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Evidence for Horizontal Transfer of the EcoT38I Restriction- Modification Gene to Chromosomal DNA by the P2 Phage and Diversity of Defective P2 Prophages in Escherichia coli TH38 Strains

机译：大肠杆菌TH38菌株中P2噬菌体和缺陷P2噬菌体多样性将EcoT38I限制性修饰基因水平转移至染色体DNA的证据

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A DNA fragment carrying the genes coding for a novel EcoT38I restriction endonuclease (R.EcoT38I) and EcoT38I methyltransferase (M.EcoT38I), which recognize G(A/G)GC(C/T)C, was cloned from the chromosomal DNA of Escherichia coli TH38. The endonuclease and methyltransferase genes were in a head-to-head orientation and were separated by a 330-nucleotide intergenic region. A third gene, the C.EcoT38I gene, was found in the intergenic region, partially overlapping the R.EcoT38I gene. The gene product, C.EcoT38I, acted as both a positive regulator of R.EcoT38I gene expression and a negative regulator of M.EcoT38I gene expression. M.EcoT38I purified from recombinant E. coli cells was shown to be a monomeric protein and to methylate the inner cytosines in the recognition sequence. R.EcoT38I was purified from E. coli HB101 expressing M.EcoT38I and formed a homodimer. The EcoT38I restriction (R)-modification (M) system (R-M system) was found to be inserted between the A and Q genes of defective bacteriophage P2, which was lysogenized in the chromosome at locI, one of the P2 phage attachment sites observed in both E. coli K-12 MG1655 and TH38 chromosomal DNAs. Ten strains of E. coli TH38 were examined for the presence of the EcoT38I R-M gene on the P2 prophage. Conventional PCR analysis and assaying of R activity demonstrated that all strains carried a single copy of the EcoT38I R-M gene and expressed R activity but that diversity of excision in the ogr, D, H, I, and J genes in the defective P2 prophage had arisen.

机译：从DNA的克隆DNA中克隆了一个DNA片段，该片段带有编码新型EcoT38I限制性核酸内切酶（R.EcoT38I）和EcoT38I甲基转移酶（M.EcoT38I）的基因。大肠杆菌TH38。核酸内切酶和甲基转移酶基因呈头对头方向，并被330个核苷酸的基因间区域隔开。在基因间区域中发现了第三个基因C.EcoT38I基因，与R.EcoT38I基因部分重叠。基因产物C.EcoT38I既充当R.EcoT38I基因表达的正调节剂，又充当M.EcoT38I基因表达的负调节剂。从重组大肠杆菌细胞中纯化的M.EcoT38I被证明是一种单体蛋白，可以在识别序列中甲基化内部胞嘧啶。 R.EcoT38I从表达M. Eco T38I的大肠埃希氏菌HB101中纯化，形成同型二聚体。发现在 A 和 Q 基因之间插入了 Eco T38I限制性（R）-修饰（M）系统（RM系统）。有缺陷的噬菌体P2，在染色体 loc I处被裂解，这是在两个 E 中观察到的P2噬菌体附着位点之一。大肠杆菌 K-12 MG1655和TH38染色体DNA。十株 E 。检查大肠杆菌 TH38在P2噬菌体中是否存在 Eco T38I R-M基因。常规PCR分析和R活性测定表明，所有菌株均携带 Eco T38I RM基因的单个拷贝并表达R活性，但 ogr ，<缺陷P2传播中出现了em> D ， H ， I 和 J 基因。 展开▼

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期刊名称 Journal of Bacteriology

作者
Keiko Kita; Hideaki Kawakami; Hiroaki Tanaka;
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年(卷),期 2003(185),7

年度 2003

页码 2296–2305

总页数 10

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中图分类微生物学;

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专利

1. Evidence for Horizontal Transfer of the EcoT38I Restriction- Modification Gene to Chromosomal DNA by the P2 Phage and Diversity of Defective P2 Prophages in Escherichia coli TH38 Strains [J] . Keiko Kita, Hideaki Kawakami, Hiroaki Tanaka Journal of bacteriology . 2003,第7期

机译：大肠杆菌TH38菌株中P2噬菌体和缺陷P2噬菌体多样性将EcoT38I限制性修饰基因水平转移至染色体DNA的证据

2. Evidence of Horizontal Transfer of theEcoO109I Restriction-Modification Gene to Escherichia coli Chromosomal DNA [J] . Keiko Kita, Junko Tsuda, Toshinobu Kato, Journal of bacteriology . 1999,第21期

机译：EcoO109I限制性修饰基因水平转移到大肠杆菌染色体DNA的证据

3. The Defective Prophage Pool of Escherichia coli O157: Prophage–Prophage Interactions Potentiate Horizontal Transfer of Virulence Determinants [J] . Akira Sawaguchi, Atsushi Iguchi, Keisuke Nakayama, PLoS Pathogens . 2009,第5期

机译：大肠杆菌O157的缺陷型噬菌体池：噬菌体与噬菌体的相互作用增强了毒力决定簇的水平转移

4. Do enterotoxigenic Escherichia coli strains isolated from Australian pigs carry transferable antimicrobial resistance genes of public health significance? [C] . M.G. Smith, T.A. Chapman, D. Jordan, Biennial Conference of the Australasian Pig Science Association . 2007

