Linker Scanning Mutagenesis by Three-Step PCR

互联网2014-02-13

853

A number of mutagenesis methods allow the systematic survey of a region of transcriptional regulatory sequence for identifying functional elements. In these methods, clusters or blocks of point mutations are introduced at discrete locations that span a suspected regulatory region of a gene. The individual mutants are then examined for retention of transcriptional activity typically in a reporter gene assay. Traditional methods, including linker-scanning mutagenesis (1 ) and microscale “shot-gun” gene synthesis (2 ), are either tedious and time-consuming or relatively inefficient at producing the desired mutated sequence. A modification of the PCR-based mutagenesis method originally described by Li and Shapiro (3 ) is much simpler, faster, and more efficient than the traditional methods.

相关产品推荐

荧光定量PCR（qRT-PCR）| 实时荧光定量PCR实验代测| 荧光定量PCR实验（realtime PCR）服务

询价

disA/disA蛋白/Cyclic di-AMP synthase (c-di-AMP synthase) (Diadenylate cyclase)蛋白/Recombinant Mycobacterium paratuberculosis DNA integrity scanning protein DisA (disA)重组蛋白

￥69

CLASP2/CLASP2蛋白Recombinant Human CLIP-associating protein 2 (CLASP2)重组蛋白Cytoplasmic linker-associated protein 2 Protein Orbit homolog 2 Short name: hOrbit2蛋白

￥5268

GoldStar Probe One Step RT-qPCR Kit，阿拉丁

￥1797.90

///蛋白/Three-finger toxin 3FTx-Oxy6蛋白/Recombinant Oxyuranus microlepidotus Toxin 3FTx-Oxy6重组蛋白

￥69