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Transformation of lacZ using different promoters in the commercially important red alga, Gracilaria gracilis

机译:LacZ在商业上重要的红藻中使用不同启动子的转化,Gracilaria Gracilis

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This paper reports the first successful transformation of?Gracilaria gracilis(Stackhouse) M. Steentoft, L.M. Irvine and W.F. Farnham with?lacZ-containing plasmids by microparticle bombardment. Transient expression of the?lacZ reporter gene was compared under the control of three different viral promoters including the Simian virus 40 (SV40) promoter, the Cytomegalovirus (CMV) promoter and the Cauliflower mosaic virus 35S (CaMV 35S) promoter. In thalli transformed with vectors containing either the SV40 or CMV promoter,?lacZ presence?was confirmed by histological staining 2 and 3 days post-bombardment. In thalli transformed with the vector containing the CaMV 35S promoter,?lacZ presence was confirmed by histological staining 1, 2, 3 and 5 days post-bombardment. Sectioning and histological staining of bombarded thalli showed that recombinant bombarded DNA penetrated cells to below the epidermal layer of the thallus. PCR analysis verified the presence of the?lacZ gene in plasmid-bombarded thalli from the first day post-bombardment onwards. β-Galactosidase activity varied depending on the type of promoter used. These results form an important foundation for the development of a successful transformation protocol for?G. gracilis.
机译:本文报告了第一次成功转型?Gracilaria Gracilis(Stackhouse)M. Steentoft,L.M. Irvine和W.f. Farnham与含有含Lacz的质粒通过微粒轰击。在包括Simian病毒40(SV40)启动子的三种不同病毒启动子,巨细胞病毒(CMV)启动子和花椰菜马赛克病毒35s(CAMV 35S)启动子的控制下进行了瞬态表达。在Thalli用含有Sv40或CMV启动子的载体转化,αSacZ存在?通过后轰击后2和3天通过组织学染色确认。在Thalli用含有Camv 35s启动子的载体转化,通过轰击后1,2,3和5天通过组织学染色来确认LacZ存在。轰击的Thalli的切片和组织学染色显示重组轰击DNA渗透细胞以低于晶粒层的表皮层。 PCR分析验证了在轰击后的第一天从轰击后的质粒轰击的质粒轰击的存在的存在。 β-半乳糖苷酶活性取决于所用启动子的类型。这些结果形成了一个成功转型议定书的重要基础。 Gracilis。

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