Effects of light on basidiocarp maturation in Coprinus macrorhizus

The effect of white light on basidiocarp maturation in Coprinusmacrorhizus was examined. The results obtained showed that basidiocarpmaturation was separable into five successive phases in regardto photosensitivity: phase 1 in which light triggered maturation;phase 2 in which light delayed maturation; phase 3 in whichlight stopped maturation; phase 4 in which light acceleratedmaturation; and phase 5 in which light had no effect upon theprogress of maturation. The relation between the light effect and the events duringspore formation including nuclear fusion, meiosis and sterigmaformation was examined with the following results: the lightof phase 1 initiated nuclear fusion; the light given in phase2 delayed the initiation of nuclear fusion and the later progressup to prophase 1; without the darkness of phase 3, meiosis neverproceeded beyond prophase 1; and the light given in phase 4accelerated the progress from the initiation of nuclear fusionto prophase 1. (Received August 15, 1977; )     

Stipe elongation during basidiocarp maturation in Coprinus macrorhizus: Mechanical properties of stipe cell wall

Stipe elongation during basidiocarp maturation in the wild-type,#5026+5132, and the elongationless mutant, NG0398, of Coprinusmacrorhizus was studied, and the following results were obtained.

1. In the wild-type the middle zone of the stipe elongated 8.4times in 15 hr during maturation, while in the mutant it elongatedoaiy 2.2 times.
2. Component cells of the stipe elongated inparallel with thestipe elongation in both the wild-type andthe mutant. The widthof stipe cells was almost constant duringelongation in thewild-type, while it increased 2 times in themutant. Cell volumeincreased ca. 8 times in both stocks.
3. Theosmotic value of stipe cells was almost constant (0.45–0.50M) throughout elongation of both the wild-type and the elongationlessstipes.
4. Mechanical properties of the cell wall were examinedby measuringshrinkage, extensibility and minimum stress-relaxationtime(To) of the stipe during maturation. These parameters weredirectlyproportional to the elongation rate to follow.
5. Whenthe wild-type stipes were incubated in various concentrationsof mannitol solution and then in plain buffer solution, theextensibility of the stipe after the incubation in mannitolsolutions changed proportionally with the stipe length afterthe mannitol treatment, and To with the elongation capacityin plain buffer solution.

(Received March 3, 1977; )     

Stipe elongation during basidiocarp maturation in Coprinus macrorhizus: Changes in polysaccharide composition of stipe cell wall during elongation

Changes in polysaccharide composition of stipe cell wall werefollowed during basidiocarp maturation in wild-type stock (#5026+5132)and the elongationless mutant (NG0398) of Coprinus macrorhizus,and then the correlation between contents of the respectivepolysaccharide components and mechanical properties of stipecell wall was examined. Polysaccharides of stipe cell wall werefractionated into five fractions, i.e., fraction I, II, IIIand IV polysaccharides and chitin. In the wild type, the content(% of cell wall) of fraction I decreased during an early phaseof maturation and then remained unchanged. Fraction III andIV contents increased once and then decreased. Fraction II andchitin contents remained almost constant during an early phaseof maturation and then increased as stipe elongation proceeded.On the basis of the correlation between the polysaccharide contentsand mechanical properties, it was suggested that the higherproportion of fraction III and/or fraction IV content(s) stimulatedstipe elongation, and that the higher proportion of fractionII and/or chitin content(s) resulted in lower rate of elongation.In the mutant, changes in the contents of the respective polysaccharideswere basically similar to those in the wild type. Thus, differencesin the rate of stipe elongation and mechanical properties betweenthe wild type and the mutant could not be simply explained interms of polysaccharide content. (Received June 27, 1977; )     

Photo-induced karyogamy in a Basidiomycete, Coprinus macrorhizus

In Coprinus macrorhizus, the fruit-body matured when two 2-hrlight periods were given separately after the formation of theprimordium. The karyogamy may be triggered by the exposure tothe second light, because fusion of two nuclei in the basidiumwas always observed 12 hr after exposure to the second light,irrespective of the time when given. (Received August 15, 1973; )     

Purification and Identification of the Fruiting-Inducing Substances in Coprinus macrorhizus

Substances which are effective in inducing fruiting bodies in monokaryotic mycelia of the fis(+) strain of Coprinus macrorhizus were purified and characterized. The active components of fruiting-inducing substances were identified as adenosine-3'-monophosphate, adenosine 3',5'-cyclic monophosphate (cyclic AMP), and a protein which is bound with the cyclic AMP. Cyclic AMP was synthesized from adenine within mycelia of the mutant strains which form monokaryotic fruiting bodies without the addition of fruiting-inducing substances, but not in those of the strains which do not form monokaryotic fruiting bodies. The proteins which bind with cyclic AMP were detected in crude extracts of mycelia of those strains which form monokaryotic fruiting bodies and of the dikaryon, but not in those of the strains which do not form monokaryotic fruiting bodies.     

