Use of most molecular marker systems depends on the polymerase chain reaction (PCR), which is an important technique for amplifying specific DNA sequences.
大多数分子标记体系的利用都取决于聚合酶链反应(PCR),这是一项扩增特定DNA序列的重要技术。
The results of PCR molecular detection, marker genes and foreign target-gene with insect-resistance were quite regular.
PCR分子检测与转化的标记基因和外源目的基因抗性三者极有规律性。
The genomic DNA PCR indicated that the genetic homogeneity between NIL-PL01 and NIL-APL01 reached 98.6%, which were being used in screening the molecular marker linked to apetalous trait.
利用随机引物对基因组DNA扩增结果表明,NIL -PL0 1和NIL -APL0 1之间多态性差异较小,遗传同质性达98.6 % ,该材料正用于筛选与无花瓣性状紧密连锁的分子标记。
应用推荐