• Viral detection by reverse transcription polymerase chain reaction (RT-PCR) assay, and.

    采用逆转录聚合酶链式反应(RT - PCR)检测病毒

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  • Various reverse transcriptasepolymerase chain reaction (RTPCR) methods are available but are of variable sensitivity.

    有各种逆转录酶聚合酶链反应(扩增核糖核酸基因组RTPCR)检测试验方法灵敏度各相同

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  • RTPCR products from clinical samples may also be used for genotyping of the virus, allowing comparisons with virus samples from various geographical sources.

    临床样品RT-PCP制品用于病毒基因分型,与采不同区域病毒取样做出比较

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  • Quantitative RT-PCR results indicated representation of OsBTB gene expression was corresponding with the selected resistant and pathogenesis-related genes.

    定量PCR结果表明基因表达模式选取的抗性及抗性相关基因表达模式一致。

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  • The result indicated that fluorogenetic quantitation RT-PCR may be used as a good reference in detection of H5N1 TIV.

    说明荧光定量RT-PCR方法可以对临床上H5N1源流感病毒检测提供参考

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  • These RT-PCR products were sequence verified.

    这些RT - PCR扩增产物序列验证

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  • Myrosinase activity was detected in all the tested organs except for pulp, which is consistent with the result of RT-PCR.

    活性测定表明,除了果肉其它器官有芥子酶活性,RT-PCR结果一致的。

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  • Methods RNA from human peripheral blood mononuclear cells were extracted and target genes were amplified by RT-PCR.

    方法提取外周血单个细胞RNA,反转录聚合酶链反应(RT-PCR扩增目的基因

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  • Methods MDR1 gene expression in case of 30 leukemia and 8 healthy persons' peripheral blood have been detested by fluorescence-quantitative reverse transcription-polymerase chain reaction (RT-PCR).

    方法应用荧光定量逆转录-多聚酶链反应(RT -PCR)检测了30急性白血病患者8正常人外周血MDR1基因表达

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  • One step nested reverse transcriptase-polymerase chain reaction (RT-PCR) was used.

    使用一步逆转录聚合酶链扩增法(RT - PCR)。

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  • Methods HGV RNA in plasma of 84 IVDUs was detected by reverse transcription polymerase chain reaction (RT PCR).

    方法采用逆转录聚合酶链反应(RT - PCR)检测84例静脉毒瘾者血浆标本。

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  • The intracellular pattern recognition receptor NOD1 is detected in human lung epithelial cells by RT-PCR.

    并用RT-PCR的方法检测上皮细胞模式识别受体NOD1的表达。

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  • Methods: the blood samples were collected from HFRS patients between 2000 ~ 2001, and the m segment genome of hantavirus was amplified by RT-PCR.

    方法采集2000 ~ 2001年肾综合征出血热(HFRS)患者血液标本,通过逆转录聚合酶链反应(RT - PCR)扩增坦病毒M片断基因

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  • ConclusionDue to specificity on enterovirus, the RT PCR method has some value in the diagnosis of enterovirus infections.

    结论RT - PCR方法具有肠道病毒特异性肠道病毒感染诊断有一定应用价值

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  • The results of semi-quantitative RT-PCR experiments supported the reliability of our microarray analysis.

    半定量反转录-聚合酶链反应验证了芯片分析结果可靠性

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  • Results: the linear amplification range of PCR and the best cycle number and template of RT-PCR were obtained.

    结果获取了PCR线性扩增范围,确定RT - P CR最佳循环次数模板量。

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  • Objective to evaluate the clinicopathologic significance of the detection of peritoneal micrometastases in gastric cancer by reverse transcriptase-polymerase chain reaction (RT-PCR).

    目的评估逆转录聚合酶链式反应(RT PCR)方法检测胃癌腹腔微转移临床病理意义

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  • The results of RT-PCR analysis for 7 differently expressed genes were coincident with those of microarray assay.

    PCR技术对其中7个基因表达差异验证结果基因芯片结果一致

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  • Mutation analysis was detected by direct sequencing RT-PCR products.

    直接测序法检测RT PCR产物基因变异

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  • Analysis of RT-PCR and sequencing indicated that the ncRNA gene had two different transcripts through alternatively splicing pattern.

    PCR测序结果分析,发现这个非编码RNA基因通过选择性剪接产生两种不同转录产物。

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  • Methods 40 patients with lung cancer were studied to detect TTF-1 gene by using reverse transcription-polymerase chain reaction assay (RT-PCR).

    方法采用逆转录—聚合酶链反应(RT - PCR)方法检测40患者的肺癌组织ttf - 1基因的表达。

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  • Methods Total RNAs of tumor tissues were extracted and were detected by RT-PCR.

    方法提取肿瘤组织rna反转录聚合酶链式反应(RT - pcr)法进行检测。

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  • The level of promiscuous gene expression was detected by RT-PCR.

    利用RT - PCR方法检测小鼠胸腺异位基因表达水平

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  • The level of promiscuous gene expression was detected by RT-PCR.

    利用RT - PCR方法检测小鼠胸腺异位基因表达水平

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