Studies on the Hill reaction of membrane fragments of blue-green algae III. Fluorescence characteristics of membrane fragments of Anabaena variabilis and Anabaena cylindrica

Fluorescence spectra of the pigment system at –196°Cin membrane fragments of Anabaena variabilis and A. cylindricawere investigated. The fluorescence spectra of membrane fragments having four emissionbands at 645–655, 685, 695 and 725 nm were basically similarto those reported for intact cells of blue-green algae, thoughthe emission from phycocyanin (645–655 nm) was far strongerwith membrane fragments than with intact algal cells. Incubation of membrane fragments of A. variabilis in a dilutebuffer (10^–2M, pH 7.5) caused an increase in the 645 nmfluorescence and slight decreases in the 685 and 695 nm fluorescences,but had no influence on the 725 nm fluorescence. The decreasein the 685 and 695 nm fluorescences of A. cylindrica was moremarked and had the same kinetics as the inactivation of photosystemII reaction measured by DPIP-photoreduction. When membrane fragments of A. cylindrica were incubated in thebuffer solution at room temperature or in the presence of MgCl₂(10^–3M) at 0°C; phycobilin aggregates, which emittedthe 655 and 685 nm fluorescence, were solubilized. This solubilizationwas not observed with membrane fragments of A. variabilis. (Received August 31, 1972; )     

Nutrient Solution pH Control using Dipolar Buffers in Studies of Trifolium repens L. Nitrogen Nutrition

In studies of Trifolium repens nitrogen nutrition, the controlof nutrient solution pH using dipolar buffers, was evaluatedin tube culture under sterile conditions. Five buffers; MES,ADA, ACES, BES and MOPS with pK₂s (20 °C) of 6.15, 6.60,6.90, 7.15 and 7.20 respectively, at a concentration of 2.0mol m^–3, were provided to inoculated Trifolium repensgrowing in nutrient solution containing 7.13 mol m^–3 nitrogenas (NH₄)₂SO₄. Initial pH of each solution was adjusted to theappropriate buffer pK₂ Two buffers, ADA and ACES completelyinhibited plant growth. The remaining buffers had little effectin limiting pH change, although plant dry matter was higherand nodule numbers lower in the presence of these buffers. MESand MOPS were supplied to nutrient solutions with and without7.13 mol m^–3 (NH₄)₂SO₄, at concentrations ranging from0–12 mol m^–3. MES at 9 mol m^–3 and 12 molm^–3 reduced growth of plants reliant on the symbiosisfor providing nitrogen. The provision of MES to plants providedwith NH₄⁺ significantly increased plant yield and reduced nodulenumber at all concentrations. MOPS did not affect plant yieldor nodule number. The use of dipolar buffers in legume nitrogennutrition studies is considered in terms of buffering capacity,and the side effects on plant growth and symbiotic development. Key words: Ammonium, Dipolar buffer, Nitrogen nutrition, pH control, Symbiosis, Trifolium repens     

Simulating the Mineral Environment of Aluminium Toxic Soils in Plant Cell Culture

The development of a medium for studying aluminium toxicityin plant cell cultures is described. To prevent the precipitationof Al added to the standard cell culture medium, it was necessaryto lower the phosphate concentration from 1250 mmol m^–3to10 mmol m^–3, and the pH from 5.8 to 4-0. Two additionalmodifications were the use of unchelated iron and a reductionin the calcium concentration from 3.0 mol m^–3 to 0.1 molm^–3. Since the gelling properties of agar are inhibitedat pH 4.0, cells were cultured on filter paper supported bypolyurethane foam sturated with liquid medium. The only limitationto the growth of plated Nicotiana plumbaginifolia Viv. cellson the modified medium was the reduced phosphate concentration.This was partly overcome by ‘preloading’ the cellswith phosphate prior to each experiment. In addition, the filterpaper with adhering cells was transferred to fresh medium everysecond day to replenish phosphate, and to re-establish the initialpH of4.0 (which otherwise drifts upward). With the modifiedmedium, Al toxicity was observed in plated N. plumbaginifoliacells at both 200 mmol m^–3 and 400 mmol m^–3 Al.There was no toxicity at these Al concentrations when the normalphosphate concentration or pH were restored to the modifiedmedium. Partial alleviation of Al toxicity occurred with restorationof the normal calcium concentration or chelated iron. Chelationof Al with citrate or EDTA also mitigated Al toxicity. In additonto Al toxicity, the modified medium should also prove usefulfor studying other metal toxicities in plant cell culture. Key words: Al toxicity, Cell culture, Nicotiana plumbaginifolia     

