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1.
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; )  相似文献   

2.
  1. 1. Analyses of cytochrome types in intact cells of aerobically-and anaerobically-grownPs. denitrificans indicated a higherratio of cytochrome c to cytochrome b in the former than inthe latter.
  2. 2. Anaerobically-grown cells contained about twotimes as muchcryptocytochrome c as did aerobically-grown cells.
  3. 3. Crystalline cryptocytochrome c obtained from the solublefraction of cell-free extracts of aerobically-grown cells manifestedthe same properties as cryptocytochrome c from anaerobically-growncells, i. e., absorption maxima, autooxidizability, redox potential,molecular weight, haem content, etc.
  4. 4. Cryptocytochrome cwas reversibly converted to a true haemochrometype spectrumby alcohols, detergents, carboxylic acid salts,guanidine saltor high pH values.
(Received December 16, 1968; )  相似文献   

3.
We have isolated a new flagellar mutant in Chlamydomonas reinhardtii.When the mutant was cultured under the white fluorescent lamp({small tilde}4,800 lux), most cells had no flagella. However,when the cultures were put in the dark, flagellation occurred.Greater than 70% of the cells had flagella within 12–16h after the transfer. The flagellar morphology varied from "rod-shape"(same as the wild-type flagella) to "disk-shape". The disk-shapedflagella had the axonemes which were curved into a loop withinthe swollen membrane. Hence, this mutant is called loop-1. Light-inhibitionof flagellation was restored in the presence of 10–5 MDCMU. The spectral dependency of the photo-inhibition of flagellation,determined using the Okazaki Large Spectrograph, showed maximaleffectiveness at 400–420 nm and 600–680 nm. Theseresults suggest that photosynthesis inhibits flagellation ofloop-1 cells. (Received July 27, 1989; Accepted January 29, 1990)  相似文献   

4.
LAPWOOD  D. H. 《Annals of botany》1957,21(1):167-184
  1. 1. Three organisms, Flavobacterium sp., Pseudomonas sp. designatedNo. 169 and Pseudomonas syringae, were compared with a pathogenBacterium aroideae. Although they all produced pectolytic enzymeof equal activity on potato extracts, only the pathogen wasable to parasitize the vegetable tissue, except when the watercontent of the latter was increased.
  2. 2. It was evident thatsuccess or failure of an attack was determinedwithin 24 hoursfrom inoculation. The events taking place duringthis periodwere studied in some detail with potato extractsand potatotubers. On dilute extracts the pathogen grew rapidly,with anacid drift of the medium, and pectolytic enzyme wasdetectablewithin a few hours from inoculation. The weaker organismsgrewslowly, with no acid-forming tendency, and showed a delayinenzyme secretion. Differences in growth and in secretionofenzyme were further accentuated when the extract approachedthe strength of potato sap.
  3. 3. No obvious qualitative differenceswere found between thepectolytic enzymes secreted by the fourorganisms.
  4. 4. The failure of the weak organisms to attacknormal potatotissue can be ascribed to their slower rates ofgrowth and enzymicsecretion which allow the host time to forma protective barrier.On the other hand, rapid growth and thesecretion of enzymewithin a few hours enabled B. aroideae tobecome establishedbefore a wound reaction could take place.
  相似文献   

5.
  1. Based on the microscopic observations, two stages, "giant cellstage" and the subsequent "palmelloid body stage", were distinguishedin the process of formation of giant Chlorella induced by theaddition of sugars. The "giant cell" is much larger in sizethan the control cell, but the other morphological featuresare the same as those of the latter. The "palmelloid body" isa form composed of many conjoined autospores.
  2. When a highconcentration of glucose was maintained in the medium,gigantismwas also maintained. Under this condition, the algashows acyclic transformation between "giant cell" and "palmelloidbody"without returning to the small single cells.
  3. Large amountsof carbohydrate composed of hexose were foundto be accumulatedin the giant algal cells, and it was inferredthat this carbohydrateaccumulation causes greater enlargementof cell volume as comparedwith control cells.
  4. Uronic acids, which were found to be absentin the control cells,were formed and lost in the cells culturedin the glucose mediumin parallel with the appearance and disappearanceof gigantism.
  5. Pectic substances, from which uronic acids areconsidered tobe derived during the extraction procedure, werefound to bepresent only in giant Chlorella.
  6. The conjoinedautospores in giant Chlorella (at the palmelloidbody stage)were separated to some extent by the addition ofEDTA, and theresulting cells were similar to control Chlorellacells.
  7. Basedon these results it was inferred that inductive formationofthe pectic substances is causally related with the appearanceof "palmelloid body".
1 Present address: Department of Chemistry, College of GeneralEducation, Osaka University, Toyonaka, Osaka.  相似文献   

