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It is concordant with routine PCR method. 并與常規PCR法具有很好的一致性。
The ISOObp promoter of PNZIP gene was cloned by adaptor PCR method. 因此，我們利用接頭PCR技術(shù)克隆了PNZIP基因的啟動(dòng)子。
The applications of Mullis' PCR method are already many. 原理簡(jiǎn)介：PCR技術(shù)的基本原理是DNA的半保留復制。
A multiplex- PCR method for detection bovine materials in foodstuffs. 動(dòng)物飼料中牛成分的復合PCR檢測方法。
The expression of cyclin D1 and CDK4 were detected by RT PCR method. RT PCR檢測細胞周期素D1(cyclinD1)、細胞周期蛋白依賴(lài)激酶 4 (CDK4 )mR NA的表達。
Meanwhile, the PCR method is superior to immunohistochemistry in detecting HPV. 在檢測上，PCR方法優(yōu)于免疫組織化學(xué)染色，值得提倡和推廣。
Using PCR method, BBTV or CMV can be detected from the banana leaf tissue equivalent to 100 ng. 用PCR方法可從相當于100ng的葉片組織中檢測到BBTV和CMV。
Objective To develop a PCR method for the determination of porcine parvovirus(PPV). 目的建立豬細小病毒(PPV)PCR檢測方法。
The results prove that adapter ligation PCR method is workable to clone carnation CHS promoter. 然后利用銜接頭PCR的方法進(jìn)行了香石竹CHS啟動(dòng)子克隆的初步研究，得到了約500bp和800bp的PCR產(chǎn)物，目前克隆測序工作正在進(jìn)行。
This is to develop a rapid,sensitive and specific fluorescence PCR method detecting listeria monocytogenes in food. 發(fā)展一種快速、敏感、特異的熒光PCR方法檢測食品中單核細胞增生李斯特氏菌。
In order to improve diagmostic procedure of E. suis, the PCR method was established. 鑒于上述原因,為了建立特異準確的診斷方法,本研究開(kāi)展了附紅細胞體病的聚合酶鏈式反應(PCR)診斷方法的研究。
The sensitive and specific PCR method for detection E. granulosus from dog faeces was preliminarily developed. 初步建立了靈敏、特異的檢測家犬糞便中細粒棘球絳蟲(chóng)的PCR方法。
PCR method was considered as the gold standard, which showed the highest specificity (100%) and sensitivity (100%). PCR法是檢測MRSA的金標準,特異性和靈敏度均為100%25。
The NDI gene in mtDNA was amplified with regular PCR method, and the PCR product was sequenced after purified. 用PCR擴增人線(xiàn)粒體NDI基因片段，PCR產(chǎn)物經(jīng)純化后測序和核苷酸同源性分析。
Conclusions PCR method in which 139-141 as primer is suitable for rapid detection of Salmonella. 結論在沙門(mén)菌的快速檢測中,宜采用以139-141為引物的PCR檢測法。
Objective:This study was to establish a immuno in situ PCR method for the diagnosis of HCMV active infection. 目的:建立用于診斷HCMV活動(dòng)性感染的原位免疫PCR方法。
Conclusion The fluorogenic Quantitative PCR method for the detection of Plasmodium falciparum is simple and accurate. 結論建立了檢測惡性瘧原蟲(chóng)的熒光定量PCR方法，較常規PCR技術(shù)更為簡(jiǎn)便、快速、準確，有很好的應用前景和研究?jì)r(jià)值。
According to the sequence of GAPDH gene available in GenBank,a SYBR Green I dye based on real-time PCR method is developed. 根據GenBank中鴨GAPDH基因的序列設計引物;建立了基于SYBR Green I染料技術(shù)的real-time PCR方法.
All of the 51 Bt were analyzed by the PCR method with general primers of cry1, cry2, cry3, cry4, cry-n, cry7, cry8, cry11, cry13 and cyt genes. 對51 株Bt 分離菌株的cry 基因進(jìn)行了PCR 鑒定。
Six truncated Cryllel proteins were induced in Ecoli BL21(DE3) containing six deleted fragments from cryllel gene by PCR method. 本研究通過(guò)PCR擴增的方法，以cry1Ie1全長(cháng)基因為模板，分別得到不同末端缺失的基因片段，轉化大腸桿菌BL21(DE3)中，誘導表達，得到6種末端缺失的蛋白。

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