Specific inhibitory effect of copper on cellular division in Chlorella

By growing Chlorella ellipsoidea synchronously by the techniqueof TAMIYA et al. with some modifications, it was demonstratedthat cellular division of ripened cells (L₂- and L₃-cells) inthe dark is specifically inhibited—especially stronglyat pH 6.3—by cupric ion present in the medium. The possibleattack site of cupric ion in cellular division of this algais discussed. (Received March 12, 1969; )     

Synthesis of Bis-piperazine-type pH Buffer Agents and Their Application to Mammalian Cell Cultures

New bis-piperazine-type pH buffer agents were synthesized and their buffering properties were evaluated. The compounds proved to have two-fold larger pH buffering ability than 2-[4-(2-hydroxyethyl)-1-piperazinyl]ethanesulfonic acid (HEPES), a Good’s buffer traditionally used to control the pH value of culture media.

Human-human hybridoma HB4C5 cells were cultured in a serum-free medium containing these buffer agents. The cell growth and antibody production, using 1,2-N,N′-bis[N′′,N′′′-di(2-sulfonoethyl)piperazinyl]ethane, were greater than when HEPES.     

Influence of pH on the transition from yeast-like cells to chlamydospores in Aureobasidium pullulans

When A. pullulans is grown on a glucose medium with a limiting nitrogen source and low buffer capacity, the yeast-like cells that are originally present undergo a transition to chlamydospores. The initial pH must be around 6 for the transition to take place under optimal conditions. On the above-mentioned medium pH decreases to values below 2 in the first two days; if this decrease is prevented, either by buffering the medium or by repeatedly adjusting the pH to its original value no chlamydospores form.     

Comparison of growth characteristics of New Zealand isolates of the prymnesiophytes Chrysochromulina quadrikonta and C.camella with those of the ichthyotoxic species C.polylepis

Chrysochromulina quadrikonta (Prymnesiophyceae), a quadriflagellatespecies previously unrecorded in New Zealand, was isolated fromNelson Harbour, New Zealand, in autumn 1991. It bears unmineralizedplate and spine scales, which morphologically are most likethose of Chrysochromulina ericina. Chrysochromulina quadrikonta,Chrysochromulina camella (isolated from the Marlborough Sounds,New Zealand) and Chrysochromulina polylepis (an ichthyotoxicspecies originally isolated from Scandinavia) grew most rapidly(growth rates, or divisions per day, of 1.41, 1.49 and 1.43,respectively) when cultured in a seawater-based general-purposenutrient medium at a salinity of 24% and pH 7.9, with only C.camellastill growing at 42% Chrysochromulina quadrikonta and C.camellagrew optimally at 25°C. and C.polylepis between 15 and 20°C;only C.polylepis grew at 10°C. Chrysochromulina quadrikontagrew optimally with potassium nitrate and ammonium chlorideas nitrogen source, whereas C.camella and C.polylepis grew equallywell with urea as nitrogen source. Only C.quadrikonta and C.polylepishad a selenium requirement. Unlike C.polylepis, neither of theNew Zealand isolates was phagotrophic nor ichthyotoxic.     

Studies on the Growth in Culture of Plant Cells: IV. THE INITIATION OF DIVISION IN SUSPENSIONS OF STATIONARY-PHASE CELLS OF ACER PSEUDOPLATANUS L.

Techniques are described whereby a culture medium can be ‘conditioned‘by separation from a dense cell suspension either by a sinteror by a dialysis membrane. The enhanced growth-promoting activityof the conditioned, as compared with a new medium, is revealedby using a low density of cells (15 x 10³ or less cells perml) to initiate the test cultures from a stationary-phase suspension.The optimum pH of the conditioned medium is c6.4. To obtaina conditioned medium of high activity it is necessary to usean appropriate volume ratio of culture medium to conditioningcell suspension and to limit the conditioning period. Conditioningof the culture medium reduces by a factor of 10 (i.e. down toc. 1000 cells per ml) the minimum effective cell density neededfor self-sustaining growth. There therefore exists a population-dependentrequirement which is not met by the conditioned medium as nowprepared. The retention of the activity of the conditioned mediumin various situations has been studied as a preliminary to workon the chemical basis of conditioning.     

