Effects of Temperature, Agitation, and Donor Strain on Chromosome Transfer in Escherichia coli K-12

Thomas H. Wood

首页> 外文期刊>Journal of bacteriology >Effects of Temperature, Agitation, and Donor Strain on Chromosome Transfer in Escherichia coli K-12

【24h】

Effects of Temperature, Agitation, and Donor Strain on Chromosome Transfer in Escherichia coli K-12

机译：温度，搅拌和供体菌株对大肠杆菌K-12中染色体转移的影响

获取原文

掌桥外文数据库（机构版） >>

开具论文收录证明 >>

文献代查 >>

页面导航

摘要
著录项
相似文献
相关主题

摘要

Recombinant production in Escherichia coli K-12 can be described by three parameters: (i) the distance x of a selected male marker from the donor origin; (ii) the gradient constant k (the probability of interruption of the donor chromosome per unit distance during transfer into a recipient cell); and (iii) the extrapolate number A (the probability that a donor cell will produce a recombinant inheriting the donor marker contiguous with the origin). It is usually assumed that chromosomal distances can be measured by marker entry times, i.e., that the velocity of chromosome transfer v is constant along the chromosome. The dependencies of k, A, x, and v on temperature, agitation during mating, and donor strain were studied. The transfer velocity of the HfrH chromosomal region from the origin to his increases 15-fold between 16 and 43 C, and the chromosomal regions studied have the same temperature dependence that was found for the separate transfer velocities of the O-trp and trp-his regions. These data and radiation studies on chromosome transfer indicate that, at a given temperature, chromosomal transfer velocity varies by less than 10% as the distance of any given region from the origin increases. The gradient constant k is temperature-independent between 20 and 45 C if mating times at different temperatures are inversely proportional to the chromosome velocities; also, k is insensitive to agitation during mating and is not decreased by mating on membrane filters. However, the extrapolate number A is highly temperature-dependent, having its maximum value between 30 and 38 C. These results suggest that the spontaneous interruption of transfer which produces the gradient of transfer is a property of the chromosome itself and not of the fragility of the connection between mating cells.

机译：大肠杆菌K-12中的重组生产可以通过三个参数来描述：（i）所选雄性标记与供体来源的距离 x ; （ii）梯度常数 k （在转移到受体细胞过程中每单位距离供体染色体被破坏的概率）; （iii）外推数 A （供体细胞产生重组体，该重组体继承与来源连续的供体标记）。通常假设可以通过标记进入时间来测量染色体距离，即染色体转移 v 的速度沿染色体是恒定的。研究了 k，A，x 和 v 对温度，交配时的搅拌和供体应变的依赖性。 HfrH染色体区域从原点到 his 的转移速度在16至43 C之间增加了15倍，并且所研究的染色体区域具有与温度的独立依赖的相同的温度依赖性。 O- trp 和 trp-his 地区。这些有关染色体转移的数据和辐射研究表明，在给定的温度下，随着任何给定区域与原点之间距离的增加，染色体转移速度的变化小于10％。如果在不同温度下的交配时间与染色体速度成反比，则梯度常数 k 在20至45 C之间与温度无关。同样， k 在交配期间对搅动不敏感，并且不会因在膜滤器上交配而降低。但是，外推数 A 高度依赖温度，其最大值在30到38 C之间。这些结果表明，自发的传递中断（产生传递梯度）是染色体的一个特性。本身，而不是配对单元之间连接的脆弱性。 展开▼

著录项

来源
《Journal of bacteriology》 |1968年第6期|共8页

作者
Thomas H. Wood;
展开▼

作者单位

展开▼

收录信息

原文格式 PDF

正文语种

中图分类微生物学;

关键词

相似文献

外文文献

中文文献

专利

1. GENE TRANSFER BY F′ STRAINS OF ESCHERICHIA COLI K-12 II. Interaction Between F-Merogenote and Chromosome During Transfer [J] . James Pittard, Edward A. Adelberg Journal of bacteriology . 1963,第6期

