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PCR检测鼠疫耶尔森氏菌研究进展 总被引:3,自引:0,他引:3
快速确诊鼠疫对鼠疫的防治工作至关重要。传统的细菌学“四步检查法”和血清学方法检测虽可确诊鼠疫,但存在烦琐、费时、费用高、不能进行快速诊断等弊病。PCR方法具有快速、特异、敏感的特点,尤其对培养条件苛刻、生长缓慢或已死亡的病原体检测优势更为明显,国内外学者现已建立了多种PCR方法用于鼠疫的检测,鼠疫PCR方法简便安全,是流行病学调查和紧急情况下检测鼠疫的有力手段。 相似文献
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鼠疫耶尔森氏菌LcrV(V抗原)的研究进展 总被引:6,自引:0,他引:6
鼠疫耶尔森氏菌作为鼠疫的病原菌,致病机制十分复杂,其中LcrV(V抗原)是最早发现的一种能产生保护性免疫的毒力决定因子。随着研究的不断深入,人们对LcrV的功能、在预防和治疗鼠疫中的应用有了新的认识。本文将就LcrV功能、应用方面的最新研究进展进行综述。 相似文献
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应用肽核酸探针检测鼠疫耶尔森氏菌 总被引:6,自引:0,他引:6
目的:利用特异的肽核酸(PNA)探针、链霉亲和素包被的磁珠和cy5纳米颗粒,通过荧光扫描技术,建立一种特异、快速、准确地检测鼠疫耶尔森氏菌的方法。方法:针对鼠疫耶尔森氏菌pMT1质粒上的caf1基因设计并合成一对特异PNA探针,经生物素标记后,分别与链霉亲和素包被的磁珠和cy5纳米颗粒结合;将探针与待测鼠疫耶尔森氏菌的基因组DNA杂交后,利用荧光扫描技术进行检测。探讨了多个实验因素对测定的影响,并进行了特异性和灵敏度检测。结果:建立并优化了利用PNA探针检测鼠疫耶尔森氏菌的方法,得到较好的线性关系;检测的灵敏度为0.9μg/mL(待测DNA)。结论:PNA探针与靶基因的结合不易受杂交液离子强度的影响,结合后具有较高的稳定性。本研究建立的分析方法能够灵敏、特异、稳定地对鼠疫耶尔森氏菌进行定量检测,为鼠疫的监控、诊断提供了有力手段。 相似文献
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鼠疫耶尔森氏菌LcrV基因的克隆及序列分析 总被引:1,自引:0,他引:1
为了研究鼠疫耶尔森氏菌(Y.pestis)保护性抗原V蛋白,从基因库中查得Y.pestis LcrV基因DNA序列,针对序列设计合成了一对PCR扩增引物,以本所保存的Y.pestis菌种为模板进行基因扩增,结果获得长约980bp的DNA片段。将扩增产物回收纯化,克隆至pGEM-T载体,构建重组载体pGEN-T/ypV,经过PCR,酶切鉴定,并对pGEM-T/ypV中的V基因片段进行测序,分析测序结果与己知序列相同,表明获得了LcrV基因。 相似文献
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鼠疫耶尔森氏菌质粒上重要毒力相关基因的克隆与表达 总被引:1,自引:0,他引:1
鼠疫耶尔森氏菌含有3种质粒pMT1、pPCP1和pCD1,这3种质粒编码鼠疫耶尔森氏菌的多种重要毒力因子。首先通过生物信息学技术选定了18种可能重要的毒力相关基因作为拟克隆和表达的目的基因。通过:PCR技术、TA克隆技术、双酶切技术获得目的片段。这些目的片段再分别克隆入原核表达载体pET32a中,构建了一系列重组表达质粒,其中12个重要的毒力相关基因在原核表达载体pET32a中有稳定的高效表达,表达量占细菌总蛋白的20%~40%。实验结果为进一步研究质粒编码的毒力因子的结构与功能,及其作为新型疫苗选择的可能性奠定了基础。 相似文献
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鼠疫耶尔森氏菌是烈性传染病鼠疫的病原菌,该菌在媒介(跳蚤)和宿主(哺乳动物)之间的循环过程中,基因表达适应环境谱的变化。本介绍鼠疫耶尔森氏菌适应环境信号如不同温度、离子浓度、pH等条件下的基因表达调控研究现状。 相似文献
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鼠疫耶尔森菌的全基因组序列已测定完成,在染色体上有4000多个编码序列和149个假基因,并含有大量的插入序列,3个毒性质粒上也含有诸多与致病性有关的基因,本主要就鼠疫耶尔森菌的染色体及质粒pYV/pCD1,pFra/pMT1和PST/pPCP1的基因结构,组成特征和已知的毒性基因定位等方面的研究作一综述。 相似文献
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IS1OO周围序列多态性分析技术的建立及其在鼠疫耶尔森氏菌分型中的应用 总被引:2,自引:0,他引:2
建立鼠疫耶尔森氏菌IS1000周围序列多态性(ISCP)分析技术,并探讨其在鼠疫耶尔森氏菌分型中的应用,根据鼠疫杆菌CO92株IS100的基因序列在其两端设计两条向外延伸的引物进行PCR扩增,电泳,获得的指纹图用RAPD,PHYLIP和Treeview软件分析,建立的ISCP分析技术稳定,可靠,利用该技术分析17个生态型的271株鼠疫耶尔森氏菌,扩增结果表明,指纹图有一定的差异,经RAPD,PHYLIP和Treeview分析可分为3个类型,IS100在鼠疫耶尔森氏菌染色体中虽然分布较广,但其周围序列变异较小,在遗传上较稳定,可作为鼠疫耶尔森氏菌的基因标志,研究该菌的分型与进化。 相似文献
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Rapid detection of Yersinia pestis with multiplex real-time PCR assays using fluorescent hybridisation probes 总被引:6,自引:0,他引:6
Tomaso H Reisinger EC Al Dahouk S Frangoulidis D Rakin A Landt O Neubauer H 《FEMS immunology and medical microbiology》2003,38(2):117-126
