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Simple and Efficient Targeting of Multiple Genes Through CRISPR-Cas9 in .

G3 (Bethesda). 2016; 
Lopez-ObandoMauricio,HoffmannBeate,GéryCarine,Guyon-DebastAnouchka,TéouléEvelyne,RameauCatherine,BonhommeSandrine,NoguéFa
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PCR Cloning and Subcloning Each fragment was cloned into pUC57 (GenScript) or pDONR207 (Invitrogen) backbones. Get A Quote

摘要

Powerful genome editing technologies are needed for efficient gene function analysis. The CRISPR-Cas9 system has been adapted as an efficient gene-knock-out technology in a variety of species. However, in a number of situations, knocking out or modifying a single gene is not sufficient; this is particularly true for genes belonging to a common family, or for genes showing redundant functions. Like many plants, the model organism has experienced multiple events of polyploidization during evolution that has resulted in a number of families of duplicated genes. Here, we report a robust CRISPR-Cas9 system, based on the codelivery of a CAS9 expressing cassette, multiple sgRNA vectors, and a cassette... More

关键词

AP2/ERF transcription factor,CRISPR-Cas9,KAI2,butenolide receptor,moss,multiple gene targe