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recombinant retrovirus expression vector 衣殼蛋白基因
Recombinant retroviral expression vector 重組逆轉錄病毒載體
Construction and identification of recombinase Cre expressing retrovirus expression vector 重組酶Cre的逆轉錄病毒載體的構建及鑒定
Construction of human antisense BMP-2 retrovirus expression vectors and its biological effects on human osteosarcoma cells 反義人骨形態(tài)發(fā)生蛋白2基因逆轉錄病毒表達載體的構建及其對骨肉瘤細胞生物學(xué)行為的影響
Construction for retroviral expression vector of high expression and easy isolation of human hBD2 人hBD2高表達易分離逆轉錄表達載體構建
The gene segments mentioned above were cloned into the multiple cloning sites of retrovirus vector pLXSN to construct an attenuated superantigen expression vector pLXSN SEA (D227A) linker CD80tm modulated by cis acting element of AFP gene. 將上述片斷插入逆轉錄病毒載體 pLXSN的多克隆位點(diǎn) ,構建AFP基因順式作用元件調控的肝癌特異性減毒超抗原表達載體 (pLXSNSEA(D2 2 7A) linker CD80tm)。
Fig.1.Construction of the shuttle expression vector pRL_hEGF. 標題：圖1.;穿梭表達載體pRL_hEGF的構建。
Construction of Retroviral Expressing Vector N2A/hGM-CSF and its Preliminary Expression in COS-7 Cell 逆轉錄病毒表達載體N2A/hGM－CSF的構建及其在COS－7細胞的初步表達
The pPIC9K/Ang-1 yeast expression vector was constructed successfully. 成功構建pPIC9K/Ang-1畢氏酵母表達載體。
Aim To construct a CHO cell expression vector carrying coamplification gene. 目的構建攜帶共擴增基因的CHO細胞表達載體。
And then the CED-9 gene was inserted into plant expression vector pBI121 under the control of CaMV 35S promoter. 在此基礎上再構建重組表達載體pBI-ced9，將CED-9基因置于CaMV35S啟動(dòng)子控制之下。
The baculovirus expression vector pAC-HBs-Fc for complete IgG antibody against HBsAg was successfully constructed. 已成功構建表達載體pAC-HBs-Fc,為表達抗人HBsAg的IgG全抗體奠定了基礎。
The cDNA was subcloned into prokaryotic expression vector pET3d and overexpressed in E. coli BL21(DE3). 將該cDNA插入原核表達載體pET3d并在大腸桿菌BL21(DE3)中過(guò)量表達。
Objective To construct the antisense expression vector of human Na + H + exchanger 1 (NHE 1). 目的構建人Na+ H+ 交換蛋白 1(Na+ H+ exchanger 1,NHE 1)基因反義真核表達載體。
Cloning of recombinant human BMP2 gene in eukaryotic expression vector provide basis for BMP2's expression. 克隆獲得人骨形成蛋白 2基因 ,并得到此基因的真核表達載體 ,為人骨形成蛋白 2的表達打下了基礎。
Objective:To construct expression vector of human ID4 gene promoter on the basis of bioinformatics analysis. 目的:基于生物信息學(xué)分析構建人ID4基因啟動(dòng)子表達載體,以其作為研究ID4基因啟動(dòng)子表達調控分析的工作基礎。
The recombinant constitutive expression vector pGAP9K-gat was constructed by inserting the aim gene into pGAP9K. PCR拼接獲得250bp的目的基因序列,將目的基因克隆于pGAP9K,獲得組成型表達載體pGAP9K-gat。
The competent Agrobacterium tumefacien was transformed by rice expression vector p13W4-CTB and pCWUN respectively. 水稻表達載體P13w4一cTB和pcWIJN分別轉化感受態(tài)根瘤土壤桿菌，經(jīng)過(guò)PcR篩選和酶切鑒定，獲得根瘤土壤桿菌轉化子。
For mass production of hEGF, Bombyx mori baculovirus expression vector system was adopted in this experiment. 為了高效表達人表皮生長(cháng)因子，我們采用了家蠶桿狀病毒表達系統(Bombyx mori baculovirus expression vector system, BMBEVS)。
The BADH and CMO ORF were obtained and the plant expression vector pCU1303-BADH, pCU1303-CMO were constructed. 設計帶特定酶切位點(diǎn)的特異引物,分別克隆了麥冬BADH和CMO的編碼區片段,構建了植物表達載體pCU1303-BADH和pCU1303-CMO。

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