Mutagenesis byN-methyl-N-nitroso-N-nitroguanidine in synchronized cultures ofMycobacterium phlei

Conditions of maximum induction of back mutations byN-methyl-N-nitroso-N′-nitroguanidine (“nitrosoguanidine”) were studied in auxotrophic mutants ofMycobacterium phlei. In asynchronous cultures the effects of pH, buffer molarity and concentration and exposure time to nitrosoguanidine were studied. It was shown that between 6 and 10, pH does not affect the induction of back mutations but that with increasing pH up to 9 the lethal effect of nitrosoguanidine on cells is increased. Protracted treatment with nitrosoguanidine or buffer molarity did not affect the induction of back mutations. It was found with several strains ofMycobacterium phlei that it is most efficient to treat a culture with 0.5 mg or 1 mg nitrosoguanidine/ml for 20 min at pH 6. On the basis of these findings a method of induction of back mutations by nitrosoguanidine was developed for populations with synchronous cell division.     

Electronmicroscopic comparison of the acid-fast and non-acid-fast strain ofMycobacterium phlei

Ultrastructure of the acid-fast PA strain ofMycobacterium phlei and its non-acid-fast PN mutant was studied in an electron microscope. Results of electronmicroscopic studies were supplemented with observation under an optical microscope, cultivation and chemical analysis of the wall mucopeptide. The effect of lysozyme and glycine on ultrastructure of cells of these strains was also followed. Electron microscopy revealed main differences in thickness and structure of cell walls, in intracellular membraneous system and in shape of rods of the studied strains.     

Esterases in mycobacteria

It was found that a submerged culture ofMycobacterium phlei degrades simple esters (ethylacetate and ethylbutyrate) as well as synthetic lipids (triacetine and tributyrine). The effect of pH on the rate of degradation of tributyrine was investigated and the maximum activity of esterases found within a wide range of pH. The activity of esterases was followed during growth of a submerged culture ofMycobacterium phlei. Esterases were not released into the cultivation medium during growth or even during the early stationary phase. Only a low steady activity of esterases could be demonstrated in a filtrate of the cultivation liquid. The total activity of esterases reached its maximum after a 6–11 day incubation. The specific activity of esterases reached a maximum on the 6th day of incubation; its value decreased to about one half and did not change substantially on prolonged incubation. Changes in the specific activity of esterases were found to be time-related with changes of pH and a decrease of the specific activity was associated with a release of macromolecular compounds into the incubation medium. Esterases as well as other macromolecular compounds were isolated from the filtrate of the cultivation medium ofMycobacterium phlei. The isolated preparation contained 60–72% total activity of esterases present in the filtrate of the cultivation liquid.     

The attempt to transform streptomycin-resistance inMycobacterium phlei

Acid-fast and non-acid-fast strains ofMycobacterium phlei were used for the induction of streptomycin-resistance by isolated DNA. Biological activity of a transforming principle isolated from the cells homogenized in a Hughes press was confirmed. No reproducible positive results were obtained under given experimental conditions. Possible reasons for the lack of positive results are discussed.     

The induction of pigmentation change in a non-acid-fast strain ofMycobacterium phlei by ultraviolet radiation

Five scotochromogenic mutants and 11 achromogenic mutants were induced by UV irradiation of the non-acid-fast photochromogenic PN strain ofMycobacterium phlei. Spontaneous scotochromogenic and achromogenic mutants were not obtained. Colonies of the scotochromogenic mutants are orange, except for one mutant which is ochre. Three mutants are resistant to STM. Out of 11 achromogenic mutants 3 were induced by UV treatment of the original photochromogenic strain, 8 were prepared from the scotochromogenic mutant. No significant differences in the sensitivity to UV rays were found among the scotochromogenic mutant, achromogenic mutant and the photochromogenic PN strain ofMycobacterium phlei under the given experimental conditions. Scotochromogenic mutants and most achromogenic mutants are stable and suitable for further genetic investigation. Pigmentation changes can be used as genetic marker in mutation studies.     

Adsorption of a hydrophobic bacterium onto hematite: Implications in the froth flotation of the mineral

Summary The present study reports on the relationship between adsorption ofMycobacterium phlei onto hematite and flotation of the mineral. From light and scanning electron microscopy, contact angle and electrophoretic mobility observations it was found thatM. phlei is more negatively charged than hematite, that it readily accumulates onto the mineral and that it functions as a flotation collector for the mineral with optimum flotation taking place at about pH 2.5.     

The effect of daylight on the biosynthesis of carotenoids by non-acid-fast strains ofMycobacterium phlei

The changes of the cell pigment composition of two non-acid-fast forms ofMycobacterium phlei (PN, PNR), caused by exposure to daylight, were studied. Though during cultivation in the dark carotenes were mostly produced, cultures exposed to the light mostly formed their oxygen-containing derivatives. Xanthins derived from lycopene, the main carotenoid formed by the PNR strain, were obtained from the mycelium of this mycobacterium after it was exposed to daylight. The exposure of the PN culture to daylight results in the formation of xanthins and in the stimulation of lycopene synthesis.     

