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Query: UNIPROT:P06889 (
Mol
)
630,302
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
The Ti-plasmids are naturally self-transmissible from their normal host Agrobacterium to E. coli. They are however unable to stably establish themselves as a replicon in E. coli. It is nevertheless possible to study the Ti-plasmids in E. coli with the help of Ti::
RP4
cointegrate plasmids that transfer and maintain themselves very efficiently in E. coli. An E. coli harbouring such a Ti::
RP4
plasmid is unable to catabolize octopine and unable to induce crown-gall tumours on plants.
Mol
Gen Genet 1978 Jul 25
PMID:In vivo transfer of the ti-plasmid of Agrobacterium tumefaciens to Escherichia coli. 15 May 36
The region of the phage lambda chromosome containing the attachment site (P.P') and the genes int and xis, excised by the action of endonuclease R.EcoRI, has been inserted into the unique site for that enzyme on the promiscuous conjugative plasmid,
RP4
, generating the recombinant plasmid RP4att lambda. Transformants containing the hybrid plasmid were recognised by their ability to allow efficient lysogenization by phage lambda b2 (Weil and Signer, 1968; Echols et al., 1968) containing the mutant attachment site delta. P'. The construction and properties of the hybrid plasmid RP4att lambda are described.
Mol
Gen Genet 1979
PMID:In vitro insertion of the lambda attachment site into the plasmid RP4. 23 25
Insertion of transposon T n1 into the E. coli JC411 chromosome results in a sharp increase of plasmid
RP4
integration frequency. This effect is absent in JC1553 recA cells. The
RP4
integration with the chromosome is probably accomplished via recA-dependent recombination between transposon Tn1 inserted into the chromosome and the same transposon in the
RP4
plasmid.
Mol
Gen Genet 1978 May 31
PMID:Transposon-mediated insertion of R factor into bacterial chromosome. 35 20
The freeze thaw transfection procedure of Dityatkin et al. (1972) was adapted for the transfection and transformation of A. tumefaciens. Transfection of the strains B6S3 and B6-6 with DNA of the temperate phage PS8cc186 yielded a maximum frequency of 2 10(-7) transfectants per total recipient population. In transformation of the strain GV3100 with the P type plasmid
RP4
a maximum frequency of 3.5 10(-7) transformants per total recipient population was obtained. Agrobacterium Ti-plasmids were introduced in the strain GV3100 with a maximal efficiency of 4.5 10(-8). These experiments provide further evidence that the Ti-plasmid is responsible for the oncogenic properties of A tumefaciens and for its capacity to induce "opine" synthesis in Crown-gall plant cells.
Mol
Gen Genet 1978 Jul 11
PMID:Transfection and transformation of Agrobacterium tumefaciens. 35 47
We used the hybrid plasmid pAS8 in order to conduct the genetic analysis of
RP4
plasmid. The presence of two replicons in the hybrid plasmid permitted to expand the spectrum of deletion mutants of
RP4
isolated, which are capable to autonomous replication. The shortening of the hybrid plasmid was achieved by P22 transduction, by induction of deletion mutants using mitomycin C, as well as by seletion of Tra- mutants on the basis of resistance of cells to P-specific phages. These techniques have lead to isolation of clones possessing different combinations of plasmid resistance determinants. Comparison of phenotypic characteristics of deletion plasmids pAS9, pAS10, pAS11, pAS12 and pAS10-2 permitted to propose the map for pAS8 plasmid with the following sequence of markers: tra--kam--ColE1--amp--tet... Heteroduplex analysis of deletion mutants of pAS8 permitted to construct a physical map and to elaborate in greater detail the functional map of
RP4
plasmid. The correlation between the ability of mutants to replicate in polA(TS) strain at nonpermissive conditions and the length of the deleted segment permitted to map rep genes of
RP4
on a region with coordinates 9.8--17.3 kb. A relationship between the manifestation of incompatibility of mutants with Inc P-1 plasmids and the length of deletions points out that inc genes are located on DNA region with coordinates 2.1--9.8 kb. The analysis of replication of deletion mutants and the manifestation of incompatibility just as of the data about the size of appropriate deletions permitted to make the conclusion about the functional and genetic independence of the replication control and incompatibility control in
RP4
plasmid.
