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A simple improved-throughput xylem protoplast system for studying wood formation

机译:用于研究木材形成的简单的提高通量的木质部原生质体系统

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Isolated protoplasts serve as a transient expression system that is highly representative of stable transgenics in terms of transcriptome responses. They can also be used as a cellular system to study gene transactivation and nucleocytoplasmic protein trafficking. They are particularly useful for systems studies in which stable transgenics and mutants are unavailable. We present a protocol for the isolation and transfection of protoplasts from wood-forming tissue, the stem-differentiating xylem (SDX), in the model woody plant Populus trichocarpa. The method involves tissue preparation, digestion of SDX cell walls, protoplast isolation and DNA transfection. Our approach is markedly faster and provides better yields than previous protocols; small (milligrams)- to large (20 g)-scale SDX preparations can be achieved in ~60 s, with isolation of protoplasts and their subsequent transfection taking ~50 min. Up to ten different samples can be processed simultaneously in this time scale. Our protocol gives a high yield (~2.5 × 10~7 protoplasts per g of SDX) of protoplasts sharing 96% transcriptome identity with intact SDX.
机译:分离的原生质体充当瞬时表达系统,就转录组反应而言,该系统高度代表稳定的转基因。它们还可以用作细胞系统来研究基因反式激活和核质蛋白运输。它们对于无法获得稳定的转基因和突变体的系统研究特别有用。我们提出了从模型木本植物毛果杨(Populus trichocarpa)的木材形成组织,茎分化木质部(SDX)中分离和转染原生质体的协议。该方法涉及组织制备,SDX细胞壁消化,原生质体分离和DNA转染。与以前的协议相比,我们的方法明显更快,并且提供了更高的收益。大约60 s即可完成小(毫克)至大(20 g)规模的SDX制备,分离原生质体并随后转染约50分钟。在此时间范围内,最多可以同时处理十个不同的样本。我们的方案可提供高产(每g SDX约2.5×10〜7个原生质体)原生质体,与完整SDX共享96%的转录组同一性。

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