Genome Center and Department of Biochemistry and Molecular Medicine, University of California, Davis, California 95616, United States.
Biochemistry. 2011 Jun 7;50(22):5033-41. doi: 10.1021/bi200393g. Epub 2011 May 11.
Zinc finger nucleases (ZFNs) have been used to direct precise modifications of the genetic information in living cells at high efficiency. An important consideration in the design of ZFNs is the number of zinc fingers that are required for efficient and specific cleavage. We examined dimeric ZFNs composed of [1]+[1], [2]+[2], [3]+[3], [4]+[4], [5]+[5], and [6]+[6] zinc fingers, targeting 6, 12, 18, 24, 30, and 36 bp, respectively. We found that [1]+[1] and [2]+[2] fingers supported neither in vitro cleavage nor single-strand annealing in a cell-based recombination assay. An optimal ZFN activity was observed for [3]+[3] and [4]+[4] fingers. Surprisingly, [5]+[5] and [6]+[6] fingers exhibited significantly reduced activity. While the extra fingers were not found to dramatically increase toxicity, directly inhibit recombination, or perturb the ZFN target site, we demonstrate the ability of subsets of three fingers in six-finger arrays to bind independently to regions of the target site, possibly explaining the decrease in activity. These results have important implications for the design of new ZFNs, as they show that in some cases an excess of fingers may actually negatively affect the performance of engineered multifinger proteins. Maximal ZFN activity will require an optimization of both DNA binding affinity and specificity.
锌指核酸酶 (ZFNs) 已被用于高效地定向对活细胞中的遗传信息进行精确修饰。在 ZFNs 的设计中,一个重要的考虑因素是实现有效和特异性切割所需的锌指数量。我们研究了由 [1]+[1]、[2]+[2]、[3]+[3]、[4]+[4]、[5]+[5] 和 [6]+[6] 锌指组成的二聚体 ZFN,分别靶向 6、12、18、24、30 和 36 bp。我们发现 [1]+[1] 和 [2]+[2] 锌指既不支持体外切割,也不支持细胞内重组测定中的单链退火。[3]+[3] 和 [4]+[4] 锌指表现出最佳的 ZFN 活性。令人惊讶的是,[5]+[5] 和 [6]+[6] 锌指表现出显著降低的活性。虽然额外的锌指没有明显增加毒性、直接抑制重组或扰乱 ZFN 靶位点,但我们证明了六指阵列中三指子集能够独立结合靶位点的区域,这可能解释了活性降低的原因。这些结果对新 ZFNs 的设计具有重要意义,因为它们表明在某些情况下,过多的锌指实际上可能会对工程多锌指蛋白的性能产生负面影响。最大的 ZFN 活性将需要优化 DNA 结合亲和力和特异性。