Esterases in mycobacteria

Esterases ofMycobacterium phlei (acetic ester acetyl hydrolase E.C.3.1.6 and carboxylic esterhydrolase E.C.3.1.1.1.) obtained after separation on Sephadex G-100 can be temporarily, for a short time interval, activated by adding calcium ions. The activation of esterases isolated from cells was non-repeteable, whereas the temporary activation of esterases from the culture filtrate could be repeated by increasing concentrations of calcium ions. However, the value of activation gradually decreased. Similarly with calcium ions strontium ions were also effective, however, higher concentrations were required and the activation was non-repeatable. Magnesium ions were practically without any effect. Possible mechanisms of the temporary activation of esterases ofMycobacterium phlei are discussed.     

The comparison of a new mutant ofMycobacterium phlei with some strains of rapidly growing mycobacteria

A red, scotochromogenic mutant of the non-acid-fast strain ofMycobacterium phlei was obtained. Mutual relationship between this mutant and rapidly growing mycobacteria was studied using complex morphological, cultivation, biochemical and serological analyses as well as determination of the base composition in DNA. Taxonomical aspects of individual analyses are discussed.     

Dynamics of growth of atypical mycobacteria in different liquid cultivation media

The dynamics of growth ofMycobacterium smegmatis, M. fortuitum andM. phlei in liquid media used also for cultivation of typical mycobacteria (Sauton, Youmans, Kirchner, Šula) was compared with that in Davis and Merrill media. In the Merrill medium glucose (as the only organic component) was replaced with another carbon source and the effect of this modification was investigated. The results obtained show that the Merrill medium, its modification in particular, is suitable for cultivation ofM. smegmatis andM. fortuitum. 2-Oxoglutarate and succinate are important as the sole carbon sources in the case ofM. fortuitum andM. phlei respectively.     

Possibilities of the conjugation process in mycobacteria

Results obtained when studying conjugation in mycobacteria by means of different methods are summarized. The method of conjugation on surface of a solid complete medium was tested with different auxotrophic mutants of different strains ofMycobacterium smegmatis. It was not possible to obtain positive results even by means of the above method. This was probably due to unsuitability of the chosen strains ofMycobacterium smegmatis. Preparation of the donor strain by transfer of the F factor fromEscherichia coli F’ORF 1ade ⁺ lac⁺ pro⁺ toMycobacterium phlei PA adeStm ^r by means of sexduction is described. Frequency of the phenotype PAade ⁺ Stm^r increased in the average by two and a half orders of magnitude with respect to the control, however, a further transfer from cultures of the cellsade ⁺ Stm^r to cells ade could not be demonstrated. Experiments aimed at transferring the R factor from strainsEscherichia coli K-12 toMycobacterium phlei were unsuccessful.     

Composition of intracellular soluble proteins inMycobacterium “rubrum” and its mutants

The composition of intracellular soluble proteins in a parental strain ofMycobacterium “rubrum” and its mutants was studied by polyacrylamide gel gradient electrophoresis. The composition of the protein fractions of the parental and the mutant strains was similar, they differed in one protein only. The presence of a 60 kDa protein should be stressed since its increased amount may be connected with a different intensity of the production of pigments in the strains studied. Translated by Č. Novotny     

The production of aflatoxin M on various substrates

Summary The ability of 44 strains ofA. flavus and 6 strains ofA. parasiticus to produce aflatoxin M on various substrates was examined. It was found that these strains produced aflatoxin M only with larger quantities of aflatoxin B. The presence of several other minor metabolites in culture extracts is described. The highest yield of aflatoxin M was produced by a strain ofA. flavus grown on maize meal.     

Growth inhibition of bacteria by tributylgermanium acetate and its reversal by blood constituents

Growth inhibition ofMycobacterium phlei by tributylgermanium acetate can be reversed by addition of large amounts of blood or blood serum to the nutrient medium; the blood erythrocyte fraction is inactive.On the other hand growth inhibition of the lactic acid bacteriaStreptococcus lactis andLeuconostoc mesenteroides can be counteracted by traces of blood or its crythrocyte fraction, by hemin and by catalase. Blood serum even in large amounts is ineffective.Whereas tributylgermanium acetate is highly active against most lactic acid bacteria studied, the antagonistic action of blood or hemin is found only with the species named. The possible mechanism of this antagonism is discussed.     

Esterases in mycobacteria

A procedure for the isolation of a crude enzyme preparation of esterases fromMycobacterium phlei was worked out. The procedure consists in breaking cells in 1% KCl by ultrasonication, ultracentrifugation at 40,000 r.p.m. and isolation of acetone and ether dried enzyme preparation. Specific activity increased 2.8-fold after completion of the procedure. Esterases fromMycobacterium phlei were separated on Sephadex of G series to two enzymes with different substrate specificity. The first enzyme, acetic ester acetyl-hydrolase (E.C. 3.1.1.6) was found to be relatively specific for ethylacetate, the second, carboxylic ester hydrolase (E.C. 3.1.1.1) for ethylbutyrate and tributyrine. Preparations of both enzymes were made from the crude extracts of cells and from a mixture of macromolecular compounds isolated from the culture filtrate ofMycobacterium phlei.     

