同位素标记探针的优点而且能精确检测特异性mRNA的表达。本研究方法操作便利,可靠精确,重复性好。 相似文献
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Detection of Borna disease virus (BDV) antibodies and BDV RNA in psychiatric patients: evidence for high sequence conservation of human blood-derived BDV RNA. 总被引:13,自引:2,他引:11 
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下载免费PDF全文 C Sauder A Müller B Cubitt J Mayer J Steinmetz W Trabert B Ziegler K Wanke N Mueller-Lantzsch J C de la Torre F A Grsser 《Journal of virology》1996,70(11):7713-7724
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Visualization of single copies of the Epstein-Barr virus genome by in situ hybridization 总被引:5,自引:0,他引:5
Conditions have been established for demonstrating small numbers of genes of the Epstein-Barr virus (EBV) in B-lymphoid cells by in situ hybridization using biotinylated EBV-specific DNA from cloned BamHI fragments of the viral genome. Single copies of EBV genomes were successfully visualized with minimal background when the probe concentration was 0.2 micrograms/ml, the DNA denaturation step was performed at 100 degrees C, and the immunochemical detection system employed a three-layer peroxidase protocol with gold-silver amplification of the diaminobenzidine substrate. The minimal target DNA detectable was about 10 kilobase pairs. In the case of sectioned cells fixed overnight with formalin, simulating conditions used in routine tissue fixation, this approach failed to demonstrate EBV DNA present at less than 100 copies per cell, that is, at the level found in Raji cells. However, when denaturation was performed using microwave irradiation with the other optimized conditions maintained, EBV DNA could be visualized in 10-20% of such cells, although not in cells known to contain fewer than 10 copies per cell. Thus, microwave irradiation partially overcomes the limit of DNA target detection imposed by formalin. 相似文献
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In situ hybridization was used to detect Epstein-Barr virus (EBV) DNA sequences under conditions where the virus DNA is replicating spontaneously and where it is induced to do so following superinfection. The in situ reaction itself is influenced by several parameters, analogous to conventional nucleic acid hybridization, consideration of which should help to optimize the designing of in situ hybridization reactions in general. Both EBV complementary RNA (cRNA) and EBV DNA synthesized in vitro can efficiently detect the virus DNA sequences in situ. The findings presented here can therefore be utilized in both the study of EBV-cell interactions and, more generally, in studies using in situ hybridization as a general approach. 相似文献
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Nakamura Y Takahashi H Shoya Y Nakaya T Watanabe M Tomonaga K Iwahashi K Ameno K Momiyama N Taniyama H Sata T Kurata T de la Torre JC Ikuta K 《Journal of virology》2000,74(10):4601-4611
Serological and molecular epidemiological studies indicate that Borna disease virus (BDV) can infect humans and is possibly associated with certain neuropsychiatric disorders. We examined brain tissue collected at autopsy from four schizophrenic patients and two healthy controls for the presence of BDV markers in 12 different brain regions. BDV RNA and antigen was detected in four brain regions of a BDV-seropositive schizophrenic patient (P2) with a very recent (2 years) onset of disease. BDV markers exhibited a regionally localized distribution. BDV RNA was found in newborn Mongolian gerbils intracranially inoculated with homogenates from BDV-positive brain regions of P2. Human oligodendroglia (OL) cells inoculated with brain homogenates from BDV-positive gerbils allowed propagation and isolation of BDVHuP2br, a human brain-derived BDV. Virus isolation was also possible by transfection of Vero cells with ribonucleoprotein complexes prepared from BDV-positive human and gerbil brain tissues. BDVHuP2br was genetically closely related to but distinct from previously reported human- and animal-derived BDV sequences. 相似文献