机译：从澳大利亚猪分离出肠毒素大肠杆菌菌株是否携带可转移的公共健康意义的抗菌性抗菌基因？

5. Regulation of chromosomal DNA replication in Escherichia coli: I. Function of an N-terminal domain in DnaA oligomer formation. II. Biochemical and genetic studies of hyperactive dnaA alleles [D] . Simmons, Lyle Adair 2003

机译：大肠杆菌中染色体DNA复制的调节：I. DnaA寡聚物形成中的N末端结构域的功能。二。过度活跃的dnaA等位基因的生化和遗传研究

6. Note: Evidence of Horizontal Transfer of the EcoO109I Restriction-Modification Gene to Escherichia coli Chromosomal DNA [O] . Keiko Kita, Junko Tsuda, Toshinobu Kato, 1999

机译：注：EcoO109I限制性修饰基因向大肠杆菌染色体DNA水平转移的证据

7. Evidence for Horizontal Transfer of the EcoT38I Restriction- Modification Gene to Chromosomal DNA by the P2 Phage and Diversity of Defective P2 Prophages in Escherichia coli TH38 Strains [O] . Kita, Keiko, Kawakami, Hideaki, Tanaka, Hiroaki 2003

机译：大肠杆菌TH38菌株中P2噬菌体和缺陷P2噬菌体多样性将EcoT38I限制性修饰基因水平转移至染色体DNA的证据

1. 抗噬菌体P2的植物乳杆菌突变菌株的筛选及其吸附特性研究 [J] . 柴诗语 ,郭静 ,孟根其其格 . 食品研究与开发 . 2019,第024期

2. 限制和修饰系统LlaBⅢ在构建抗噬菌体菌株中的作用 [J] . . 微生物学报 . 2002,第002期

1. GENE-THERAPEUTIC DNA-VECTOR BASED ON GENE-THERAPEUTIC DNA-VECTOR VTVAF17, CARRYING TARGET GENE SELECTED FROM GROUP OF GENES ANG, ANGPT1, VEGFA, FGF1, HIF1Α, HGF, SDF1, KLK4, PDGFC, PROK1, PROK2 TO INCREASE EXPRESSION LEVEL OF SAID TARGET GENES, METHOD FOR PRODUCTION AND USE THEREOF, STRAIN ESCHERICHIA COLI SCS110-AF/VTVAF17-ANG, OR ESCHERICHIA COLI SCS110-AF/VTVAF17-ANGPT1, OR ESCHERICHIA COLI SCS110-AF/VTVAF17-VEGFA, OR ESCHERICHIA COLI SCS110-AF/VTVAF17-FGF1, OR ESCHERICHIA COLI SCS110-AF/VTVAF17-HIF1Α, OR ESCHERICHIA COLI SCS110-AF/VTVAF17-HGF, OR ESCHERICHIA COLI SCS110-AF/VTVAF17-SDF1, OR ESCHERICHIA COLI SCS110-AF/VTVAF17-KLK4, OR ESCHERICHIA COLI SCS110-AF/VTVAF17-PDGFC, OR ESCHERICHIA COLI SCS110-AF/VTVAF17-PROK1, OR ESCHERICHIA COLI SCS110-AF/VTVAF17-PROK2, CARRYING GENE-THERAPEUTIC DNA VECTOR, METHOD FOR PRODUCTION THEREOF, METHOD FOR INDUSTRIAL PRODUCTION OF GENE-THERAPEUTIC DNA VECTOR [P] . 外国专利： RU2730664C2 . 2020-08-24

机译：基于基因治疗DNA载体VTVAF17的基因治疗DNA载体，携带选自基因ANG，ANGPT1，VEGFA，FGF1，HIF1α，HGF，SDF1，KLK4，PDGFC，PROK1，PROK2表达的靶基因所述的靶标基因，其生产和使用方法，应变大肠埃希氏菌SCS110-AF / VTVAF17-ANG或大肠埃希氏菌SCS110-AF / VTVAF17-ANGPT1或大肠埃希氏菌SCS110-AF / VTVAF17-VEGFA或大肠埃希氏菌SCS110-AF / VTVAF17-FGF1，或大肠埃希氏菌SCS110-AF / VTVAF17-HIF1A，或大肠埃希氏菌COLI SCS110-AF / VTVAF17-HGF，或大肠埃希氏菌SCS110-AF / VTVAF17-SDF1，或大肠埃希氏菌SCS110-AF / VTVAF17-KLK4，大肠埃希氏菌SCS110-AF / VTVAF17-PDGFC或大肠埃希氏菌SCS110-AF / VTVAF17-PROK2，携带基因-治疗性DNA载体，生产方法，工业生产方法-治疗性DNA载体