机译：大肠埃希氏菌K-12 F'株的基因转移II。 F-Merogenote和染色体之间的交互作用。

2. GENE TRANSFER BY F′ STRAINS OF ESCHERICHIA COLI K-12 I. Delay in Initiation of Chromosome Transfer [J] . James Pittard, John S. Loutit, Edward A. Adelberg Journal of bacteriology . 1963,第6期

机译：大肠埃希氏菌K-12 F'株的基因转移I.染色体转移启动的延迟

3. Abnormal Excision and Transfer of Chromosomal Segments by a Strain of Escherichia coli K-12 [J] . Peter L. Bergquist, Edward A. Adelberg Journal of bacteriology . 1972,第1期

机译：大肠杆菌菌株菌株的异常切除和转移染色体段

4. Chromosome engineering of Escherichia coli K-12 [C] . China-Japan-Korea Joint Symposium on Enzyme Engineering . 2004

机译：大肠杆菌K-12的染色体工程

5. Identification of genomic differences between Escherichia coli strains pathogenic for poultry and E. coli K-12 MG1655. [D] . Stocki, Stacy Lynn. 2003

机译：鉴定家禽致病性大肠杆菌菌株与大肠杆菌K-12 MG1655之间的基因组差异。

6. Effects of Temperature Agitation and Donor Strain on Chromosome Transfer in Escherichia coli K-12 [O] . Thomas H. Wood 1968

机译：温度搅拌和供体菌株对大肠杆菌K-12中染色体转移的影响

7. Abnormal Excision and Transfer of Chromosomal Segments by a Strain of Escherichia coli K-12 [O] . Peter L. Bergquist, Edward A. Adelberg 1972

机译：大肠杆菌菌株菌株的异常切除和转移染色体段

8. Alterations in the Pathogenicity of Escherichia coli K-12 After Transfer of Plasmid and Chromosomal Genes from Shigella flexneri. [R] . Sansonetti, P. J., Hale, T. L., Dammin, G. J., 1982

机译：转化弗氏志贺氏菌质粒和染色体基因后大肠杆菌K-12致病性的变化。

1. 后期酰基转移酶编码基因lpxL对禽致病性大肠杆菌菌株E058致病性的影响 [J] . 许慧卿 ,高璐 ,穆晓惠 . 畜牧兽医学报 . 2016,第009期

2. 大肠杆菌K-12转醛醇酶基因talB的克隆及在运动发酵单胞菌CP4中的表达 [J] . 管于平 ,刘成 ,邹少兰 . 工业微生物 . 2006,第002期

3. 大肠杆菌K-12中PFL家族基因的生物信息学分析 [J] . 韦宇拓 ,杨登峰 ,黄日波 . 广西农业生物科学 . 2005,第001期

4. 不同蔗糖浓度、供体细胞保存温度和融合温度对小鼠体细胞克隆胚胎发育的影响 [J] . 彭礼繁 ,罗光彬 ,白文林 . 广东畜牧兽医科技 . 2011,第003期

5. 一氧化氮供体SNP对不同苜蓿根瘤菌菌株生长的影响 [J] . 蔡卓山 ,尹国丽 ,师尚礼 . 草原与草坪 . 2020,第001期

6. 搅拌头尺寸对7075铝合金搅拌摩擦焊接头温度场及残余应力场的影响 [C] . 朱浩 ,赵熠朋 ,郭柱 . 2016焊接国际论坛 . 2016

7. 大肠杆菌K4软骨素合酶(KfoC)底物适应性分析及单糖供体对酶催化活性的影响 [A] . 薛佳俊 . 2016

1. 检测细菌基因水平转移DNA片段及转移供体菌株的方法 [P] . 中国专利： CN110660452B . 2020.10.27

2. 检测细菌基因水平转移以及发生水平转移DNA片段的供体菌株的方法 [P] . 中国专利： CN110660452A . 2020-01-07

3. 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

4. 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

5. 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

相关主题

Effects of Temperature, Agitation, and Donor Strain on Chromosome Transfer in Escherichia coli K-12

摘要

著录项

相似文献

相关主题

期刊订阅