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YAC transgenesis: a study of conditions to protect YAC DNA from breakage and a protocol for transfection

机译:YAC转基因:研究保护YAC DNA免受破坏的条件和转染方案

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Yeast artificial chromosomes (YACs) are providing a great boon to transgene technology by allowing the easy mutagenesis and study of very large DNAs. The large insert sizes of these vectors permit more accurate analysis of the regulation of transgene expression than smaller, more artificially assembled constructs. Transfection of mammalian cells by YACs can be accomplished by a number of methods; the most prevalent, using gel-purified DNA, is dependent upon compaction by salts to protect the large YAC DNA from breakage. We show that the common reliance on NaCl to compact YAC DNA sufficiently to protect it from breakage is not well-founded. Even the use of mixtures of polyamines and NaCl allows substantial damage to purified YACs. The use of polyamines alone in low salt buffers to compact YAC DNA provides the best protection from breakage and allows very effective transfection of murine embryonic stem (ES) cells. We provide a detailed method for ES cell transfection by YACs utilizing the DOTAP lipofection reagent that optimizes transfection efficiency and recovery of intact YACs.
机译:酵母人工染色体(YAC)通过易于诱变和研究非常大的DNA,为转基因技术提供了巨大的福音。与较小的,人工组装的构建体相比,这些载体的大插入体尺寸允许更准确地分析转基因表达。通过YAC转染哺乳动物细胞可以通过多种方法来完成。使用凝胶纯化的DNA,最普遍的方法是依靠盐的压缩来保护大的YAC DNA免受破坏。我们表明,依靠NaCl来压实YAC DNA足以保护其免受破坏的普遍依赖尚不充分。即使使用多胺和氯化钠的混合物,也可能对纯化的YAC造成实质性的损害。在低盐缓冲液中单独使用多胺来压实YAC DNA可以提供最佳的保护,防止破损,并可以非常有效地转染鼠胚胎干(ES)细胞。我们提供了利用DOTAP脂质转染试剂通过YAC转染ES细胞的详细方法,该试剂可优化转染效率和完整YAC的回收率。

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