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首页> 外文期刊>The Journal of Biochemistry >Effects of Target Sequence and Sense versus Anti-sense Strands on Gene Correction with Single-stranded DNA Fragments.
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Effects of Target Sequence and Sense versus Anti-sense Strands on Gene Correction with Single-stranded DNA Fragments.

机译:目标序列和有义链与反义链对单链DNA片段基因校正的影响。

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摘要

The correction of an inactivated hygromycin resistance and enhanced green fluorescent protein (Hyg-EGFP) fusion gene by a several hundred-base single-stranded (ss) DNA fragment has been reported. In this study, the effectiveness of this type of gene correction was examined for various positions in the rpsL gene. Sense and anti-sense ssDNA fragments were prepared, and the gene correction efficiencies were determined by co-introduction of the target plasmid containing the gene with the ssDNA fragments. The gene correction efficiency varied (0.8-9.3%), depending on target positions and sense/anti-sense strands. Sense ssDNA fragments corrected the target gene with equal or higher efficiencies as compared to their anti-sense counterparts. The target positions corrected with high efficiency by the sense fragments also tended to be corrected efficiently by the anti-sense fragments. These results suggest that the sense ssDNA fragments are useful for the correction of mutated genes. The variation in the correction efficiency may depend on the sequence of the target position in double-stranded DNA.
机译:已经报道了通过数百个碱基的单链(ss)DNA片段纠正失活的潮霉素抗性和增强的绿色荧光蛋白(Hyg-EGFP)融合基因。在这项研究中,针对rpsL基因中的各个位置检查了此类基因校正的有效性。制备有义和反义ssDNA片段,并通过将含有基因的靶质粒与ssDNA片段共同引入来确定基因校正效率。基因校正效率因靶位和有义/反义链而异(0.8-9.3%)。有义ssDNA片段与其反义对应物相比以相同或更高的效率纠正了靶基因。被有义片段高效地校正的目标位置也趋于被反义片段有效地校正。这些结果表明,有义ssDNA片段可用于校正突变的基因。校正效率的变化可能取决于双链DNA中目标位置的顺序。

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