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pYEMF, a pUC18-Derived XcmI T-Vector for Efficient Cloning of PCR Products

机译:pYEMF,pUC18衍生的XcmI T载体,可高效克隆PCR产物

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摘要

A 1330-bp DNA sequence with two XcmI cassettes was inserted into pUC18 to construct an efficient XcmI T-vector parent plasmid, pYEMF. The large size of the inserted DNA fragment improved T-vector cleavage efficiency, and guaranteed good separation of the molecular components after restriction digestion. The pYEMF-T-vector generated from parent plasmid pYEMF permits blue/white colony screening; cloning efficiency analysis showed that most white colonies (75%) were putative transformants which carried the cloning product. The sequence analysis and design approach presented here will facilitate applications in the fields of molecular biology and genetic engineering.
机译:将具有两个XcmI盒的1330-bp DNA序列插入pUC18,以构建有效的XcmI T载体亲本质粒pYEMF。插入的DNA片段较大,可提高T载体的切割效率,并确保限制性酶切后分子成分的良好分离。由亲本质粒pYEMF产生的pYEMF-T-载体可以进行蓝/白菌落筛选;克隆效率分析表明,大多数白色菌落(> 75%)是携带克隆产物的推定转化子。本文介绍的序列分析和设计方法将有助于分子生物学和基因工程领域的应用。

著录项

  • 来源
    《Molecular Biotechnology》 |2011年第3期|p.229-233|共5页
  • 作者

    Jingsong Gu; Chunjiang Ye;

  • 作者单位

    Biotechnology Department, School of Medicine and Life Sciences, University of Jinan, 106 Jiwei Road, Jinan, 250022, China;

    Biotechnology Department, School of Medicine and Life Sciences, University of Jinan, 106 Jiwei Road, Jinan, 250022, China;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

    PCR product; Cloning; T-vector; XcmI;

    机译:PCR产物;克隆;T载体;XcmI;

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