Somatic Embryogenesis and Plant Regeneration from Freely-suspended Cells and Cell Groups of Panicum maximum Jacq

Embryogenic calluses derived from cultured immature embryosand young inflorescences of Panicum maximum Jacq. were placedin Murashige and Skoog's liquid medium supplemented with 1 mg1^–1 2, 4- dichlorophenoxyacetic acid (2, 4-D) and 2.5per cent coconut water, to initiate suspension cultures. Suspensionsconsisted of two types of cells: small, richly-cytoplasmic andoften starch-containing embryogenic cells, and large, vacuolatednon-embryogenic cells. A presumed sequence of developmentalstages from single embryogenic cells to globular and heart-shapedstages of embyrogenesis was observed in the suspension cultures.Plantlets were produced from the embryoids when the suspensionswere plated in an agar medium without any hormone or with only0.2 mg 1^–12, 4-D or naphthalene acetic acid. Embryogenicsuspension cultures derived from immature embryos as well asfrom inflorescence segments gave rise to plants which showedthe normal somatic chromosome number of 2n = 4x = 32. Panicum maximum Jacq., Guinea grass, embryogenesis, regeneration, suspension culture     

The Establishments of Tissue 4

Callus cultures of 12 temperate grasses were established, somefor the first time, by incubating detached roots or whole seedlingson a Linsmaier and Skoog basal medium which contained 2, 4-dichlorophenoxyaceticacid (2, 4-D) at 1.0 mg 1^–1 as the only growth hormone.The callus, which developed in the pericycle of the roots andon the embryo of the seeds, was subcultured on the same medium;further growth of the callus varied from good in the case ofDactylis glomeraia, Agrostis tennis, Cynosurus cristatus, andPoa trivialis, to poor in several Lolium species and varieties.Most cultures developed root primordia which sometimes grewinto visible roots, but shoot primordia, none of which grewinto shoots, were found only in the callus of Lolium multiflorumvar. westerwoldicum. Cell suspension cultures were also readily established and maintainedusing the same culture medium. Most cultures contained a highproportion of round or oval cells, which ranged from 18 to 77µm in diameter or length, while many also had a significantproportion of larger, more elongated cells which varied in lengthfrom 46 to 182 µm. The cells of Dactylis glomerata werecharacteristically larger and more convoluted than the cellsof other grass species that were examined. The addition of kinetinat 0.1 mg 1^–1 to the 2, 4-D-containing culture mediumincreased the proportion of irregular-shaped cells and reducedthe dispersion of the cells, perhaps by improving cellular contactand adhesion; in some species, such as Agrostis tenuis and Phleumpratense, the presence of kinetin promoted the deposition ofstarch granules in cells.     

pH and buffer capacities of apoplastic and cytoplasmic cell compartments in leaves

After opening the stomata in CO₂-free air, darkened leaves of several plant species were titrated with CO₂ at concentrations between 1 and 16%, in air in order to reversibly decrease cellular pH values and to calculate buffer capacities from pH changes and bicarbonate accumulation using both gas-exchange and fluorescence methods for analysis. After equilibration with CO₂ for times ranging between 4.4 and 300 s, fast CO₂ release from bicarbonate indicated catalysis by highly active carbonic anhydrase. Its time constant was below 2.5 s. Additional CO₂ was released with time constants of about 5, 15 and approximately 300 s. With CO₂ as the acidifying agent, calculated buffer capacities depend on assumptions regarding initial pH in the absence of an acid load. At an initial stroma pH of 7.7, the stromal buffer capacity was about 20 mM pH-unit⁻¹ in darkened spinach leaves. At an initial pH of 7.5 it would be only 12 mM pH-unit⁻¹, i.e. not higher than expected solely on the basis of known stromal concentrations of phosphate and phosphate esters, disregarding the contribution of other solutes. At a concentration of 16%, CO₂ reduced the stromal pH by about 1 pH unit. Buffering of the cytosol was measured by the CO₂-dependent quenching of the fluorescence of pyranine which was fed to spinach leaves via the petiole. Brief exposures to high CO₂ minimized interference by effective cytosolic pH regulation. Cytosolic buffering appeared to be similar to or only somewhat higher than chloroplast buffering if the initial cytosolic pH was assumed to be 7.25, which is in accord with published cytosolic pH values. The difference from chloroplast pH values indicates the existence of a pH gradient across the chloroplast envelope even in darkened leaves. Apoplastic buffering was weak as measured by the CO₂-dependent quenching of dextran-conjugated fluorescein isothiocyanate which was infiltrated together with sodium vanadate into potato leaves. In the absence of vanadate, the kinetics of apoplastic fluorescence quenching were more complex than in its presence, indicating fast apoplastic pH regulation which strongly interfered with the determination of apoplastic buffering capacities. At an apoplastic pH of 6.1 in potato leaves, apoplastic buffering as determined by CO₂ titration with and without added buffer was somewhat below 4 mM pH-unit⁻¹. Thus the apoplastic and cytosolic pH responses to additions of CO₂ indicated that the observed cytoplasmic pH regulation under acid stress involves pumping of protons from the cytosol into the vacuole of leaf cells, but not into the apoplast. Received: 27 November 1998 / Accepted: 22 March 1999     