The objective of the present study was to establish a system of real-time polymerase chain reactions (PCRs) for the specific detection of Yersinia pestis using the LightCycler (LC) instrument. Twenty-five strains of Y. pestis, 94 strains of other Yersinia species and 33 clinically relevant bacteria were investigated. Assays for the 16S rRNA gene target and the plasminogen activator gene (resides on the 9.5-kb plasmid) and for the Y. pestis murine toxin gene and the fraction 1 antigen gene (both on the 100-kb plasmid) were combined for the use in two multiplex assays including an internal amplification control detecting bacteriophage lambda-DNA. Applying these multiplex assays, Y. pestis was selectively identified; other bacteria yielded no amplification products. The lower limit of detection was approximately 0.1 genome equivalent. Rat or flea DNA had no inhibitory effects on the detection of Y. pestis. The results obtained using the multiplex real-time assays showed 100% accuracy when compared with combinations of conventional PCR assays. We developed and evaluated a highly specific real-time PCR strategy for the detection of Y. pestis, obtaining results within 3 h including DNA preparation. 相似文献
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影响耶尔森氏鼠疫杆菌基因组密码子使用的因素分析 总被引:2,自引:2,他引:2
基因组密码子使用的影响因素分析有助于发现影响密码子使用的进化动力学 ,对发现和预测进化的方向和模式有重要的作用。同时 ,分析完整的基因组可以发现特定基因组中密码子的使用模式 ,从而重新设计高效的PCR引物和外源导入基因 ,促进外源基因在特定生物体中的高效率表达。导致瘟疫等外源性感染疾病的耶尔森氏鼠疫杆菌完整基因组序列已经测序公布。为了对鼠疫杆菌的同义密码子使用的进化模式有更加深入的了解 ,详细的研究分析鼠疫杆菌的基因组密码子的使用模式和影响密码子使用的因素。结果发现 ,尽管鼠疫杆菌基因组序列中“G” “C”含量相对较低 (4 7.6 4 % ) ,高水平表达基因的密码子第三位碱基使用胞嘧啶 (C)的频率比表达水平低的基因使用胞嘧啶 (C)有显著的提高 ,表达水平较低的基因在密码子的第三位碱基更趋向使用鸟嘌呤 (G)。在表达水平高低的两组基因中 ,对密码子的第三位碱基使用腺嘌呤 (A)和胸腺嘧啶 (T)总体上趋于随机使用。基因的表达水平与对应分析的第一条向量轴呈高度相关 (R =0 .6 3,P <0 .0 0 0 1)。通过分析比较表达水平高低两组基因的密码子使用模式发现 ,基因的表达水平对于密码子使用有显著的影响。GC skew分析结果显示 ,复制转录阶段的选择对密码子使用有一定的影响。在不同长度 相似文献
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S.S. Bardarov T.D. Sirakova J. Kriakov A. Karakashyan K. Markov 《FEMS microbiology letters》1990,71(3):277-279
Chromosomal DNA from reference Yersinia strains was digested individually with 9 restriction endonucleases. DNA fragments were separated and analyzed by electrophoresis through agarose gels. The clearest fragment patterns were obtained when EcoRI was employed. The Y. pestis fragment pattern obtained after the use of this enzyme showed the presence of a unique DNA fragment with molecular mass 1400 bp. This DNA fragment was cloned, purified, labeled with 32P and then used to probe EcoRI digests of all three Yersinia species. A strong hybridization signal was obtained with Y. pestis strain. No such signal was found with Y. pseudotuberculosis or Y. enterocolitica. These results indicate that the DNA fragment is species specific and could be used as a diagnostic DNA probe for Y. pestis. 相似文献
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Y. Tan M. Wu H. Liu X. Dong Z. Guo Z. Song Y. Li Y. Cui Y. Song Z. Du R. Yang 《Letters in applied microbiology》2010,50(1):104-111
Aims: Gas chromatography (GC) was utilized to investigate the cellular fatty acids (CFAs) composition of 141 Yersinia pestis isolates from different plague foci of China, and 20 Yersinia pseudotuberculosis strains as well.
