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A novel procedure for selective cloning of NotI linking fragments from mammalian genomes.

机译：一种从哺乳动物基因组选择性克隆NotI连接片段的新方法。

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摘要

A novel procedure has been developed for selective cloning of NotI linking fragments from mammalian genomes. Since the majority of the NotI sites in mammalian genomes are considered to be localized in so-called HTF (HpaII tiny fragment) islands, an HTF library was constructed as an initial step to enrich the NotI sites. The plasmid DNAs were isolated en masse from the HTF library and digested with NotI. Linearized plasmid DNAs derived from NotI linking clones were efficiently separated from undigested circular DNAs by an unique pulsed field polyacrylamide gel electrophoresis (PF-PAGE). The linear DNAs were eluted from the gel, recircularized with T4 DNA ligase and introduced into E. coli cells. About 95% of the transformants were found to contain NotI linking fragments. The procedure will thus provide a simple and useful way of collecting NotI linking fragments for long range physical mapping of mammalian genomes.

机译：已经开发了一种新方法，用于选择性克隆来自哺乳动物基因组的NotI连接片段。由于哺乳动物基因组中的大多数NotI位点被认为位于所谓的HTF（HpaII小片段）岛中，因此构建了一个HTF文库作为富集NotI位点的第一步。从HTF文库中大规模分离质粒DNA，并用NotI消化。通过独特的脉冲场聚丙烯酰胺凝胶电泳（PF-PAGE），可以有效地将NotI连接克隆衍生的线性化质粒DNA与未消化的环状DNA分离。从凝胶上洗脱线性DNA，用T4 DNA连接酶重新环化并导入大肠杆菌细胞。发现约95％的转化体含有NotI连接片段。因此，该方法将提供一种收集NotI连接片段的简单而有用的方式，用于哺乳动物基因组的远距离物理作图。

著录项

期刊名称 Nucleic Acids Research
作者
T Ito; Y Sakaki;
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作者单位

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年(卷),期 1988(16),19
年度 1988
页码 9177–9184
总页数 8
原文格式 PDF
正文语种
中图分类分子生物学;
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专利

1. A novel procedure for selective cloning of NotI linking fragments from mammalian genomes [J] . Takashi Ito, Yoshiyuki Sakaki Nucleic acids research . 1988,第19期

机译：从哺乳动物基因组选择性克隆NotI连接片段的新方法
2. Detection and cloning of an X-linked locus associated with a NotI site that is not methylated on mouse inactivated X chromosome by the RLGS-M method. [J] . Takada S, Kamiya M, Arima T, Genomics . 1999,第1期

机译：通过RLGS-M方法检测和克隆与不在小鼠灭活的X染色体上甲基化的NotI位点相关的X连锁基因座。
3. NotI linking/jumping clones of human chromosome 3: mapping of the TFRC, RAB7 and HAUSP genes to regions rearranged in leukemia and deleted in solid tumors [J] . Allikmets R, Boldog F, Gizatullin R.Z, FEBS Letters . 1997,第2a3期

机译：NotI连接/跳跃人类染色体3的克隆：将TFRC，RAB7和HAUSP基因定位到白血病中重排并在实体瘤中缺失的区域
4. Selectively controlling the 2D organization of mammalian cells: Templated assembly by selective removal (TASR) for medical applications [C] . Agarwal G., Livermore C. 2014 40th Annual Northeast Bioengineering Conference . 2014

机译：选择性控制哺乳动物细胞的2D组织：用于医学应用的选择性去除（TASR）模板化装配
5. Detecting linked changes in fast-evolving genomes. [D] . Ahn, Chaehyung. 2005

机译：检测快速发展的基因组中的连锁变化。
6. Construction of a human chromosome 3 specific NotI linking library using a novel cloning procedure. [O] . E R Zabarovsky, F Boldog, T Thompson, 1990

机译：使用新型克隆程序构建人类3号染色体特异性NotI连接文库。
7. A novel procedure for selective cloning of NotI linking fragments from mammalian genomes. [O] . Ito, T, Sakaki, Y 1988

机译：一种从哺乳动物基因组选择性克隆NotI连接片段的新方法。

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