Händel Eva-Maria, Alwin Stephen, Cathomen Toni
Charité Medical School, Institute of Virology (CBF), Berlin, Germany.
Mol Ther. 2009 Jan;17(1):104-11. doi: 10.1038/mt.2008.233. Epub 2008 Nov 11.
Precise manipulations of complex genomes by zinc-finger nucleases (ZFNs) depend on site-specific DNA cleavage, which requires two ZFN subunits to bind to two target half-sites separated by a spacer of 6 base pairs (bp). ZFN subunits consist of a specific DNA-binding domain and a nonspecific cleavage domain, connected by a short inter-domain linker. In this study, we conducted a systematic analysis of 11 candidate-based linkers using episomal and chromosomal targets in two human cell lines. We achieved gene targeting in up to 20% of transfected cells and identified linker variants that enforce DNA cleavage at narrowly defined spacer lengths and linkers that expand the repertoire of potential target sites. For instance, a nine amino acid (aa) linker induced efficient gene conversion at chromosomal sites with 7- or 16-bp spacers, whereas 4-aa linkers had activity optima at 5- and 6-bp spacers. Notably, single aa substitutions in the 4-aa linker affected the ZFN activity significantly, and both gene conversion and ZFN-associated toxicity depended on the linker/spacer combination and the cell type. In summary, both sequence and length of the inter-domain linker determine ZFN activity and target-site specificity, and are therefore important parameters to account for when designing ZFNs for genome editing.
锌指核酸酶(ZFNs)对复杂基因组的精确操作依赖于位点特异性DNA切割,这需要两个ZFN亚基与由6个碱基对(bp)的间隔区隔开的两个靶半位点结合。ZFN亚基由一个特定的DNA结合结构域和一个非特异性切割结构域组成,通过一个短的结构域间连接子相连。在本研究中,我们使用两种人类细胞系中的游离型和染色体靶标,对11种基于候选的连接子进行了系统分析。我们在高达20%的转染细胞中实现了基因靶向,并鉴定出在狭窄定义的间隔区长度上增强DNA切割的连接子变体,以及扩展潜在靶位点库的连接子。例如,一个九氨基酸(aa)的连接子在具有7或16 bp间隔区的染色体位点诱导了高效的基因转换,而4 aa的连接子在5和6 bp间隔区具有最佳活性。值得注意的是,4 aa连接子中的单个氨基酸替换显著影响ZFN活性,并且基因转换和ZFN相关毒性均取决于连接子/间隔区组合和细胞类型。总之,结构域间连接子的序列和长度均决定ZFN活性和靶位点特异性,因此是设计用于基因组编辑的ZFN时需要考虑的重要参数。