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首页> 外文期刊>Photosynthesis Research >Minimal Extent of Sequence Homology Required for Homologous Recombination at the psbA Locus in Chlamydomonas reinhardtii Chloroplasts using PCR-generated DNA Fragments
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Minimal Extent of Sequence Homology Required for Homologous Recombination at the psbA Locus in Chlamydomonas reinhardtii Chloroplasts using PCR-generated DNA Fragments

机译:使用PCR产生的DNA片段在莱茵衣藻叶绿体中psbA位点进行同源重组所需的最小序列同源性

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摘要

The Del1 mutant of the green alga Chlamydomonas reinhardtii with a defined deletion in the chloroplast encoded psbA gene is unable to grow photoautotrophically. We show here that this mutant can be transformed with PCR-generated psbA fragments of varying length to yield photosynthetically growing colonies. PCR fragments need not be purified but can be directly precipitated from the amplification reaction onto tungsten particles, allowing fast and efficient mutagenesis experiments. Flanking regions bordering the deletion breakpoints have been systematically shortened from both sides. The shortest fragment giving rise to significant numbers of transformants contains about 50 bp upstream and 120 bp downstream of the deletion breakpoint. This technique greatly simplifies comprehensive structure–function analyses of the D1 protein in Chlamydomonas, but could perhaps be adapted to other chloroplast genes in this or other organisms as well.
机译:绿藻衣藻衣藻的Del1突变体在叶绿体编码的psbA基因中有明确的缺失,无法自养。我们在这里显示此突变体可以用不同长度的PCR产生的psbA片段转化,以产生光合生长的菌落。 PCR片段无需纯化,但可以直接从扩增反应中沉淀到钨颗粒上,从而可以进行快速有效的诱变实验。从两侧系统地缩短了与缺失断点接壤的侧翼区域。产生大量转化体的最短片段在缺失断点上游约50 bp,下游约120 bp。这项技术极大地简化了衣藻D1蛋白的综合结构-功能分析,但也许可以适应该生物体或其他生物体中的其他叶绿体基因。

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