6.
  1. Addition of exogenous acetate or ethanol to autotrophic culturesof Euglena gracilis strain Z induces formation of the glyoxylateby-pass.
  2. Visible light decreases the activity of malate synthasein greenEuglena by about 50%. No such effect was found in apermanentlybleached mutant.
  3. Aconitase activity parallelsthat of malate synthase, but isocitricdehydrogenase activityis constant under all conditions examined.
  4. Oxygen consumptionis proportional to the activities of malatesynthase and aconitase,but not to that of isocitric dehydrogenase.
  5. The results ofsimilar studies with other growth substrates(pyruvate, malate,succinate) suggest that some of the oxygenconsumed by C2-grownEuglena may not be associated with energyproduction.
(Received March 25, 1966; )  相似文献   

7.
  1. Enzymic activities pertaining to Porphyra tenera cytochrome553 were investigated with cell-free extracts of a red alga,Porphyra tenera, and various fractions prepared therefrom.
  2. Thealgal extracts were found to be incapable, in the dark,of catalyzingoxidation of reduced cytochrome 553 at a ratesufficient toaccount for the respiratory oxygen-uptake in theintact cell.Oxidation of cytochrome 553 was highly acceleratedon illumination.The former reaction was found to be cyanide-sensitiveand thelatter, cyanide-insensitive. Both activities were foundto belocalized in the particulate fraction of the cell extract.
  3. Significantactivities of reduced pyridine nucleotide-cytochromereductasewere discovered in the soluble fraction of the cellextract,the reaction being two or three times faster with TPNHthanwith DPNH as electron donor. There was no reaction withsuccinatein the presence of cytochrome and 2,6–dichlorophenolindophenol.
  4. Porphyra tenera cytochrome 553 was shown to be localized inthe plastids of the algal cell.
  5. Possible functions of cytochrome553 in the algal metabolismwere discussed.
  相似文献   

8.
  1. Two lactate dehydrogenases, L(+)- and D(–)- lactate cytochromec reductase, were extracted from the baker's yeast after disintegrationof the cells by a FRENCH press. They are separated by electrophoresison polyacrylamide gel and their activities were compared bycolor density of formazan, the reduction product of nitrobluetetrazolium.
  2. The ratio of L-lactate cytochrome c reductaseactivity to D-lactatecytochrome c reductase activity variedto a great extent, dependingon culture conditions. L-Lactatecytochrome c reductase waspredominant in resting cells; thereverse was the case withcells in early exponential stage ofthe growth.
  3. When the cells in exponential stage of growthwere aerated withoutnitrogen source, there occurred an intensiveincrease of L-lactatecytochrome c reductase, accompanied bythe decrease of D-lactatecytochrome c reductase.
  4. Effectsof inhibitors on the activity ratio of these two enzymeswereinvestigated. o-Phenanthroline, dinitrophenol, sodium azide,chloramphenicol, British antilewisite and antimycin A favored,in this order, the formation of L-lactate cytochrome c reductase.
(Received August 18, 1966; )  相似文献   

9.
  1. The effects of 3-(4'-chlorophenyl)-1, 1-dimethylurea (CMU)onthe fluorescence of photosynthetic pigments in vivo wereinvestigatedin blue-green, red and brown algae and in isolatedspinach chloroplasts.CMU caused an increase in steady statelevel of fluorescenceof chlorophyll a, but did not influencethe fluorescence ofphycobilins. The spectrum of the fluorescenceincrement hada peak at 685 m/µ and a shoulder at 730–740mµ.These two bands probably arise from chlorophyll a(Cf684) belongingto pigment system II.
  2. On excitation of chlorophylla in a red alga, Porphyra yezoensis,a fluorescence band witha peak at 720 mµ was observedbesides a shoulder at 685mµ. The 720 m band is inferredto arise from chlorophylla (probably, Cf-1) in pigment systemI.
  3. On addition of CMUto the algal cells, the induction of fluorescencewas modifiedto take a simple time course. The induction wasobserved onlywith respect to the fluorescence of chlorophylla, but not inthe fluorescence of phycobilins. The spectrumof the "transient"fluorescence showed two emission bands ofchlorophyll a at 685mµ and 740 mµ, and was quitesimilar in form tothe spectrum of the CMU-caused increase insteady state fluorescence.
  4. These facts were interpreted in terms of the correlation offluorescence of chlorophyll a and the photochemical reactionsof photosynthesis
(Received July 20, 1967; )  相似文献   