Methods and Results: The whole cell fatty acid methyl esters (FAMEs) were obtained by saponification, methylation and extraction followed with analysis using a standardized Microbial Identification System (MIS). Y. pestis and Y. pseudotuberculosis strains are quite similar in major CFA profiles, which include 16:0, 17:0 cyclo, 3-OH-14:0, 16:1ω7c and 18:1ω7c, accounting for more than 80% of the total CFAs.
Conclusions: Yersinia pestis could be easily differentiated from Y. pseudotuberculosis by plotting the ratios of some CFA pairs, i.e.,14:0/18:0 vs 18:1ω7c/18:0, 3-OH-14:0/18:0 vs 18:1ω7c/18:0, 16:1ω7c/18:0 vs 18:1ω7c/18:0, 12:0/18:0 vs 18:1ω7c/18:0 and 12:0 ALDE/18:0 vs 16:1ω7c/18:0 fatty acids.
Significance and Impact of the Study: In the present study, the normalized Sherlock MIS and Sherlock standard libraries were used to analyse the fatty acid composition of different strains of Y. pestis and Y. pseudotuberculosis . Meanwhile, ratios of certain CFA components were found to serve as chemical markers for differentiating the two closely related bacteria that are difficult to be differentiated by simply comparing CFA profiles based on other researches. 相似文献
Methods and Results: The whole cell fatty acid methyl esters (FAMEs) were obtained by saponification, methylation and extraction followed with analysis using a standardized Microbial Identification System (MIS). Y. pestis and Y. pseudotuberculosis strains are quite similar in major CFA profiles, which include 16:0, 17:0 cyclo, 3-OH-14:0, 16:1ω7c and 18:1ω7c, accounting for more than 80% of the total CFAs.
Conclusions: Yersinia pestis could be easily differentiated from Y. pseudotuberculosis by plotting the ratios of some CFA pairs, i.e.,14:0/18:0 vs 18:1ω7c/18:0, 3-OH-14:0/18:0 vs 18:1ω7c/18:0, 16:1ω7c/18:0 vs 18:1ω7c/18:0, 12:0/18:0 vs 18:1ω7c/18:0 and 12:0 ALDE/18:0 vs 16:1ω7c/18:0 fatty acids.
Significance and Impact of the Study: In the present study, the normalized Sherlock MIS and Sherlock standard libraries were used to analyse the fatty acid composition of different strains of Y. pestis and Y. pseudotuberculosis . Meanwhile, ratios of certain CFA components were found to serve as chemical markers for differentiating the two closely related bacteria that are difficult to be differentiated by simply comparing CFA profiles based on other researches. 相似文献
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[目的]利用分子生物学实验研究鼠疫菌调控子OxyR对dps的转录调控机制.[方法]提取鼠疫菌野生株(WT)和oxyR突变株(ΔoxyR)的总RNA,采用引物延伸实验研究dps的转录起始位点,并根据产物的丰度判断OxyR对dps的调控关系.进一步采用实时定量RT-PCR的方法验证OxyR对dps的调控关系.PCR扩增dps的整个启动子区DNA序列,并纯化His-OxyR蛋白,通过凝胶阻滞实验(EMSA)验证OxyR对dps启动子区是否具有直接的相互作用.利用大肠杆菌OxyR识别基序,预测鼠疫菌OxyR对dps启动子区的结合位点,从而得出鼠疫菌OxyR对dps的转录调控机制.[结果]鼠疫菌dps有一个转录起始位点G(-40)(翻译起始位点为+1),其转录表达受OxyR的激活;体外实验及生物信息学预测结果表明OxyR能结合到dps启动子区-111到-78之间的碱基上.[结论]OxyR能直接结合到dps启动子区而激活其转录表达. 相似文献
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