Cloning of F DNA fragments carrying the origin of transfer oriT and the fertility inhibition gene finP

The two SalI fragments derived from the F transfer region that are bounded at one end by the SalI cleavage site in traM were cloned into pBR322. From these, smaller (540 bases) SalI-BglII fragments were subcloned to give plasmids containing the origin of transfer oriT (pED806) and finP (pED812), respectively, but no entire tra genes. All four plasmids were characterized by genetic tests and by restriction endonuclease analysis. pED806 could not be used to search for an F oriT-related “relaxation complex” because of its unexpected instability in the presence of Flac, and extensive efforts to prepare such a complex using other oriT⁺ plasmids were unsuccessful. We therefore suggest that a cell-free F relaxation complex does not exist. Protein synthesis directed by pED812 in minicells allowed the finP product to be tentatively identified as a 4000 M_r, protein.     

Characterisation of an in vivo system for nicking at the origin of conjugal DNA transfer of the sex factor F

Transfer of the F plasmid between conjugating Escherichia coli cells has been assumed to require endonucleolytic cleavage at a specific site (oriT) on a specific strand of the F molecule. Using a lambda transducing phage which contains oriT we have detected this nicking process in vivo. Nicking of DNA occurred in the strand that included the “transferred” F strand and at a location within the transducing segment consistent with all previous genetic and restriction enzyme cleavage data on the position of oriT in F. Genetic study of the nicking process using Flac tra^? point and deletion mutants, and also λtra phages which carried various parts of the transfer region, indicated that the products of two transfer operon genes, traY and the previously unidentified gene traZ, were directly involved in nicking at oriT. The product of traJ was also required for nicking, but the possibility that this was solely due to the regulatory function of the traJ product could not be excluded. The plasmid specificities of oriT, traY and traZ between F and the related F-like plasmids R1-19 and R100-1 were investigated using the λoriT nicking system, and shown to be consistent with those determined in genetic complementation tests. The differences in specificity observed imply that the oriT sequence of F differs from those of R1-19 and R100-1.The products of the traM and traI genes are known to be required for the initiation of DNA transfer; their possible roles in modulating the activity of the traY Z endonuclease are discussed.     

The structure and histochemistry of sclerotia ofSclerotinia minor Jagger

Summary A detailed histochemical investigation was carried out on rind, cortical and medullary hyphae of sclerotia ofSclerotinia minor Jagger. Four developmental stages, including mature sclerotia, were studied. The walls and septa of all hyphae contained chitin and -1,3 glucans, while those of the rind contained in addition, a melanin-like pigment. An extracellular matrix, which accumulated around cortical and medullary hyphae, consisted primarily of -1,3 glucans, although another polysaccharide, which could not be identified by histochemical methods, was also present. Phenolic material was deposited around the extracellular matrix and in the few interhyphal spaces that remained at maturity. Glycogen was present throughout the cytoplasm of hyphae of the cortex and medulla, at all stages of their differentiation. Polyphosphate granules were laid down within small vacuoles and as sclerotia matured, became most common in the cortical region. Protein bodies developed rapidly in cortical and medullary hyphae until at maturity, they were the most obvious interhyphal feature. These bodies were either round or elongated in shape, the elongated ones often lying parallel to the long axis of the hyphae, and in close association with strands of endoplasmic reticulum. No lipid reserves were detected.Mrs. S.Lowry.     

Biotransformations by microbial Baeyer-Villiger monooxygenases stereoselective lactone formationin vitro by coupled enzyme systems

Summary The regio- and stereoselective biotransformation of bicyclo (3. 2. 0) hept-2-en-6-one by the NADH-dependent Baeyer-Villiger monooxygenase from camphorgrownPseudomonas putida NCIMB 10007 has been shown to yield a chiral lactone not accessible by curently-used biocatalysts. The biotransformation can be conductedin vitro using two alternative coupled enzyme systems (alcohol dehydrogenase and monooxygenase: formate dehydrogenase and monooxygenase) within situ recycling of NAD⁺/NADH.     