Effect of cyclic AMP on glycogen phosphorylase in Coprinus macrorhizus.

Glycogen phosphorylase (1,4-alpha-D-glucan:orthophosphate alpha-glucosyltransfase, EC 2.4.1.1) activity was found in mycelial extracts of Coprinus macrorhizus concurrently with decrease of glycogen content in mycelial cells. Incubation of the enzyme sample with cyclic AMP and ATP leads to a 3-fold activation of the glucogen phosphorylase activity. Activation of the enzyme partially purified through Sepharose 6B required a cellular fraction containing cyclic AMP-dependent protein kinase.     

Effects of light on fruit-body formation in a basidiomycete, Coprinus macrorhizus

A basidiomycete, Coprinus macrorhizus produced only vegetativemycelia, when cultured under continuous darkness. Under continuouswhite light, visible tiny primordia formed on the 6th day afterinoculation, followed by normal development to fruit-bodies.Spores disseminated on the 11th day. However, when cultureswhere transferred to continuous darkness after the formationof primordia, rudimentary pilei with slender stalks formed.Abundant hairy hyphae were produced along the entire surfaceof the slender stalks. Thus, light was required-for both theinitiation and development of the fungal fruit-body. A fairy ring of primordia formed along the narrow region ofmycelia formed just prior to the exposure to light, provideda colony was pre-grown for more than 4 days in the dark, thenexposed to light for 24 hr or longer. Exposure to light for at least 48 hr during the period between24th and 96th hr after primordium initiation was required fornormal maturation of the fruit-body. This 48 hr light periodneeded for maturation of the fruit-body could be substitutedby two, 2 hr light periods given at the beginning and the endof the 48 hr period. We have tentatively concluded that lightis required at two definite stages for fruit-body developmentafter formation of the primordium. Effective wavelengths for both the initiation and developmentof fruit-bodies were in the near ultraviolet and blue regions. (Received July 24, 1972; )     

Basidiospore formation in monokaryotic fruiting bodies of a mutant strain of Coprinus macrorhizus

The process of basidiospore formation in a mutant strain Fis^c of Coprinus macrorhizus, a heterothallic species of Basidiomycete, which forms monokaryotic fruiting bodies was examined. A single nucleus in a young basidium divided mitotically and two daughter nuclei were fused subsequently. The fused nucleus then divided meiotically forming four basidiospores on a basidium. The typical chromosome behaviours in the first meiotic prophase were observed. Synaptonemal complexes were observed in a basidium at the first meiotic prophase. A continuous illumination of fruiting bodies was effective to arrest meiosis in monokaryotic fruiting bodies at the particular stage of meiotic division.     

Adenosine 3',5'-monophosphate-receptor protein and protein kinase in Coprinus macrorhizus

A single cAMP-receptor protein could be detected in mycelial extracts of Coprinun macrorhizus by using the photoaffinity cAMP-analogue, 8-N3-cAMP. The protein which specifically bound 32P-labeled 8-N3-cAMP had an apparent molecular weight of 46,000 as determined by an SDS-polyacrylamide gel electrophoresis system. The 46,000-dalton protein was characterized by the dissociation constant for [32P]-8-N3-cAMP, and by the nucleotide specific inhibition of [32P]-8-N3-cAMP binding. The 46,000-dalton protein was co-chromatographed on a DEAE-cellulose column with cAMP-dependent protein kinase. The levels of [32P]-8-N3-cAMP-binding and protein kinase activities in mycelial extracts of strains used was always in parallel. The result indicated that the 46,000-dalton protein may be a regulatory subunit of protein kinase with the capacity to bind cAMP. cAMP-dependent protein kinase of this fungus was immunologically different from those of higher animals.     

Sequential production of enzymes and basidiospore formation in fruiting bodies of Coprinus macrorhizus

The production of NADP-dependent glutamate dehydrogenase was initiated at the stage of first meiotic prophase in pileus cells but not in stipe cells of dikaryotic and monokaryotic fruiting bodies in Coprinus macrorhizus. The production of chitinase and glucanases assayed with laminarin and lichenan was observed after the completion of meiosis only in pileus cells. The light conditions that were effective for the delay or inhibition of cellular events in the pileus cells were also effective for the delay or inhibition of enzyme production. But all sporeless mutants tested, which were defective at the various stages of basidiospore formation, produced the normal levels of these enzymes. The results indicate that the sequential production of enzymes and cellular events leading to basidiospore formation in pileus cells are independent from each other.Abbreviation GDH_NADP NADP-dependent glutamate dehydrogenase     

Relationship between deficiency of phosphoglucose isomerase in Coprinus macrorhizus and fruiting body formation.

