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A YAC contig encompassing the XRCC5 (Ku80) DNA repair gene and complementation of defective cells by YAC protoplast fusion.一个包含XRCC5(Ku80)DNA修复基因的酵母人工染色体连续克隆系,以及通过酵母人工染色体原生质体融合对缺陷细胞进行互补。
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Specific cloning of human DNA as yeast artificial chromosomes by transformation-associated recombination.通过转化相关重组将人类DNA作为酵母人工染色体进行特异性克隆。
Proc Natl Acad Sci U S A. 1996 Jan 9;93(1):491-6. doi: 10.1073/pnas.93.1.491.
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Direct cloning of yeast genes from an ordered set of lambda clones in Saccharomyces cerevisiae by recombination in vivo.通过体内重组从酿酒酵母中一组有序的λ克隆直接克隆酵母基因。
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Cloning and characterization of EagI YACs from human chromosome 21.来自人类21号染色体的EagI酵母人工染色体的克隆与特性分析
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Extrachromosomal maintenance and amplification of yeast artificial chromosome DNA in mouse cells.酵母人工染色体DNA在小鼠细胞中的染色体外维持与扩增
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Construction and characterization of a YAC library with a low frequency of chimeric clones from flow-sorted human chromosome 9.来自流式分选的人类9号染色体的低嵌合克隆频率酵母人工染色体文库的构建与鉴定
Genomics. 1993 Dec;18(3):553-8. doi: 10.1016/s0888-7543(05)80355-6.
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A model system to assess the integrity of mammalian YACs during transformation and propagation in yeast.一种用于评估哺乳动物酵母人工染色体(YACs)在酵母中转化和增殖过程中完整性的模型系统。
Genomics. 1994 May 1;21(1):7-17. doi: 10.1006/geno.1994.1218.
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Efficient manipulation of the human adenovirus genome as an infectious yeast artificial chromosome clone.作为感染性酵母人工染色体克隆对人腺病毒基因组进行有效操作。
Proc Natl Acad Sci U S A. 1994 Jun 21;91(13):6186-90. doi: 10.1073/pnas.91.13.6186.
10
Recombination during transformation as a source of chimeric mammalian artificial chromosomes in yeast (YACs).转化过程中的重组作为酵母人工染色体(YACs)中嵌合哺乳动物人工染色体的来源。
Nucleic Acids Res. 1994 Oct 11;22(20):4154-62. doi: 10.1093/nar/22.20.4154.

通过转化相关重组克隆从啮齿动物-人类杂交细胞中高度选择性分离人类DNA作为环状酵母人工染色体。

Highly selective isolation of human DNAs from rodent-human hybrid cells as circular yeast artificial chromosomes by transformation-associated recombination cloning.

作者信息

Larionov V, Kouprina N, Graves J, Resnick M A

机构信息

Laboratory of Molecular Genetics, National Institute of Environmental Health Sciences, National Institutes of Health, Research Triangle Park, NC 27709, USA.

出版信息

Proc Natl Acad Sci U S A. 1996 Nov 26;93(24):13925-30. doi: 10.1073/pnas.93.24.13925.

DOI:10.1073/pnas.93.24.13925
PMID:8943037
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC19470/
Abstract

Transformation-associated recombination (TAR) can be exploited in yeast to clone human DNAs. TAR cloning was previously accomplished using one or two telomere-containing vectors with a common human repeat(s) that could recombine with human DNA during transformation to generate yeast artificial chromosomes (YACs). On basis of the proposal that broken DNA ends are more recombinogenic than internal sequences, we have investigated if TAR cloning could be applied to the generation of circular YACs by using a single centromere vector containing various human repeats at opposite ends. Transformation with these vectors along with human DNA led to the efficient isolation of circular YACs with a mean size of approximately 150 kb. The circular YACs are stable and they can be easily separated from yeast chromosomes or moved into bacterial cells if the TAR vector contains an Escherichia coli F-factor cassette. More importantly, circular TAR cloning enabled the selective isolation of human DNAs from monochromosomal human-rodent hybrid cell lines. Although < 2% of the DNA in the hybrid cells was human, as much as 80% of transformants had human DNA YACs when a TAR cloning vector contained Alu repeats. The level of enrichment of human DNA was nearly 3000-fold. A comparable level of enrichment was demonstrated with DNA isolated from a radiation hybrid cell line containing only 5 Mb of human DNA. A high selectivity of human DNA cloning was also observed for linear TAR cloning with two telomere vectors. No human-rodent chimeras were detected among YACs generated by TAR cloning. The results with a circular TAR cloning vector or two vectors differed from results with a single-telomere vector in that the latter often resulted in a series of terminal deletions in linear YACs. This could provide a means for physical mapping of cloned material.

摘要

转化相关重组(TAR)可用于酵母中克隆人类DNA。TAR克隆以前是通过使用一个或两个含端粒的载体来完成的,这些载体带有常见的人类重复序列,在转化过程中可与人类DNA重组以产生酵母人工染色体(YAC)。基于断裂的DNA末端比内部序列更具重组活性这一观点,我们研究了TAR克隆是否可通过使用一个在两端含有各种人类重复序列的单着丝粒载体来应用于环状YAC的产生。用这些载体与人类DNA一起转化可高效分离出平均大小约为150 kb的环状YAC。这些环状YAC是稳定的,如果TAR载体含有大肠杆菌F因子盒,它们可以很容易地与酵母染色体分离或转移到细菌细胞中。更重要的是,环状TAR克隆能够从单染色体人类 - 啮齿动物杂种细胞系中选择性分离人类DNA。尽管杂种细胞中<2%的DNA是人类DNA,但当TAR克隆载体含有Alu重复序列时,高达80%的转化体含有人类DNA YAC。人类DNA的富集水平接近3000倍。从仅含5 Mb人类DNA的辐射杂种细胞系中分离的DNA也证明了类似的富集水平。对于使用两个端粒载体的线性TAR克隆,也观察到了人类DNA克隆的高选择性。在TAR克隆产生的YAC中未检测到人类 - 啮齿动物嵌合体。使用环状TAR克隆载体或两个载体的结果与使用单端粒载体的结果不同,后者通常会导致线性YAC中出现一系列末端缺失。这可为克隆材料的物理图谱绘制提供一种方法。