丁香实验_LOGO
登录
提问
我要登录
|免费注册
点赞
收藏
wx-share
分享

cDNA Cloning by Inverse Polymerase Chain Reaction

互联网

628
Since the first report on cDNA cloning in 1972 (1 ), this technology has been developed into a powerful and universal tool in the isolation, characterization, and analysis of both eukaryotic and prokaryotic genes. But the conventional methods of cDNA cloning require much effort to generate a library that is packaged in phage or plasmid and then to survey a large number of recombinant phages or plasmids. There are three major limitations of those methods. First, a substantial amount (at least 1 μg) of purified mRNA is needed as starting material to generate libraries of sufficient diversity (2 ). Second, the intrinsic difficulty of multiple sequential enzymatic reactions required for cDNA cloning often leads to low yields and truncated clones (3 ). Finally, screening of a library with hybridization technique is time-consuming.
提问
扫一扫
丁香实验小程序二维码
实验小助手
丁香实验公众号二维码
扫码领资料
反馈
TOP
打开小程序