Growth Stimulation by Conditioned Medium and Spermidine in Low-Density Suspension Cultures of Rice

Suspension cultures of Oryza sativa L. var IR 20 grew in Murashigeand Skoog medium (MS) supplemented with 2,4-D and kinetin ina density-dependant manner with a critical minimum inoculation-densityof 10,000 cells ml^–1. Conditioned medium obtained fromthese cultures and added to MS+2,4-D+kinetin induced the growthof cultures at 1,000 cells ml^–1. Growth stimulation byconditioned medium was mimicked by spermidine but not by otherpolyamines viz. putrescine and spermine. This is the first reportof a polyamine substituting for conditioned medium in cultures. ² Present address: Vice-Chancellor, Pondicherry University,Pondicherry 605 014, India.     

Der Einflu{beta} verschiedener Lichtqualitaten auf Chlorophyllgehalt und Wachstum von Gewebekulturen aus Crepis capillaris (L.) WALLR.

The influence of different light qualities on chlorophyll contentand growth of tissue cultures from Crepis capillaris (L.) WALLR. Tissue cultures from Crepis capillaris growing on media (M₁; M₂ ; M₂-E) formed chlorophyll and intact chloroplasts onlyin the short wave length region of the visible spectrum (350–550nm). In red light (600–700 nm) as well as in darknessthey lost their chlorophyll after 8–10 weeks. The growth of Crepis-cultures was strongly influenced by lightand the nitrogen of the medium. The highest increase in freshweight (425–485% increase in 3 weeks) was attained inred light or in darkness on M₂ by cultures which had lost theirchlorophyll completely. M₂ contains nitrates, ammonium saltsand amino acids. In contrast, the increase in fresh weight ofgreen cultures growing on M₂ in blue or white light was considerablylower (155–180% increase in 3 weeks). Omission of amino acids, (M₂-E), resulted in the reduction ofthe growth (increase of fresh weight in 3 weeks: 120%) of thechlorophyll-free cells growing in the dark. Green cultures behaveddifferently on M₂-E. In white light they attained an increasein fresh weight of 245%. This suggests that the growth promotingeffect of the amino acids can be replaced by light. Results with cultures growing on M₁, which contains neitherammonium salts nor amino acids, point in the same direction.Green cultures in white or blue light grew better (90–100%increase in fresh weight in 3 weeks) on this "deficient" mediumthan chlorophyll-free tissues in red light or in darkness (20–30%increase in fresh weight in 3 weeks). Some aspects of thesefindings which concern the effect of light on growth are discussed. (Received November 28, 1969; )     

Effects of Glycollate on the Growth of a Planktonic Chlorella

The duration of the lag phase in cultures of a planktonic strainof Chlorella pyrenoidosa growing from small inocula under conditionsof light limitation was shortened by the addition of 1 mg 1^–1of glycollate to the medium. Of eight related compounds tested,none, with the possible exception of lactate, had a similareffect. Addition of 1 mg 1^–1 of glycollate also considerablyincreased the relative growth-rate of the alga at low (500 lux)but not at higher light intensities. This effect was not, however,specific to glycollate. Concentrations of glycollate (20 mg1^–1) higher than those normally produced in cultures byexcretion had an inhibitory effect on growth.     