Mol
Gen Genet 1978 Oct 24
PMID:Mapping of RP4 plasmid using deletion mutants of pAS8 hybrid (RP4--ColE1). 36 65
The his and nif genes of the P1 type plasmid pRD1 were lost at a high frequency in a recA+ but not in a recA- Escherichia coli host during growth in a non-selective medium. 92% of the His- Nif- segregants after 6 subcultures retained the genetic markers of the precursor plasmid
RP4
, while the remainder lost all of the pRD1 markers with the concomitant loss of ccc-DNA. Plasmids purified from the His- Nif- segregants resembled
RP4
in the physical and genetic properties examined. The contour length of pRD1 DNA molecules from a recA- strain was 49 micrometer corresponding to a molecular weight of 101 Mdals and the buoyant density was 1.715 g/cm3. In contrast, the contour lengths of plasmid molecules isolated from a recA+ host carrying pRD1 fell into 3 size classes of 49, 19 and 2 micrometer corresponding to molecular weights of 101, 39 and 4 Mdals respectively and two DNA species of buoyant density 1.715 and 1.719 g/cm3 were observed.
Mol
Gen Genet 1979 Mar 09
PMID:Spontaneous degradation of pRD1 DNA into unique size classes is recA dependent. 37 20
RP4
-trp hybrid plasmid containing Escherichia coli whole tryptophan operon was conjugatively transferred from E. coli to Rhizobium leguminosarum strains carrying mutations in different trp genes, converting their Trp- phenotype to Trp+. That the phenotype change of the R. leguminosarum cells was due to the presence of the E. coli tryptophan operon was verified by the isolation of
RP4
-trp hybrid plasmid from the R. leguminosarum conjugant cells, and by re-transfer of
RP4
-trp plasmid by conjugation back to E. coli trp and Pseudomonas putida trp strains. Enzymatic activities of anthranilate synthetase and beta subunit of tryptophan synthetase in crude extracts of R. leguminosarum cells containing
RP4
-trp plasmid were much higher than that of the wild-type cells and were not repressed by the presence of tryptophan in the culture medium.
Mol
Gen Genet 1979 Mar 20
PMID:Expression of Escherichia coli tryptophan operon in Rhizobium leguminosarum. 37 25
RP4
-prime plasmids containing chromosomal fragments of either Escherichia coli or Rhizobium meliloti were constructed in vitro. When introduced into E. coli or R. meliloti respectively, they promoted a polarized transfer of the chromosome as demonstrated either by the gradient of transfer of various markers or by the study of the genetic constitution of recombinants. In E. coli, mobilization was shown to be dependent upon the presence of a functional rec A system. Inheritance of markers was due to their integration into the chromosome of the recipient as shown by the need for a functional rec A system in the recipient E. coli or by mobilization of recessive markers in R. meliloti. The system described could be applied to genetic mapping in any Gram negative bacteria.
Mol
Gen Genet 1979 Jun 20
PMID:Use of RP4-prime plasmids constructed in vitro to promote a polarized transfer of the chromosome in Escherichia coli and Rhizobium meliloti. 38 51
R plasmid
RP4
inhibits the fertility of R. lupini. An
RP4
carrying R. lupini donor strain is no longer capable of transferring chromosomal genes. After loss of
RP4
the R. lupini fertility reappears. Plasmid
RP4
spontaneously mutates at high frequency in R. lupini.
RP4
mutants which do not inbibit fertility were isolated. These mutants were always transfer-defective, too. It is postulated that the genetic information for fertility inhibition in R. lupini is a substantial part of the transfer unit of the
RP4
plasmid.
Mol
Gen Genet 1978 Jun 14
PMID:Fertility inhibition in Rhizobium lupini by the resistance plasmid RP4. 67 1
Plasmids have been constructed by insertion of DNA from Rhizobium leguminosarum or Proteus mirabilis into
RP4
(an R factor of group P). Such recombinant plasmids retain the wide host range of the parental plasmid, being as efficiently transmissible as the unmodified
RP4
and are stably maintained in rapidly growing cultures. The recombinant plasmids, even though each contained a DNA sequence absolutely identical with that of the host strain, are no more efficient at mobilizing the transfer of chromosomal genetic information from that host strain than was unmodified
RP4
. We therefore conclude that an unknown factor must be essential in the process of chromosome mobilization and rate limiting for that process.
Mol
Gen Genet 1976 Sep 23
PMID:Properties of plasmids constructed by the in vitro insertion of DNA from Rhizobium leguminosarum or Proteus mirabilis into RP4. 78 66
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