A mutant (pgi) of Coprinus macrorhizus deficient in phosphoglucose isomerase did not grow on fructose and grew poorly on glucose. The pgi mutation inhibited the formation of monokaryotic and dikaryotic fruiting bodies.     

Timing of DNA replication during the meiotic process in monokaryotic basidiocarps of Coprinus macrorhizus

By applying the method of fluorescent microscopy to propidium iodide stained cells, change in the relative amount of DNA in a basidium was examined during the meiotic process in Coprinus macrorhizus. In the monokaryotic basidiocarp of the mutant strain Fis^c, mitotic DNA replication was first induced soon after a 3h-illumination period on the 10th day of culture, and subsequently meiotic DNA replication occurred after karyogamy.     

An investigation of the effects of light on basidiocarp formation of Coprinus domesticus

Coprinus domesticus, grown on a synthetic agar medium, failed to produce primordia and basidiocarps unless exposed to light. Lightdark cycles are not required for maturation of basidiocarps. Short exposure to white light induced primordia, but a longer exposure was necessary for primordia to develop into basidiocarps. The length of exposure to light was related inversely to the length the stipe finally attained. Young basidiocarps were phototropic, growing towards the light. The mycelium of cultures were dark brown following exposure to white and blue light, but the mycelium was light yellow in cultures grown in darkness. The blue end of the visible spectrum at intensities ranging from 1.5–3 × 10⁴ ergs/cm²/sec induced mature basidiocarps, whereas green, red and far red failed to induce basidiocarps and primordia.Department of Biology contribution no. 90     

Intraspecific heterokaryon and fruit body formation in Coprinus macrorhizus by protoplast fusion of auxotrophic mutants

Summary Fusion of protoplasts of Coprinus macrorhizus mutants with different amino acid requirements resulted in the production of prototrophic clones at frequencies of 1–4% of the protoplasts surviving the fusion treatment. The frequencies were at least 200 times higher than those of the appearance of revertants. Few prototrophic colonies appeared also when the mutant protoplasts were individually subjected to fusion treatment, or when they were mixedly cultured without fusion treatment. It was thus concluded that intraspecific heterokaryons were formed by protoplast fusion.The auxotrophic mutants did not form fruit bodies when cultured singly or mixedly with each other. In contrast, the heterokaryons produced by protoplast fusion between the mutants of compatible mating types developed into fruit bodies with intermediate morphology of those of the strains from which the mutants were derived. Heterokaryons were also formed by fusion of mutant protoplasts with identical mating genotype, but they failed to form fruit bodies.Abbreviations PEG polyethyleneglycol - HEPES N-2-hydroxyethylpiperazine-N-2-ethane sulfonic acid     

An efficient method for the isolation of mycelial protoplasts from Coprinus macrorhizus and other basidiomycetes

Summary A mixture of commercially available chitinase and cellulase released mycelial protoplasts of Coprinus macrorhizus in yields exceeding 10⁸/ml plasts from C. macrorhizus Fis^C regenerated hyphae and developed into normal fruiting bodies at frequencies of 20%–50%. The same method also released good yields of protoplasts from several other edible mushroom species.     

Control of adenosine 3',5'-monophosphate level and protein phosphorylation by depolarizing agents in Coprinus macrorhizus

The treatment of mycelial cells with membrane-active antibiotics, uncouplers of oxidative phosphorylation and KCl leads to a transient increase in adenosine 3',-5'-monophosphate (cyclic AMP) levels in Coprinus macrorhizus. The maximal values and duration of increase in the cyclic AMP level depended on the kind and amount of these drugs. The treatment with these drugs simultaneously resulted in a rapid increase in the phosphorylation of three cellular proteins. The levels and time course of phosphorylation of these proteins were paralleled with the increase of cyclic AMP level in response to the drugs used. Thus, the treatment of these drugs causes the transient increase of cyclic AMP level and cyclic AMP stimulates the phosphorylation of particular proteins by activating protein kinases.     

Purification and characterization of an ubiquitin-immuno-reactive protein localized in the cap of young basidiocarp in the basidiomycete Coprinus cinereus.

The ubiquitin-immuno-reactive protein with a molecular weight of 27,800 daltons, which is mainly present in the cap of young basidiocarp, was purified from the basidiomycete Coprinus cinereus. The molecular weight of the native protein was approximately 55,000 as determined by gel filtration chromatography. The isoelectric point of the protein was 4.4. The amino-terminal sequence of the protein was also determined.