2. GENE-THERAPEUTIC DNA VECTOR BASED ON THE GENE-THERAPEUTIC DNA VECTOR GDTT1_8NAS12, CARRYING THE TARGET GENE SELECTED FROM A GROUP OF GENES DDC, IL10, IL13, IFNB1, TNFRSF4, TNFSF10, BCL2, HGF, IL2 TO INCREASE THE EXPRESSION LEVEL OF SAID TARGET GENES, A METHOD FOR PRODUCTION AND USE THEREOF, A STRAIN ESCHERICHIA COLI JM110-NAS/GDTT1_8NAS12-DDC OR ESCHERICHIA COLI JM110-NAS/GDTT1_8NAS12-IL10 OR ESCHERICHIA COLI JM110-NAS/GDTT1_8NAS12-IL13 OR ESCHERICHIA COLI JM110-NAS/GDTT1_8NAS12-IFNB1 OR ESCHERICHIA COLI JM110-NAS/GDTT1_8NAS12-TNFRSF4 OR ESCHERICHIA COLI JM110-NAS/GDTT1_8NAS12-TNFSF10 OR ESCHERICHIA COLI JM110-NAS/GDTT1_8NAS12-BCL2 OR ESCHERICHIA COLI JM110-NAS/GDTT1_8NAS12-HGF OR ESCHERICHIA COLI JM110-NAS/GDTT1_8NAS12-IL2, CARRYING A GENE-THERAPEUTIC DNA VECTOR, METHOD FOR PRODUCTION THEREOF, A METHOD FOR INDUSTRIAL PRODUCTION OF A GENE-THERAPEUTIC DNA VECTOR [P] . 外国专利： RU2734726C1 . 2020-10-22

机译：基于基因治疗DNA矢量GDTT1_8NAS12的基因治疗DNA矢量，携带从一组基因中选择的目标基因DDC，IL10，IL13，IFNB1，TNFRSF4，TNFSF10，BCL2，HGF，IL2可以增加表达水平基因，一种生产和使用其的方法，应变大肠埃希氏菌JM110-NAS / GDTT1_8NAS12-DDC或大肠埃希氏菌JM110-NAS / GDTT1_8NAS12-IL10或大肠埃希氏菌JM110-NAS / GDTT1_8NAS12-IL13或大肠埃希氏菌COLI JM110-NAS / GDTT1_8NAS12-IL13 IFNB1或ESCHERICHIA COLI JM110-NAS / GDTT1_8NAS12-TNFRSF4或ESCHERICHIA COLI JM110-NAS / GDTT1_8NAS12-TNFSF10或ESCHERICHIA COLI JM110-NAS / GDTT1_8NAS12-BCL2或ESCHERICHIA COLI JM110-NAS / GDTT1_8NAS12 IL2，携带基因治疗性DNA载体，其生产方法，工业生产基因治疗性DNA载体的方法

3. Gene therapeutic DNA vector based on VTvaf17 gene therapeutic DNA vector carrying a target gene selected from the group of genes ANG, ANGPT1, VEGFA, FGF1, HIF1α, HGF, SDF1, KLK4, PDGFC, PROK1, PROK2 to increase the expression level of these target genes, method its preparation and use, Escherichia coli strain SCS110-AF / VTvaf17-ANG or Escherichia coli SCS110-AF / VTvaf17-ANGPT1 or Escherichia coli SCS110-AF / VTvaf17-VEGFA or Escherichia coli SCS110-AF / VTvaf17-Fichia-SC110 AF / VTvaf17-HIF1α or Escherichia coli SCS110-AF / VTvaf17-HGF or Escherichia coli SCS110-AF / VTvaf17-SDF1 or Escherichia coli SCS110-AF / VTvaf17-KLK4 or Escherichia coli SCS110-AF / VTviFi10 SCF110 AF / VTvaf17-PROK1 or Escherichia coli SCS110-AF / VTvaf17-PROK2 carrying a gene therapy DNA vector, a method for its preparation, a method for the industrial production of a gene therapy DNA vector [P] . 外国专利： RU2018147085A . 2020-06-29

机译：基于VTvaf17基因治疗DNA载体的基因治疗DNA载体，其携带选自ANG，ANGPT1，VEGFA，FGF1，HIF1α，HGF，SDF1，KLK4，PDGFC，PROK1，PROK2的靶基因以增加这些靶标的表达水平基因，方法的制备和使用，大肠杆菌菌株SCS110-AF / VTvaf17-ANG或大肠杆菌SCS110-AF / VTvaf17-ANGPT1或大肠杆菌SCS110-AF / VTvaf17-VEGFA或大肠杆菌SCS110-AF / VTvaf17-Fichia-SC110 AF /VTvaf17-HIF1α或大肠杆菌SCS110-AF / VTvaf17-HGF或大肠杆菌SCS110-AF / VTvaf17-SDF1或大肠杆菌SCS110-AF / VTvaf17-KLK4或大肠杆菌SCS110-AF / VTviFi10 S1携带基因治疗DNA载体的大肠杆菌SCS110-AF / VTvaf17-PROK2，其制备方法，工业生产基因治疗DNA载体的方法

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Evidence for Horizontal Transfer of the EcoT38I Restriction- Modification Gene to Chromosomal DNA by the P2 Phage and Diversity of Defective P2 Prophages in Escherichia coli TH38 Strains

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