• Conclusion: The MAGE-3 fragment can be used in eukaryotic and prokaryotic gene expression.

    结论该片用于真核表达

    youdao

  • We isolated and purified EBP effectively, and obtained EBP with biological activity for the first time with gene cloning method and prokaryotic expression system.

    通过基因克隆等方法,选择表达系统对目的蛋白进行分离纯化,初步获得活性人内毒素结合肽ebp

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  • To clone gene of the TRAIL and construct its prokaryotic expression vector.

    目的克隆人TRAIL基因构建原核表达载体。

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  • Methods: PCR, gene cloning and successive sub cloning, DNA sequencing, prokaryotic temperature induction, etc. were used.

    方法采用PCR克隆连续克隆,序列分析原核温度诱导表达方法。

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  • The function of gene has been identified using Prokaryotic expression system and Arabidopsis thaliana (A. thaliana) transformation systems. The study has got following results:1.

    利用序列分析技术克隆抗逆相关基因,并通过原核表达体系转基因技术进行功能验证。

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  • Objective To modify the HA1 gene of high pathogenic avian influenza virus (HPAIV) and to build an efficient prokaryotic expression system of it.

    目的高致病性禽流感病毒血凝素基因建立有效原核表达体系

    youdao

  • Horizontal gene transfer is an important evolutionary mechanism in prokaryotic genome evolution and has been widely studied.

    核生物的进化过程中,基因横向转移一个重要进化机制

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  • AIM To clone human heat shock protein 72 (HSP72) gene, do prokaryotic expression and purify HSP72 protein for further study.

    目的克隆人休克蛋白72 (HSP72)基因,原表达纯化蛋白产物,以探讨其生物学功能。

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  • Objective To construct the clone vector of S gene in occult hepatitis B virus infection. To analyse its mutations and to construct its prokaryotic expression vector.

    目的构建克隆载体分析隐匿性乙型肝炎病毒S基因突变情况,构建原核融合蛋白表达载体。

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  • Objective to clone human heat shock protein 70 (HSP70) gene for the construction of a prokaryotic expression vector.

    目的克隆人休克蛋白70 (HSP70)基因构建其原核高效表达载体

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  • Objective To isolate human arresten gene with Chinese origin for efficient prokaryotic expression.

    目的克隆中国人阻滞原基因高效表达。

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  • ConclusionThe augementer of liver regeneration gene was cloned from the liver tissue of 2 week old SD rat and the protein encoded by the gene was expressed in the prokaryotic cells.

    结论2周龄大鼠组织成功克隆再生增强因子基因获得了核细胞高效表达

    youdao

  • AIM: to clone human MAGE 3 gene, to induce its prokaryotic expression and to purify the protein.

    目的克隆人MAGE3基因并进行原表达分离纯化

    youdao

  • Objective To construct the prokaryotic expression vector of the sporozoite surface antigen gene of Eimeria tenella GZ strain and expression in Escherichia coli.

    目的构建柔嫩艾美耳球虫子孢子表面抗原表达载体,并且大肠杆菌中表达。

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  • AIM: to clone rat neurotrophin-4 (NT-4) total gene and construct expression plasmid for prokaryotic cells.

    目的克隆大鼠神经营养因子4全长基因构建真核细胞表达质粒

    youdao

  • Objective: to construct a prokaryotic expression vector containing esophageal cancer related gene 2 ECRG2 and observe its expression in Escherichia coli e.

    目的构建食管癌相关基因2ECRG2原核表达质粒,大肠杆菌e

    youdao

  • Objective to construct the prokaryotic expression vector of human neuronal pentraxin 2 (NPTX2) gene, induce the expression of the recombinant fusion protein in e.

    目的在大肠埃希菌中表达神经元正五聚蛋白2 (NPTX2),并重组蛋白进行纯化、鉴定。

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  • In this study, the Aer toxin gene was cloned and expressed in prokaryotic system and the antigenicity of its recombinant protein was analyzed.

    该领域国外研究热点水气单胞菌毒素基因组结构、相关毒力因子基因克隆序列比较以及毒素蛋白表达和致病机理等方面。

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  • We use gene recombination technology to build the prokaryotic MGC5306 expression system, and we have successfully expressed MGC5306 (98-204aa).

    我们利用基因重组技术构建MGC5306的原表达体系成功表达了MGC5306 (98- 204aa)。

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  • To construct the recombinant prokaryotic expression vector containing the ESAT-6 gene of Mycobacterium Boris, purification, expression the fusion protein identified.

    构建牛结核分枝杆菌esat - 6基因表达载体,诱导表达、纯化并初步鉴定蛋白

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  • To construct the recombinant prokaryotic expression vector containing the ESAT-6 gene of Mycobacterium Boris, purification, expression the fusion protein identified.

    构建牛结核分枝杆菌esat - 6基因表达载体,诱导表达、纯化并初步鉴定蛋白

    youdao

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