Proteolytic stability of recombinant human serum albumin secreted in the yeast Saccharomyces cerevisiae

 In order to direct the persistent expression of recombinant human serum albumin (HSA) from the GAL10 promoter in the yeast Saccharomyces cerevisiae, we carried out periodic feeding of galactose during shake-flask cultures. Unexpectedly, the recombinant protein secreted was observed to undergo rapid degradation, which was apparently accelerated by carbon-source feeding. The extracellular degradation of HSA occurred even in the strain deficient in the major vacuolar proteases PrA and PrB, and in the strain lacking the acidic protease Yap3p (involved in the generation of HSA-truncated fragments). Interestingly, the degradation correlated closely with the acidification of extracellular pH and thus was significantly overcome either by buffering the culture medium above pH 5.0 or by adding amino acid-rich supplements to the culture medium, which could prevent the acidification of medium pH during cultivation. Addition of arginine or ammonium salt also substantially minimized the degradation of HSA, even without buffering. The extracellular degradation activity was not detected in the cell-free culture supernatant but was found to be associated with intact cells. The results of the present study strongly suggest that the HSA secreted in S. cerevisiae is highly susceptible to the pH-dependent proteolysis mediated by cell-bound protease(s) whose activity and expression are greatly affected by the composition of the medium. Received: 23 August 1999 / Received revision: 8 November 1999 / Accepted: 12 December 1999     

Growth and Maintenance of an Embryogenic Cell Culture of Daylily (Hemerocallis) on Hormone-free Medium

Callus cultures of the diploid daylily (Hemerocallis) clone‘Autumn Blaze’ were initiated and maintained inhormone-containing nutrient medium. At various times (from 6weeks to 1 year) after being initiated, hormone-derived cultureswere evaluated for their ability to be maintained and to multiplyon hormone-free medium at low pH (between pH 4 and 4.5). Cultureshad to be exposed to hormone-containing medium for at least12 weeks before they could be maintained on hormone-free mediumat low pH. The transition to maintainability on low pH hormone-freemedium included the production of many aberrant embryonal forms('neomorphs'). However, all hormone-derived cultures testedconsisted entirely of preglobular stage proembryos (PGSPs) after12–24 weeks on low pH hormone-free medium. PGSP cultureshave been maintained and multiplied as such for over 1 yearon low pH hormone-free medium. PGSPs continue their developmentinto various somatic embryo stages when cultured on hormone-freemedium buffered at pH 5.8. The production of well-formed somaticembryos was greatly enhanced when PGSPs were plated on activatedcharcoal impregnated filter papers that were placed on top ofthe agar surface. The gross morphology and histology of thePGSPs and stages of somatic embryo development are presented.The work shows that the ability of hormone-free medium at lowpH to permit PGSP multiplication without development into laterstages of embryo development is not restricted to carrot. Hemerocallis cv, ‘Autumn Blaze’, daylily, somatic embryogenesis, hormone-free medium, tissue culture     

In vitro Propagation of Red Cabbage (Brassica oleracea L. var. capitata)

By manipulation of various growth regulators and physical conditions,plants have been regenerated from excised roots, stem segments,cotyledons, leaves, and callus cultures of red cabbage (Brassicaoleracea var. capitata) grown under in vitro conditions. Shootbuds were induced on isolated root segments (1 cm long) culturedon Murashige and Skoog's medium and the frequency of bud formationwas greatly enhanced by the addition of kinetin (0.5 part 10^–6).Callus obtained from the seeds, cotyledons, and hypocotyl segmentscultured on a medium fortified with 2,4-D (1 part 10^–6),kinetin (0.1 part 10^–6), and coconut milk (10%, v/v) hasbeen repeatedly subcultured. The callus is slow growing, andon transference to a kinetin (2 parts 10^–6) and IAA (2parts 10^–6) medium underwent morphogenesis to give riseto plants. The significance of the propagation of red cabbageby in vitro culture is pointed out.     