10.
A list of the determinations in this work is given below:
  1. Under standard conditions with a photoperiod, the generationtime is five days. The generation time is shorter in continuouslight.
  2. There are temperature-dependent cleavage and mitoticgradientswithin a colony.
  3. A diurnal peak of mitosis occurstwo hours before the onsetof darkness.
  4. Under standard conditions(a) the mitotic index rises to a maximumof 10 per cent, twodays after inoculation; (b) the mitotictime is ten minutes;and (c) the mitotic rate is 71 cells per103cells per hour atthe mitotic peak.
  相似文献   

11.
  1. The sugars which induced gigantism of Chlorella cells wereglucose,fructose, galactose, mannose, xylose and arabinose.These sugarswere utilized as respiratory substrates by thealgal cells.
  2. The cellular division of Chlorella was stimulatedby glucoseand galactose, but suppressed by fructose, mannose,xylose andarabinose, while all these sugars evoked gigantism.No correlationwas found between cellular division and gigantism,
  3. The photosynthetic activity of giant Chlorella varied withthesorts of sugars added. It was decreased by glucose, fructoseand mannose, but was unaffected by other sugars such as galactose,xylose and arabinose.
  4. The respiratory activity of giant Chlorellacells as much higherthan that of control cells.
  5. The amountsof protein-N and dry weight per unit volume of giantChlorellawere much less than those of control cells.
1 Present address: Department of Chemistry, College of GeneralEducation, Osaka University, Toyonaka, Osaka.  相似文献   

12.
  1. A substance which inhibits indoleacetic acid (IAA)-and naphthaleneaceticacid (NAA)-induced elongation of Avena coleoptile section andIAA-induced Avena coleoptile curvature was found in an ethersoluble neutral fraction of water extract of sunflower leavesand in agar blocks containing the diffusate from young sunflowerleaves.
  2. This substance also inhibits the growth of isolatedsunflowerepicotyl.
  3. The Rf value (0.9) of the substance ona paper chromatogramdeveloped with ammoniacal iso-propanolindicates that it isidentical with the inhibitor reported byAUDUS et al. (1956),but not with inhibitor-ß.
  4. Theinhibitor can be transported from leaf to stem, and thetransportseems to be accelerated by illuminating the leaf.
  5. The auxindiffused from sunflower leaf into agar block may beidenticalwith IAA.
  6. A substance, which has the same properties as theinhibitorfrom sunflower leaf, was obtained in crystalline formfrom theleaf of Jerusalem artichoke.
  7. The mechanism of growthinhibition caused by this crystallinesubstance seems to involveinactivation of a sulfhydryl group.
  8. The reason why the stemgrowth of sunflower seedlings is reducedby strong light isdiscussed: the amount of the inhibitor transportedfrom leafto stem is increased under strong light, and in thestem, growthinhibition is caused by a direct effect of thisinhibitor ongrowth and by its inhibiting effect on the transportof IAAfrom leaf to stem.
1 Present address: Botanical Garden, Faculty of Science, Universityof Tokyo, Tokyo (Received February 15, 1961; )  相似文献   

13.
Using diploid strains of Saccharomyces cerevisiae and S. ellipsoideus,the following facts were found:
  1. Indole-3-acetic acid, 2,4-dichlorophenoxyacetic acid and -naphthaleneaceticacid produced stable variants differing in the cell form andin the response to the actions of auxin to elongate cells, toinduce respiration- deficient mutation and to promote sporulation.
  2. The auxins also produced stable variants differing in theabilityto form spores.
  3. Acetic acid had no above-menthionedactions of auxin.
  4. Spore-formation and cell elongation of someof auxin-inducedvariants were controlled by auxin.
Biological significance of the auxin-induced variation is discussedand the usefulness of some of these variants as experimentalmaterial for auxin physiology in general is pointed out. (Received November 1, 1966; )  相似文献   

