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Efficient production of Cre-mediated site-directed recombinants through the utilization of the puromycin resistance gene pac: a transient gene-integration marker for ES cells.

机译：通过利用嘌呤霉素抗性基因pac：ES细胞的瞬时基因整合标记可有效生产Cre介导的定点重组子。

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Gene targeting in embryonic stem (ES) cells is a powerful tool for generating mice carrying specifically designed mutations in the germline. Puromycin can completely kill ES cells within 24 to 48 h whereas G418 and hygromycin cannot. We have, therefore, proposed that the puromycin N-acetyltransferase ( pac ) gene, may be utilized as a transient gene-integration marker. Using a circular expression vector of cre and pac genes, Cre-mediated mutant cells were effectively enriched by pulse treatment of puromycin without stable integration of their genes. We have thus demonstrated the first application of pac as a transient gene-integration marker for ES cells.

机译：胚胎干（ES）细胞中的基因靶向是一种强大的工具，可用于产生在种系中携带专门设计的突变的小鼠。嘌呤霉素可以在24至48小时内完全杀死ES细胞，而G418和潮霉素则不能。因此，我们提出了嘌呤霉素N-乙酰基转移酶（pac）基因可用作瞬时基因整合标记。使用cre和pac基因的环状表达载体，通过脉冲处理嘌呤霉素可有效富集Cre介导的突变细胞，而无需稳定整合其基因。因此，我们证明了pac作为ES细胞的瞬时基因整合标记的首次应用。

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期刊名称 Nucleic Acids Research
作者
M Taniguchi; M Sanbo; S Watanabe; I Naruse; M Mishina; T Yagi;
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年(卷),期 1998(26),2
年度 1998
页码 679–680
总页数 2
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. Efficient production of Cre-mediated site-directed recombinants through the utilization of the puromycin resistance gene, pac: a transient gene-integration marker for ES cells. [J] . Taniguchi M, Sanbo M, Watanabe S, Nucleic Acids Research . 1998,第2期

机译：通过利用嘌呤霉素抗性基因pac高效生产Cre介导的定点重组子，pac是ES细胞的瞬时基因整合标记。
2. Efficient production of Cre-mediated site-directed recombinants through the utilization of the puromycin resistance gene, pac: A transient gene-integration marker for ES cells [J] . Ichiro Naruse, Makoto Sanbo, Masahiko Taniguchi, Nucleic acids research . 1998,第2期

机译：利用嘌呤霉素抗性基因pac高效生产Cre介导的定点重组子：pac是ES细胞的瞬时基因整合标记
3. The functional recombinant first extracellular (EC1) domain of PACAP receptor PAC1 normal form (PAC1-EC1(N)) recognizes selective ligands and stimulates the proliferation of PAC1-CHO cells. [J] . Yu R, Li J, Wang J, Neuroscience Letters: An International Multidisciplinary Journal Devoted to the Rapid Publication of Basic Research in the Brain Sciences . 2010,第1期

机译：PACAP受体PAC1正常形式（PAC1-EC1（N））的功能性重组第一细胞外（EC1）结构域识别选择性配体并刺激PAC1-CHO细胞的增殖。
4. TRANSIENT GENE EXPRESSION: A NOVEL MAMMALIAN CELL-BASED TECHNOLOGY FOR RECOMBINANT PROTEIN PRODUCTION: A historical and technical perspective [C] . F.M. WURM, L. BALDI, J. P. GIRARD, Annual Meeting of the Japanese Association for Animal Cell Technology . 2003

机译：瞬态基因表达：一种新型哺乳动物细胞的重组蛋白质生产技术：历史和技术视角
5. Efficient Generation of Recombinant Hydrazides for the Production of Scarce Proteins and Development of Chemical Probes for Detecting Protein Sulfenylation [D] . Ekanayake, Oshini . 2020

机译：用于生产稀缺蛋白质的重组含肼的高效产生以及用于检测蛋白质磺化化的化学探针的发育
6. Genetic Approach To Study the Relationship between Penicillin-Binding Protein 3 Mutations and Haemophilus influenzae β-Lactam Resistance by Using Site-Directed Mutagenesis and Gene Recombinants [O] . Yumi Osaki, Yumiko Sanbongi, Midori Ishikawa, 2005

机译：利用定点诱变和基因重组研究青霉素结合蛋白3突变与流感嗜血杆菌β-内酰胺抗性关系的遗传方法
7. Efficient production of Cre-mediated site-directed recombinants through the utilization of the puromycin resistance gene, pac: a transient gene-integration marker for ES cells. [O] . Taniguchi, M, Sanbo, M, Watanabe, S, 1998

机译：通过利用嘌呤霉素抗性基因pac：ES细胞的瞬时基因整合标记，可有效生产Cre介导的定点重组子。
8. Mutagenicity Testing in Mammalian Cells. Multiple Drug-Resistance Markers [R] . Carver, J. H. , Adair, G. M. , Wandres, D. L. 1979

机译：哺乳动物细胞的致突变性测试。多种耐药标记物

Efficient production of Cre-mediated site-directed recombinants through the utilization of the puromycin resistance gene pac: a transient gene-integration marker for ES cells.

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