Influence of ionic composition,buffering agent,and pH on the histochemical demonstration of myofibrillar actomyosin ATPase

Summary The influence of the composition of the preincubation medium on the histochemical demonstration of myofibrillar actomyosin ATPase, including a variety of carboxylic acid and non-carboxylic acid buffering compounds and neutral salts, was studied. In inorganic salt-free systems the rate of the activation of type I fibers and inactivation of type II fibers was accelerated when the carboxylic acids had longer chain length or multiple carobxyl groups. Of these factors, the number of carboxyl groups was dominant with a 100 mM citrate buffer producing a sharp differentiation between fiber types. In contrast, the time course of the response was exceptionally long in an acetate buffer. The time course of the ATPase reaction was also modified by other buffers at pH 4.60. The most notable were an ascorbate — glycine buffer system which produced little or no deviation from the alkaline preincubation staining pattern after prolonged preincubation and a pyrophosphate system which produced a rapid change. Neutral salts in the preincubation medium accelerated the time course of the inactivation — activation process with the order for the halogen salts of K⁺ being F⁻<Cl⁻<Br⁻<I⁻, which is a progression by molecular weight. The only sequence for cations on the myofibrillar actomyosin ATPase was Li⁺< Na⁺<K⁺. The response to salts was concentration dependent. An interaction existed between buffering compound, type of salt, and pH. These experiments demonstrate that the histochemical differentiation of fiber types by the myofibrillar actomyosin ATPase reaction depends upon a modification of some component(s) of the myofibrillar complex that can be influenced by a number of factors.     

Stabilization of the synthetic media for plant tissue and cell cultures

In standardMurashige-Skoog medium, particularly at pH higher than 5.0 and after heat sterilization, there is a tendency for turbidity or a sediment to appear, and for the acidity to increase by 0.2 to 0.5 degrees pH. The sediment is an amorphous precipitate of ferric phosphate and partly also of ferrous phosphate. In a stock iron solution prepared by chelation of ferrous sulphate with an equimolar quantity of the complexone Na₂EDTA. up to 10% free Fe^II ions could be detected. By titration of a concentrated complexon solution it was found that in the presence of an excess of Na₂EDTA (at the approximate molar ratio Fe^II: Na₂EDTA 1: 2) chelation of this free iron takes place to such an extent that its concentration falls to as little as 0.1%. Media with iron stabilized in this way are quite clear and maintain the adjusted pH for up to several weeks. The heat sterilization, too, does not lead to any precipitation or to a shift in pH within the broad range of adjusted values pH 4.8 – 6.0. We also attempted to increase the relatively low buffering capacity of Murashige-Skoog medium. The addition of sodium citrate (1.25 mmol 1^-1) and particularly of citrate-phosphate buffer (at a final concentration of 1.97 mmol citric acid and 6.07 mmol dibasic sodium phosphate per litre of medium) to the Murashige-Skoog medium considerably increased its buffering capacity, so that at the end of the subculture interval of tobacco cell suspensions the adjusted acidity changed only slightly (pH 5.40 ± 0.15). A thorough evaluation of the growth parameters of tobacco batch cultures (cell counts, vital staining, kinetics of DNA and protein synthesis) failed to reveal any negative effect either of additional chelation or of the buffering components.     

Photoinhibition of Glucose Uptake in Chlorella

In colorless mutant cells of Chlorella vulgaris (M125), endogenousrespiration in the dark was not affected by 30-min preilluminationwith white light (9,000 mW?m^–2), while exogenous respirationof glucose or fructose was inhibited significantly by the sametreatment in air, but not under N₂. This light effect on exogenousrespiration was accompanied by an inhibition of hexose uptake. When autotrophically grown wild-type cells of Chlorella vulgaris(211-11h) were incubated in glucose medium with DCMU, lightalso greatly inhibited glucose uptake and growth. Blue lightwas very effective, while red light had only a slight effect.This photoinhibitory effect was also observed in algal cellsthat had been grown in a glucose-containing medium in the dark. Using SDS-gel electrophoresis, a new protein peak with a molecularweight of 35–40 kDa was detected in plasma membrane-richcell wall fractions when Chlorella vulgaris (211-11h) cellswere transferred to a glucose-containing medium. This peak disappearedafter the algal cells were returned to the glucose-free medium.These findings suggest that this protein includes the hexose-carrierprotein. Blue light significantly inhibited the formation ofthis protein during incubation in a glucose-containing medium. ¹ Present address: Laboratory of Chemistry, Faculty of PharmaceuticalSciences, Teikyo University, Sagamiko, Kanagawa 199-01, Japan. (Received July 31, 1986; Accepted March 12, 1987)