插入载体
- insertion vector;insertional vector
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结果:PCR及序列分析显示融合基因插入载体正确;
Results : The gene insertion was proved correct using PCR and DNA sequencing .
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抗体基因插入载体的频率,高比例的丢失意味着筛选的低效率;
The frequency of gene fusing , high deletion of antibody gene meaning low efficiency ;
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方法设计特异引物,用RT-PCR方法从乳腺癌组织扩增获得目的片段,利用T/A克隆将PCR产物插入pMD-18T载体;
Methods The interested segment was obtained by reverse transcription PCR with the designed specific primers , and inserted into pMD-18T vector by T / A match .
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将其插入表达载体pET-32a,获得了重组表达载体pET-32a-CD4。
Then the segment was inserted into vector pET-32a and reconstructed the recombinant vector , named pET-32a-CD4 .
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双酶切及测序结果表明:目标基因已成功插入表达载体pET-32a(+)。
Restriction endonuclease digestion analysis and sequencing data revealed that the target gene has been successfully inserted the expression vector pET-32 a ( + ) .
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利用PCR技术从猪伪狂犬病毒基因组中克隆gE抗原表位基因,并将其插入到载体pET-22b(+)中,构建成原核表达质粒pET-22b(+)-gE,使其在E。
By PCR , a gE antigen epitope gene was obtained from the genome of swine pseudorabies virus . We inserted the gene into an expression vector to yield the recombinant plasmid pET-22b ( + ) - gE .
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方法:用DNA重组技术构建EGF基因并插入表达载体pQE-40,与载体上的6×His标签融合,获得的表达质粒pQE-EGF转化E。
Methods : An artificial egf gene was constructed with recombinant DNA technology and inserted into pQE-40 to get a expression plasmid pQE-EGF , in which egf was fused with 6 × His tag . Plasmid pQE-EGF was transformed into E.
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方法用PCR的方法由含survivin基因的真核表达载体扩增所需目的片段,然后将该片段插入逆转录病毒载体pMIG。
Methods Survivin fragments were amplified from eukaryotic expression vectors by PCR , then cloned into pMIG retroviral vectors .
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以往技术的局限是对BAC的修饰需要多步的克隆把目的序列插入到穿梭载体上。
One of the original limits of BAC modification technique required multiple cloning steps to target foreign sequences into the shuttle vector .
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插入PGEMT载体,转化至大肠杆菌;
TR cDNA was inserted into pGEM-T vector , and then be transformed into Escherichia coli .
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结果1.经琼脂糖凝胶电泳鉴定证实Gax基因成功插入到目的载体上,获得重组腺病毒。
The Gax gene was successful connection with the adenovirus vectors , which was examined by the agarose gel electrophoresis . 2 .
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将CP基因插入原核表达载体pBAD/HisC中,转化E。
The CP gene was inserted into pBAD / His C vector and expressed in E.
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结果酶切鉴定证实人IκBα基因cDNA已插入原核表达载体pET32a(+)。
Results Endonucleases digestion confirmed that I κ B α gene cDNA has been inserted into the prokaryotic expression vector pET-32a ( + ) .
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用PCR法扩增了牛疱疹病毒Ⅰ型BarthaNu/67株gB基因,将其插入原核表达载体pBAD/TOPO中构建重组质粒pBAD-gB。
The gB gene fragment of bovine herpesvirus-1 Bartha Nu / 67 strain was amplified by PCR and inserted into prokaryotic expressing vector pBAD / TOPO .
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目的克隆编码mdr1基因的启动子并插入荧光素酶报告基因载体。
Objective To clone the promoter of multi-drug resistance 1 gene and insert it into a luciferase reporter gene vector .
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将目的基因片段插入原核表达载体pET-15b来构建表达质粒pET-15b/RgpAcd。
The correctly fragment was linked with and cloned into a prokaryotic expression vector pET-15b .
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用RT-PCR的方法钓取端粒酶RNA基因的cDNA,并将其反向插入到逆转录病毒载体pLNCX上,构建hTR基因的反义表达质粒。
The cDNA of hTR ( human telomerase RNA ) gene was cloned by the means of RT-PCR and inserted into the reverse transcription virus vector ( PLNCX ) to construct the antisense expression plasmid of hTR gene .
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从银屑病皮损表皮中提取总RNA,反转录成cDNA,常规方法将目的基因插入原核表达载体pGEX-4T-1和真核表达载体pCR3.1,表达和纯化相应蛋白和表位肽段。
Total RNA was isolated from epidermis of psoriasis patients and mRNA was reversely transcribed into cDNA . The epitope genes were inserted into prokaryote ( pGEX-4T-1 ) and eukaryote expression vector ( pCR3.1 ) .
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将其全基因序列分三段先后插入到PUC19/18质粒载体中。
The gene sequences divided into three successively inserted into a plasmid vector , PUC19 / 18 .
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病毒和多种聚合物材料曾被用作将治疗性基因插入患病细胞的载体。
Viruses and various polymer materials have been used in efforts to insert therapeutic genes into diseased cells .
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结果重组质粒通过双酶切产生了0.78kb目的插入片段及4.68kb载体片段;
Results The recombinant plasmid cut by incision enzyme EcoR I and Kpn I overnight generated a 0.78 kb fragment and a 4.68 kb fragment in 1 % agarose gel electrophoretogram .