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小麦(Triticum aestivum L.)原生质体电穿孔转化。

Transformation of wheat (Triticum aestivum L.) through electroporation of protoplasts.

机构信息

Department of Biochemistry, The University of Queensland, 4072, Brisbane, Australia.

出版信息

Plant Cell Rep. 1994 Dec;14(2-3):192-6. doi: 10.1007/BF00233789.

Abstract

Protoplasts isolated from embryogenic suspension cultures of wheat (Triticum aestivum cv. Hartog) were electroporated in the presence of plasmid pEmuGN and/or pEmuPAT, which contained the reporter gene gus and selectable marker gene bar, respectively. Under optimised electroporation conditions, up to 0.9% of viable protoplasts displayed gus activity two days after electroporation. To select for phosphinothricin (PPT) resistant colonies, electroporated protoplasts were incubated for six weeks in a medium containing 10 μg/ml PPT. The cells surviving the selection were maintained as individual colonies on solid medium or as suspension cultures. More than 60% of these colonies exhibited tolerance to 40 μg/ml PPT when tested 10 months after initial selection. To date, 57 green plants have been regenerated from these colonies and 24 have been transferred to soil. Southern blot analyses of colonies and plants, using the bar gene sequence as the probe, confirmed transformation of the cells. Positive PAT assays of both regenerated colonies and plants indicated the presence of the bar gene product. These results provide a basis for the establishment of routine procedures for transformation of wheat by direct gene transfer into protoplasts.

摘要

原生质体从小麦(Triticum aestivum cv. Hartog)胚性悬浮培养物中分离出来,在质粒 pEmuGN 和/或 pEmuPAT 的存在下进行电穿孔,这两个质粒分别含有报告基因 gus 和选择标记基因 bar。在优化的电穿孔条件下,在电穿孔后两天,多达 0.9%的活原生质体显示出 gus 活性。为了选择草丁膦(PPT)抗性菌落,电穿孔的原生质体在含有 10 μg/ml PPT 的培养基中培养六周。在选择后 10 个月,存活下来的细胞在固体培养基或悬浮培养物中作为单个菌落维持。这些菌落中有超过 60%的对 40 μg/ml PPT 具有耐受性。迄今为止,已经从这些菌落中再生了 57 株绿色植物,其中 24 株已移栽到土壤中。用 bar 基因序列作为探针的菌落和植物的 Southern blot 分析证实了细胞的转化。再生菌落和植物的阳性 PAT 分析表明存在 bar 基因产物。这些结果为通过直接基因转移到原生质体中建立小麦常规转化程序提供了依据。

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