Regiospecific biotransformation of substituted norbornanones by microorganisms

Summary The regiospecific biotransformation of (±) 5-acetoxy-7-fluoronorbornan-2-one into the equivalent bridgehead lactone of use as a source of substituted cyclopentane synthons containing four successive chiral centres has been demonstrated using washed-cell suspensions of cyclohexanol-grownAcinetobacter sp NCIB 9871. Conditions to optimise production of such 2-oxabicyclooctanones (substrate concentration<25mM, pH 7.35, 30°C) have been characterised.     

Microbial metabolism of alkylbenzene sulphonates the oxidation of key aromatic compounds by a Bacillus

A Bacillus species originally elected for growth at the expense of alkylbenzene sulphonate detergents was found to metabolise a wide range of aromatic compounds. p-Hydroxybenzoate (PHB) was initially hydroxylated to protocatechuate (PCA) i.e. 3,4-dihydroxybenzoate, which was oxidatively cleaved to succinate and acetyl-CoA by a classical ortho cleavage pathway initiated by a substrate-specific 3, 4-oxygenase: no evidence of an alternative meta cleavage pathway was detected. Several key enzymes of this ortho cleavage pathway were induced by growth of the Bacillus on either PHB or PCA. Both PHB and PCA were able to act as sole source of carbon for energy and overall growth of the microorganism.In strict contrast, the higher homologue p-hydroxyphenylacetate (PHPA), after initial hydroxylation to 3, 4-dihydroxyphenylacetate (DHPA), was oxidatively cleaved to 4-carboxymethyl-2-hydroxymuconic semialdehyde (CMHMS) by a meta cleavage catalysed by a substrate-specific 2, 3-oxygenase: no evidence of an alternative ortho cleavage was detected. Several lines of evidence suggested that CMHMS was not further metabolised by the Bacillus and accumulated in the growth medium. Both PHPA and DHPA were unable to act as sole source of carbon for energy and overall growth.The implication of the occurrence in a single bacterium of two separate oxidative pathways catalysing the cleavage of different aromatic nuclei have been discussed.     

Plasmid Specificity of The Origin of Transfer of Sex Factor F

The ability of F-like plasmids to promote transfer from the F origin of transfer was determined. Chromosome transfer was measured from plasmid derivatives of RecA(-) Hfr deletion strains which had lost all the F transfer genes but which in some cases retained, and in others had also lost, the origin sequence. ColV2 and ColVBtrp could initiate transfer from the F origin, but R100-1, R1-19, and R538-1 drd could not. These results can be correlated with the plasmid specificity of the traI components of the different plasmid transfer systems, supporting the hypothesis that the origin of transfer is the site of action of the traI product. Most F-like plasmids, including R1-19 and R538-1 drd, could transfer ColE1, consistent with previous findings that the (plasmid-specific) traI product is not necessary for ColE1 transfer by Flac; ColE1 transfer may be initiated by a ColE1-or host-determined product. R100-1 and R136fin(-) could not transfer ColE1 efficiently, apparently because of differences residing in their pilus-forming genes.     

The phosphorylation and subsequent metabolism of 1-aminopropan-2-ol

Rat liver mitochondria contain an apparently substrate-specific 1-aminopropan-2-ol kinase activity. Indirect evidence also indicates the presence of a phosphoryl-1-aminopropan-2-ol cytidylyl transferase activity. A possible role for these two enzymes in the incorporation of 1-aminopropan-2-ol as a phospholipid base is considered in the light of this and other data.     

L-Threonine acetaldehyde-lyase in a strain of Bacillus subtilis

1.

1. l-Threonine aldolase (l-threonine acetaldehyde-lyase, EC 4.1.2.5) has been identified in threonine-grown cell-free extracts of the aerobic microorganism Bacillus subtilis.