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桥式PCR,一种简易连接DNA标签序列的方法(英文) 被引量:1

Bridge PCR,An Easy Way for Concatemerizing DNA Tags
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摘要 MAST方法采用人工文库的DNA标签序列鉴定mRNA的可接近位点。大量的标签序列通过扩增和克隆测序达到阐明mRNA结合位点图。设计了单一引物的PCR,其引物在标签序列两端结合搭桥,在扩增中DNA标签序列在搭桥引物的作用下进行连接,连接的标签序列再克隆和测序。十几条这样的连接产物包含了上千条标签序列。该PCR方法简单、高效以用于高通量的方式对标签序列测序。 In MAST ( mRNA accessible site tagging), the DNA tags from synthesized library were employed for identifying mRNA accessible sites. A large number of tags were amplified and subcloned for sequencing to verify mRNA binding profiles. A PCR was designed by using one primer which bridges over the tag terminal sequences. In PCR reaction DNA tag fragments were concatemerized by a bridge primer in reaction cycles. The concatemerized tag fragments were subcloned and sequenced. Dozens of the concatemerized sequences contained thousands tags. The PCR was a simple, effective way which for sequencing tags in a high through put manner.
作者 毛建平 王全会 周颖 方静 崔玉芳
机构地区 北京放射医学研究所
出处 《中国生物工程杂志》 CAS CSCD 北大核心 2009年第11期66-69,共4页 China Biotechnology
基金 Supported by China National Science & Technology Program(2008ZXJ09001-014) National Natural Science Foundation of China(30271546)~~
关键词 生物反应器 小鼠胚胎干细胞 拟胚体 心肌细胞 分化 Bioreactor Mouse embryonic stem cells Embryoid body Cardiomyocytes Differentiation
分类号 Q75 [生物学—分子生物学]
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中国生物工程杂志
2009年 第11期

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