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It is concordant with routine PCR method. 并与常规PCR法具有很好的一致性。
The ISOObp promoter of PNZIP gene was cloned by adaptor PCR method. 因此，我们利用接头PCR技术克隆了PNZIP基因的启动子。
The applications of Mullis' PCR method are already many. 原理简介：PCR技术的基本原理是DNA的半保留复制。
Single cell 5-plex nest PCR for exons 17,19,44,45 and 48 of DMD gene was established. 获取正常男性单个淋巴细胞和无DMD家族史的单个胚胎细胞,行DMD基因外显子17、19、44、45、48的五重巢式PCR,分析扩增成功率、假阳性率和假阴性率。
A multiplex- PCR method for detection bovine materials in foodstuffs. 动物饲料中牛成分的复合PCR检测方法。
The expression of cyclin D1 and CDK4 were detected by RT PCR method. RT PCR检测细胞周期素D1(cyclinD1)、细胞周期蛋白依赖激酶 4 (CDK4 )mR NA的表达。
Methods The mRNA from normal lungs was used as template. By using the techniques of RT PCR, nest PCR and cloning, the pUC 19/SP A 6 A clone was established and sequenced. 方法以正常人肺组织mRNA为模板 ,采用逆转录反应 (RT) PCR、巢式 PCR及基因克隆技术 ,获得pUC19/SP A 6A克隆 ,并测序证实。
Meanwhile, the PCR method is superior to immunohistochemistry in detecting HPV. 在检测上，PCR方法优于免疫组织化学染色，值得提倡和推广。
Methods The ORF2 gene of TTV was amplified from the serum of a blood donor in Lanzhou region by nest PCR and inserted into vector pGEM-T then,after identification by DNA sequencing,subcloned to expression vector pET22b(+). 方法通过巢式PCR,从一份兰州地区无偿献血员血清中扩增TTV病毒的ORF2基因,并克隆到pGEM-T载体中,进行核苷酸序列分析。
X gene (HBx), enhancer II (Enh2) and basic core promoter (Bcp) of HBV in sera from HCC patients were amplified by nest PCR , and sequenced and then compared with the sequences in Genbank. 对HCC患者血清的HBV的HBx、Enh2与Bcp基因的巢式PCR产物直接测序，与Genbank中已发表序列进行对比分析。
Detection of Fetal SRY Gene from Maternal Blood by a Nested PCR. 利用套式PCR技术检测母血中胎儿SRY基因的研究
Using PCR method, BBTV or CMV can be detected from the banana leaf tissue equivalent to 100 ng. 用PCR方法可从相当于100ng的叶片组织中检测到BBTV和CMV。
Objective To establish a technique of single cell 5-plex nest PCR for Ducheme muscular dystrophy(DMD) detection and evaluate the possibility of using for preimplantation genetic diagnosis (PGD). 摘要目的：探索建立单细胞多重巢式PCR检测杜氏肌营养不良症(DMD)基因外显子17、19、44、45、48的技术，及应用于植入前遗传学诊断(PGD)的前景。
Objective To develop a PCR method for the determination of porcine parvovirus(PPV). 目的建立猪细小病毒(PPV)PCR检测方法。
Objective: To establish a technique of single cell 5-plex nest PCR for Ducheme muscular dystrophy (DMD) detection and evaluate the possibility of using for preimplantation genetic diagnosis (PGD). 目的:探索建立单细胞多重巢式PCR检测杜氏肌营养不良症(DMD)基因外显子17、19、44、45、48的技术,及应用于植入前遗传学诊断(PGD)的前景。
The results prove that adapter ligation PCR method is workable to clone carnation CHS promoter. 然后利用衔接头PCR的方法进行了香石竹CHS启动子克隆的初步研究，得到了约500bp和800bp的PCR产物，目前克隆测序工作正在进行。
This is to develop a rapid,sensitive and specific fluorescence PCR method detecting listeria monocytogenes in food. 发展一种快速、敏感、特异的荧光PCR方法检测食品中单核细胞增生李斯特氏菌。
In order to improve diagmostic procedure of E. suis, the PCR method was established. 鉴于上述原因,为了建立特异准确的诊断方法,本研究开展了附红细胞体病的聚合酶链式反应(PCR)诊断方法的研究。
The sensitive and specific PCR method for detection E. granulosus from dog faeces was preliminarily developed. 初步建立了灵敏、特异的检测家犬粪便中细粒棘球绦虫的PCR方法。
PCR method was considered as the gold standard, which showed the highest specificity (100%) and sensitivity (100%). PCR法是检测MRSA的金标准,特异性和灵敏度均为100%25。