CrisprStitch:Fast evaluation of the efficiency of CRISPR editing systems

Dear Editor,Targeted genome-editing technology using designed nucleases has been rapidly advancing and catalyzing significant breakthroughs in the life sciences.Custom-designed CRISPR editing experiments can be efficiently evaluated through nextgeneration sequencing(NGS).Nevertheless,NGS data analysis currently lacks a user-friendly pipeline capable of automatically calculating mutations and evaluating editing efficiency in bulk,as well as providing a more comprehensive visualization of results.

水稻染色体双链寡核苷酸荧光原位杂交技术

染色体制备与识别技术是遗传学研究的重要手段,而寡核苷酸荧光原位杂交(oligo-FISH)是近年来兴起的染色体识别技术。灵活高效的探针是荧光原位杂交过程中的关键因素。传统的单链寡核苷酸探针标记过程复杂,且获得单个探针的成本较高。在单链寡核苷酸探针的基础上进行改良,利用靶向全染色体(片段)的特异性引物进行扩增,将获得产物纯化,即可得到目的探针,简化了探针标记过程,降低了成本,并提高了标记效率。该文详述了水稻(Oryza sativa)改良后的双链寡核苷酸探针文库的合成及标记方法、有丝分裂时期染色体制片和探针杂交过程。通过设计梯度实验发现水稻中寡核苷酸荧光原位杂交技术染色体和寡核苷酸探针的最佳变性时间与温度分别为85℃ 3分钟30秒及90℃6分钟。该研究在水稻中建立染色体双链寡核苷酸荧光原位杂交技术,可为多种植物染色体制备与精准识别提供有力的工具。