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Construction of Tandem Repeats of DNA Fragments by a Polymerase Chain Reaction-Based Method

机译:基于聚合酶链反应的DNA片段串联重复序列的构建

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We describe a new application of megaprimer polymerase chain reaction (PCR) for constructing a tandemly repeated DNA sequence using the drought responsive element (DRE) from Arabidopsis thaliana as an example. The key feature in the procedure was PCR primers with partial complementarity but differing melting temperatures (T-m). The reverse primer had a higher T-m, a 3' end complementary to the DRE sequence and a 5' region complementary to the forward primer. The initial cycles of the PCR were conducted at a lower primer annealing temperature to generate products that served as megaprimers in the later cycles conducted at a higher temperature to prevent annealing of the forward primer. The region of overlap between the megaprimers was extended for generating products with a variable copy number (one to four copies) of tandem DRE sequence repeats (71 bp). The PCR product with four tandem repeats (4 x DRE) was used as a template to generate tandem repeats with higher copies (copy number large than four) or demonstrated to bind DRE-binding protein in an yeast one-hybrid assay using promotorless reporter genes (HIS and lacZ). This PCR protocol has numerous applications for generating DNA fragments of repeated sequences.
机译:我们描述了使用来自拟南芥的干旱反应元件(DRE)来构建串联重复的DNA序列的大型引物聚合酶链反应(PCR)的新应用。该程序的关键特征是具有部分互补性但熔解温度(T-m)不同的PCR引物。反向引物具有更高的T-m,与DRE序列互补的3'末端和与正向引物互补的5'区域。 PCR的初始循环在较低的引物退火温度下进行,以生成充当大引物的产物,在较高的温度下进行的后续循环中,以防止正向引物退火。 megaprimers之间的重叠区域被扩展以生成具有可变拷贝数(一到四个拷贝)的串联DRE序列重复序列(71 bp)的产物。具有四个串联重复序列(4 x DRE)的PCR产物用作模板,以产生具有更高拷贝数(拷贝数大于4)的串联重复序列,或在使用无启动子报告基因的酵母单杂交实验中证明与DRE结合蛋白结合。 (HIS和lacZ)。该PCR方案在产生重复序列的DNA片段方面有许多应用。

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