Function and Location of a "Germination Enzyme" in Spores of Bacillus Cereus

Gould, G. W.; Hitchins, Anthony D.; King, William L.

doi:10.1099/00221287-44-2-293

Cited by 35 publications

(26 citation statements)

References 16 publications

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“…Since then, the spore-lytic enzymes of Bacillus cereus have been isolated and extensively studied by Strange & Dark (1957), Gould et al (1966), Warth (1972) and Brown et al (1975Brown et al ( , 1977Brown et al ( , 1978. In most cases, this lytic system was found to hydrolyse the peptidoglycan of the spore cortex, resulting in germination-like changes in the spore.…”

Section: Introductionmentioning

confidence: 99%

Extraction of Spore-lytic Enzyme from Clostridium perfringens Spores

Gombas

Labbé

1981

Microbiology

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Various chemical reagents known to extract spore coat protein were used to extract spore-lytic enzyme (SLE) from intact and germinated spores of Clostridium perfringens. Of the reagents tested, 7.2 M-urea plus 10% (v/v) mercaptoethanol, pH 2.85, solubilized the most SLE activity per mg spores. The quantity of SLE extracted was dependent on the initial pH of the reagent, with a maximum between pH 2.7 and 3.0. Germinated spores yielded more SLE than non-germinated spores upon urea/mercaptoethanol extraction. SLE release during spore germination probably utilizes a trigger mechanism not satisfied by germination alone. Significant amounts of SLE were released during germination when spores were suspended in potassium chloride or a complex germinant mixture containing brain-heart infusion, yeast extract and chloramphenicol, but not during germination with sodium nitrite, which non-enzymically lysed the cortical peptidoglycan. Greater solubilization of SLE activity was obtained by urea/mercaptoethanol extraction of spores germinated with nitrite than of spores germinated with either potassium chloride or the complex germinant.

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Section: Introductionmentioning

confidence: 99%

Extraction of Spore-lytic Enzyme from Clostridium perfringens Spores

Gombas

Labbé

1981

Microbiology

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“…The enzyme was assayed by its ability to cause a decrease in the extinction of suspensions of spores which had been sensitized by incubation in thioglycollic (mercaptoacetic) acid (25 %, v/v) plus urea (6 M) at 70" for 30 min. (Gould et al 1966). The enzyme reaction was carried out in sodium phosphate buffer (100 mM, pH 8.0) at 37"; the initial extinction read at 580 nm.…”

Section: Inhibition Of Spore Germination 303mentioning

confidence: 99%

“…to 20 mg. dry wt/ml.) which had been disrupted by shaking with glass beads as described by Gould, Hitchins & King (1966). The enzyme was assayed by its ability to cause a decrease in the extinction of suspensions of spores which had been sensitized by incubation in thioglycollic (mercaptoacetic) acid (25 %, v/v) plus urea (6 M) at 70" for 30 min.…”

Section: Inhibition Of Spore Germination 303mentioning

confidence: 99%

Mechanism of the Inhibition of Germination of Bacterial Spores by -radiation in the Presence of Iodoacetamide and Iodate

Gould¹

1970

Journal of General Microbiology

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SUMMARYWhereas y-radiation alone either did not affect or stimulated spore germination, spores which had been irradiated in the presence of iodoacetamide (IAM) or potassium iodate were inhibited from germinating in germinants like L-alanine, inosine or yeast glucose broth. Activity of a lytic enzyme which may be involved in germination was mostly lost in spores irradiated in TAM, and a phosphomonoesterase was about 60 % inhibited. Spore alanine racemase was partly inactivated by y-radiation alone but, with spore protease, survived irradiation in IAM without much further loss of activity. Although spores made non-germinable by y-radiation plus IAM were nonviable as measured by colony counts, viability could be partly restored by chemical treatments known to by-pass the normal germination reactions. It was concluded that spores were inactivated by y-radiation in the presence of the potentiators through inactivation of enzyme(s) essential in the degradative reactions of germination. The enzyme inactivation was caused by iodinecontaining free radicals rather than directly by the y-radiation.

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“…Although the mechanism initiating these changes is not known, Strange & Dark (1957) and Gould, Hitchins & King (1966) suggested that they result more or less directly from depolymerization of peptidoglycan in the spore cortex, catalysed by a lytic enzyme which can be extracted from spores of some species and which can be shown to cause germination-like changes in chemically sensitized spores (Gould & King, 1969). If this is so then the excretion of peptidoglycan fragments would be expected to be one of the earliest determinable events during germination.…”

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Sequence of Events during Rapid Germination of Spores of Bacillus cereus

Dring

Gould

1971

Journal of General Microbiology

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Levinson Hyatt (1966) showed that the measurable events collectively recognized as spore germination, and previously thought to take place concurrently, occurred in Bacillus megaterium QM B I~~I in the following sequence: loss of resistance to heat and mercuric chloride; release of dipicolinic acid (DPA) ; onset of stainability; darkening of individual spores under phase contrast optics and fall in extinction of spore suspensions. Although the mechanism initiating these changes is not known, Strange & Dark (1957) and Gould, Hitchins & King (1966) suggested that they result more or less directly from depolymerization of peptidoglycan in the spore cortex, catalysed by a lytic enzyme which can be extracted from spores of some species and which can be shown to cause germination-like changes in chemically sensitized spores (Gould & King, 1969). If this is so then the excretion of peptidoglycan fragments would be expected to be one of the earliest determinable events during germination. However, if hydrolysis of peptidoglycan only commences following germination, then excretion of fragments should occur late in the sequence of events. The experiments described here were designed to resolve these possibilities.Organism. Spores of Bacillus cereus T were grown in G medium (Stewart & Halvorson, I 953). Peptidoglycan in spores was labelled with generally tritiated a,6-diaminopimelic acid (rH] DAP ; Radiochemical Centre, Amersham, Buckinghamshire) by adding [3H] DAP (40 pm. ; specific activity, 9 mCi/mmole) and cold lysine ( I mM) to cultures in the 'granular' stage of growth, just prior to the commencement of sporulation. The presence of excess lysine prevented decarboxylation of the [3H]DAP (Vinter, 1965). Spores were cleaned by centrifuging six times in ice-cold HCI (0.03~) as recommended by Murrell & Warth (1969, twice in ice-cold distilled water, and stored frozen.Germination. Spores were activated by heating in water at 70' for 30 min., washed once in water, then added (about Io8/ml.) to the following solution at 30°, to initiate germination: tris (hydroxymethyl amino methane) + HCl buffer (100 mM, pH 8.0), containing L-alanine (5 mM) and inosine (5 mM). Samples were taken at intervals, and the germination process was rapidly halted either by separating spores from the supernatant fraction in about 15 sec. by membrane filtration using filter membranes (0.45 pm. mean pore size) in Swinney filter holders on syringe barrels (Millipore Corp., Bedford, Massachusetts, U.S.A.), or by adding formaldehyde (20 % v/v) and quickly centrifuging.AnaZyses. Pellet and supernatant samples were analysed for calcium using an Atomic Absorption Spectrophotometer

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Function and Location of a "Germination Enzyme" in Spores of Bacillus Cereus

Cited by 35 publications

References 16 publications

Extraction of Spore-lytic Enzyme from Clostridium perfringens Spores

Extraction of Spore-lytic Enzyme from Clostridium perfringens Spores

Mechanism of the Inhibition of Germination of Bacterial Spores by -radiation in the Presence of Iodoacetamide and Iodate

Sequence of Events during Rapid Germination of Spores of Bacillus cereus

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