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一种用于从酵母人工染色体中重组克隆大DNA片段的新型载体。

A new vector for recombination-based cloning of large DNA fragments from yeast artificial chromosomes.

作者信息

Bradshaw M S, Bollekens J A, Ruddle F H

机构信息

Department of Biology, Yale University, New Haven, CT 06520, USA.

出版信息

Nucleic Acids Res. 1995 Dec 11;23(23):4850-6. doi: 10.1093/nar/23.23.4850.

Abstract

The functional analysis of genes frequently requires manipulation of large genomic regions embedded in yeast artificial chromosomes (YACs). We have designed a yeast-bacteria shuttle vector, pClasper, that can be used to clone specific regions of interest from YACs by homologous recombination. The important feature of pClasper is the presence of the mini-F factor replicon. This leads to a significant increase in the size of the plasmid inserts that can be maintained in bacteria after cloning by homologous recombination in yeast. The utility of this vector lies in its ability to maintain large fragments in bacteria and yeast, allowing for mutagenesis in yeast and simplified preparation of plasmid DNA in bacteria. Using PCR-generated recombinogenic fragments in pClasper we cloned a 27 kb region from a YAC containing the Hoxc cluster and a 130 kb region containing the entire Hoxb cluster. No rearrangements were seen when the recombinants in the shuttle vector were transferred to bacteria. We outline the potential uses of pClasper for functional studies of large genomic regions by transgenic and other analyses.

摘要

对基因进行功能分析常常需要对嵌入酵母人工染色体(YAC)中的大片段基因组区域进行操作。我们设计了一种酵母 - 细菌穿梭载体pClasper,它可用于通过同源重组从YAC中克隆特定的感兴趣区域。pClasper的重要特征是存在mini-F因子复制子。这使得通过酵母中的同源重组克隆后能够在细菌中维持的质粒插入片段大小显著增加。该载体的实用性在于其能够在细菌和酵母中维持大片段,允许在酵母中进行诱变并简化细菌中质粒DNA的制备。利用pClasper中通过PCR产生的重组片段,我们从一个含有Hoxc簇的YAC中克隆了一个27 kb的区域以及一个包含整个Hoxb簇的130 kb区域。当穿梭载体中的重组体转移到细菌中时未观察到重排。我们概述了pClasper通过转基因和其他分析在大片段基因组区域功能研究中的潜在用途。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f810/307474/72a4744509f2/nar00023-0120-a.jpg

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