14.
  1. The cells of Thiobacillus thiooxidans, which had been in contactwith sulfur or sulfide in air (or CO2-free air), could fix addedCOa very rapidly after replacing air with nitrogen. This fixationis designated as the postoxidative fixation.
  2. "Preoxidation"of the sulfur compounds is mandatory for theoccurrence of thepostoxidative fixation.
  3. The cells which had preliminarilyoxidized sulfide could notshow the CO2-fixation, when theywere placed under an anaerobiccondition in the absence of thesulfur compound.
  4. These results indicate that sulfur compoundsmay have an importantrole as the electron donor for the reductionof CO2, besidestheir role as the substrate of respiration tosecure energyfor the fixation of CO2
(Received March 6, 1962; )  相似文献   

15.
  1. The formation, in the dark, of phycoerythrin in the preilluminatedcells of a blue-green alga, Tolypothrix tenuis, was investigatedwith special reference to its nitrogen metabolism.
  2. On incubatingthe pre-illuminated algal cells under a darkaerobiccondition,and with nitrate as N-source, the formation of phycoerythrinoccurs after an induction period of about 5 hours. No time-lagis observed in the nitrate-uptake by the organism. Similar resultsare obtained with nitrite, ammonia, urea and arginine as N-sources.
  3. The above stated formation of phycoerythrin is suppressedbysubstances such as chloramphenicol and p-fluorophenylalanine,substances known to be potent inhibitors of protein-synthesis.
  4. On the basis of these findings, it was inferred that therearetwo consecutive processes involved in the dark-formationofphycoerythrin in the pre-illuminated cells: (i) uptake andconversionof exogenous nitrogen sources into some intermediarynitrogenouscell substances, and (ii) synthesis of the pigment-proteinfromthese substances.
(Received June 27, 1960; )  相似文献   

16.
  1. The relation between chlorophyll content and the hydrolyticactivity of chlorophyllase in Chlorella protothecoides was examined.An increase in the activity was parallel to that in chlorophyllcontent during the development of green colouration, or greeningcourse, in the bleached cells. The activity sharply declinedand a parallel disappearance of chlorophyll was also found duringbleaching of the green cells.
  2. A partially purified water-solublepreparation of chlorophyllasewas obtained by n-butanol treatmentand fractionation with coldacetone. It showed high activityand hydrolyzed 2 mg chlorophylla per hr per mg protein.
  3. Forseparation and identification of the pigments concernedin thechlorophyllase reaction, a new solvent system of paperchromatographywas introduced.
  4. When methyl chlorophyllide a and phytol wereincubated withthe enzyme, two products were formed. By comparisonwith theRf values of isolated pure substances, one was identifiedaschorophyll a and the other as chlorophyllide a. This enzymedid not catalyze the phytylation of free chlorophyllide a, butit had the ability to attach phytol to methyl chlorophyllidea. The final step in the biosynthesis of chlorophyll a is brieflydiscussed.
1 Contribution No. 158 from the Department of Biology, Facultyof Science, Kyushu University. Supported in part by a grant-in-aidfor Fundamental Scientific Research from the Ministry of Education.  相似文献   

17.
  1. Evidence was obtained which supports the hypothesis that thefirm colonies of Nostoc verrucosum, but not the softer onesof N. commune, can accumulate phosphate from the environmentby non-active means.
  2. This accumulation of phosphate was reducedby pre-treating thecolonies with chelating agents, whilst thepresence of CaCl2in the medium led to an increase.
(Received February 2, 1967; )  相似文献   