Turnover of lipids in Mycobacterium smegmatis CDC 46 and Mycobacterium phlei ATCC 354

The rates of breakdown and renewal of individual lipids in cultures of Mycobacterium smegmatis CDC 46 and Mycobacterium phlei ATCC 354 were investigated by means of a pulse labelling technique using palmitate-1-¹⁴C. The results indicated that in growing cultures of both strains phospholipids were broken down, and cardiolipin had a very rapid turnover. In chase experiments, almost 45% and 40% of the radioactivity of this component were lost respectively from M. smegmatis and M. phlei during one generation time of the cell. The other two major components, phosphatidyl ethanolamine and phosphatidylinositol mannosides showed relatively low turnover. The loss of radioactivity from phosphatidylinositol mannosides was greater in M. phlei than in M. smegmatis but the loss of radioactivity from phosphatidyl ethanolamine was higher in M. smegmatis. The pattern of loss of radioactivity from lipids was almost the same in both strains, the difference being only in the extent of loss. The differences in the cellular localization of the phospholipids indicate their different roles within the cell. Results obtained with the glyceride fraction indicated a very rapid turnover of triglycerides in both strains.Abbreviations CL Cardiolipin - PE Phosphatidyl ethanolamine - PIMx phosphatidylinositol mannosides - PIM₂A phosphatidylinositol dimannoside tetra acylated - PIM₂B phosphatidylinositol dimannoside tri acylated - PIM₅ phosphatidylinositol pentamannoside tetra acylated     

Cytochemical and biological properties ofMycobacterium bovis BCG

It was the aim of the present communication to find a simple test for a reliable discrimination ofMycobacterium bovis BCG fromMycobacterium tuberculosis. A total of 26 BCG strains, out of them 10 Czechoslovak strains (2 lyophilized cultures of BCG of different batch, 6 strains isolated from abscesses of children after BCG-vaccination and 2 strains from fatal cases after BCG-vaccination) and 16 strains obtained from foreign laboratories, were used. Of the tested characteristics a combination of 3 tests, sensitivity to 1 μg of 2-thiophene carbonylhydrazide (TCH), activity of 3 acylamidases (urease, nicotinamidase and pyrazinamidase) and a quantitative nitrate test, was found to be most advantageous. The Czechoslovak strains ofMycobacterium bovis BCG were fully sensitive to TCH, of the 3 acylamidases mentioned above only urease was positive and nitrate was reduced only little or not at all. On the other hand, strains ofMycobacterium tuberculosis were always resistant to TCH, had positive urease, nicotinamidase and pyrazinamidase and reduced nitrate very intensively.     

The replication map of the chromosome ofMycobacterium phlei

It was the aim of the present work to construct the replication map of the chromosome ofMycobacterium phlei. The method of mutagenesis of the replication point by N-methyl-N-nitroso-N’-nitroguanidine in synchronously dividing populations and the method of analysis of gene frequency were applied. The order of replication of 19 genes on the chromosome was determined by means of induction of back mutations and forward mutations in auxotrophic mutants PAleu and PAmet and in double auxotrophic mutants with methionine as a reference marker.     

Mapping of the chromosome ofMycobacterium phlei by means of mutagenesis of the replication point

The aim of the present work was to construct a replication map of the chromosome ofMycobacterium phlei. The method of mutagenesis of the replication point by means of nitrosoguanidine was applied to synchronously multiplying populations. Back mutations and forward mutations were induced m auxotrophic mutants PAmet and PAleu as well as in double auxotrophic mutants with methlomne as the reference marker and the following order of replication of eleven genes on the chromosome was thus established:leu-Eth, Res-Stm, Oyk-pur-met, arg, Cyk-Bac-inl     

The induction of mutants in a non-acid-fast strain ofMycobacterium phlei with nitrous acid

The inactivation and mutagenic effets of nitrous acid on a non-acid-fast strain ofMycobacterium phlei were studied. It was found that 0.017m NaNO₂ at pH 4.4 may be used for the induction of auxotrophic mutants, scotochromogenic and achromogenic mutants and STM-resistant mutants. Three doubly auxotrophic mutants, three mutants requiring amino acids and three mutants depending on vitamins were obtained. One mutant was not classified. Eighteen scotochromogenic mutants were isolated, seventeen of them were orange. Only ten achromogenic mutants were isolated. Twelve scotochromogenic and eight achromogenic mutants could be used in further genetic studies as they did not revert spontaneously to photochromogeny. Six auxotrophic mutants could be used due to their low frequency of spontaneous reversions. The frequency of STM-resistant mutants increased on an average seven-fold after the mutagenic treatment as compared with the spontaneous frequency.