Jung C, Claussen U, Horsthemke B, Fischer F, Herrmann R G
Botanisches Institut, Ludwig-Maximilians-Universität München, Germany.
Plant Mol Biol. 1992 Nov;20(3):503-11. doi: 10.1007/BF00040609.
We have used a standard protocol established for human chromosomes to create a chromosome-specific plasmid library from a Beta patellaris chromosome conferring nematode resistance. A monosomic addition line was chosen carrying 18 sugar-beet (Beta vulgaris L.) and one wild-beet (B. patellaris) chromosome. The wild-beet chromosome can readily be identified as a univalent during metaphase I of meiosis. Highly synchronized meiotic material was used to excise the univalents from four pollen mother cells. The chromatin was lysed in a 1 nl collection drop, the DNA purified and restricted with Rsa I, ligated into a vector containing universal sequencing primers, and amplified by the polymerase chain reaction. The amplified DNA was inserted into a standard plasmid vector and cloned. Approximately 23,000 recombinant plasmids were obtained of which 15,800 could be utilized. Their insert sizes ranged from 80 to 700 bp with an average of 130 bp. 61 clones were tested in more detail by genomic Southern hybridization with sugar-beet and wild-beet DNA. Of these 32 plasmids (52%) contained single-copy inserts, 11 (18%) were specific for wild-beet DNA indicating that the DNA cloned originates in the univalent chromosome. The application of this technique for establishing high-density RFLP maps for discrete regions of plant genomes is discussed.
我们使用了一种为人类染色体建立的标准方案,从赋予线虫抗性的扁茎甜菜染色体创建了一个染色体特异性质粒文库。选择了一个单体附加系,它携带18条甜菜(Beta vulgaris L.)染色体和1条野生甜菜(B. patellaris)染色体。在减数分裂I中期,野生甜菜染色体很容易被识别为单价染色体。使用高度同步的减数分裂材料从四个花粉母细胞中切除单价染色体。染色质在1 nl收集滴中裂解,DNA纯化并用Rsa I酶切,连接到含有通用测序引物的载体中,并通过聚合酶链反应扩增。扩增的DNA插入到标准质粒载体中并克隆。获得了大约23,000个重组质粒,其中15,800个可以使用。它们的插入片段大小在80到700 bp之间,平均为130 bp。通过与甜菜和野生甜菜DNA进行基因组Southern杂交,对61个克隆进行了更详细的测试。其中32个质粒(52%)含有单拷贝插入片段,11个(18%)对野生甜菜DNA具有特异性,表明克隆的DNA起源于单价染色体。讨论了该技术在为植物基因组离散区域建立高密度RFLP图谱中的应用。