18.
  1. Solubilization of chioroplasts with a mixture of 1 per centDuponol C and 1 per cent Span 80 (3: 1) caused a destructionof activity in the HILL reaction, but the treatment broughtabout an increase by about 60 per cent in the rate of ascorbatephotooxidation in the presence of DPIP. Heating the broken chloroplastscaused a marked decrease in the photooxidation activity. Byadding surface- active agents to the boiled preparation, theactivity was restored up to almost 80 per cent of the originallevel.
  2. With colloidal suspensions of isolated chiorophylls,ascorbatewas only slightly photooxidized in the presence ofDPIP. Byaddi tion of the surface-active agents, the activitywas greatlyenhanced.
  3. Dependency of the photooxidation bywhole and solubilized chloroplastsand isolated chlorophylla on the presence of DPIP was examined.DPIP can serve as anintermediate electron carrier in solubilizedchloroplasts aswell as in whole chloroplasts.
  4. Effect of o-phenanthrolineon ascorbate photooxidation by thesethree preparations wastested. With solubilized chloroplastsand isolated chlorophylls,the addition of the inhibitor hadno influence on their ascorbatephotooxidation either in thepresence or absence of DPIP.
  5. Treatmentof whole chloroplasts with the surface-active agentsinducedan activity of photooxidation of cytochrome c. The electron-flowpattern for the photooxidation of ascorbate by whole and solubilizedchloroplasts was briefly discussed.
1 Contribution No. 130 from the Department of Biology, Facultyof Science, Kyushu University. Aided in part by Grant-in-Aidfor Fundamental Scientific Research from the Ministry of Education. (Received August 23, 1962; )  相似文献   

19.
  1. Using the technique of synchronous culture, investigationsweremade of the effects of temperature and light-intensityon cellularlife cycle of Chlorella ellipsoidea. Some improvementsin theculture technique for obtaining a good synchrony of algalgrowthwere described.
  2. By following the changes of averagecell volume and cell numberoccurring during culturing, therates of the following processesof life cycle were determined:(i) "growth" (or the increasein cell mass) occurring from thestage of smaller cells (Da)to the stage of ripened cell (L3),(ii) "ripening" (or processofformation of "nuclear substances"as estimated from the averagenumber of daughter cells formedfrom single mother cell), and(iii) " maturing and division" which leads to the full maturationof mother cells (L-cells)and their division into separate daughtercells (D-cells).
  3. "Growth"and "ripening" were found to be dependent in light,"maturingand division" light-independent. The time requiredfor "growth"and "ripening" (C) is dependent on temperaturebut independentof light intensity, the onset of "maturing anddivision" occurringat the same time (D) of culturing undervaried light intensities.The average cell volume at this stage(L3),however, was foundto be markedly modified by light intensity;larger with highertemperatures (see Fig. 4).
  4. Changes in incubation temperature(under the condition of saturatinglight intensities) were foundto affect the life cycle in thefollowing way: (i) The timeof onset of "maturing and division"(D), varies markedly withculturing temperature; earlier athigher temperatures, (ii)The average cell volume at this stagealso depends on temperature; smaller at higher temperatures.
  5. The average number of daughtercells (n) emerging from singlemother cells, was found to beuninfluenced by culturing temperature;(4.0–4.1 underthe conditions of the present study). Itwas found that thedivision number n is remarkably varied bychanging the lightintensity in the "growth" and "ripening"phases; 2.0 at 1 kilolux,3.7 at 5 kilolux, 4.2 at saturatinglight intensities (10 and25 kilolux). This finding was explainedby assuming a light-dependentformation of "nuclear substances"during the "growth" and "ripening"phases, the quantity of thesubstances in the cell at L3 stagedeterminig the division number.
  6. The experimental data wereanalyzed reaction kinetically, therate constants and othercharacteristics of the reactions constitutingthe processesof life cycle were determined, and values forthe apparent activationenergy for each reaction were computed.The reactions were discussedwith special reference to theirrelationship with photosyntheticprocess was discussed.
(Received November 7, 1959; )  相似文献   

20.
  1. A fairly good synchronization of Scenedesmus cells was obtainedby transferring the cells grown in a medium containing a lowconcentration of iron into a medium containing relatively highconcentration of iron.
  2. During the synchronous culture in themineral medium, a goodparallelism between the average cellvolume and hydrogenaseactivity was observed.
  3. Effect of glucoseon the development of the hydrogenase activitywas variabledepending on the stage of algal growth.
  4. Iron is essentialfor the development of the hydrogenase activityand glucosesupplementary.
1On leave from Laboratory of Applied Botany, Faculty of Agriculture,Kyoto University, Kyoto.  相似文献   

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