Isolation of Hair Cells from Azolla filiculoides var. japonica Leaves

A procedure has been developed to isolate hair cells from Anabaenacontaining packets of the aquatic fern Azolla. Unbroken algalpackets, isolated by enzyme treatment and flotation on 12.5%Percoll solution, contained hair cells, Anabaena filaments andthe envelope membrane. When the packet suspension was gentlypipetted, hair cells attached to the envelope membrane becamedetached from the Anabaena filaments. Hair cells were separatedby flotation on 34% Percoll solution and further purified bysifting through nylon mesh. Both branched and unbranched cellswere isolated and about 70% remained unstained by 0.1% trypanblue. Electron microscopic observation showed that these cellswere protoplasts enclosed by a thin envelope and had well preservedinternal structures. The activities of ammonia-assimilatingenzymes in the hair cells were much higher than those in Azollaleaves, while the activities in the endophytes were repressedto very low levels. These results suggest that hair cells playan important role in the assimilation of the nitrogen whichthe endophytes fix and release into the cavity. (Received March 24, 1986; Accepted June 28, 1986)     

Reduced Phosphorus Requirement of a Mutant Azolla-Anabaena Symbiotic N2-fixing Complex

The use of the photo-autotrophic nitrogen-fixing water fernAzolla as an effective source of organic nitrogen in tropicalpaddy fields has been limited by a high phosphorus requirement.Azolla species with a minimum of 1.5 to 2.0 mM phosphate (P)requirement, under controlled conditions, are known. A local Azolla species requiring at least 1.5 mM sodium phosphatefor a normal rate of multiplication and N₂ fixation was exposedto N-methyl-N'-nitro-N-nitrosoguanidine (MNNG). The resultingmutant population had a significantly lower P requirement, butwas auxotrophic for glutamine with an extremely reduced glutaminesynthetase (GS) activity. An L-methionine-DL-sulphoximine (MSX)-resistant(MSX^r) Azolla population, having an approximately 1.5 timeshigher GS activity than that of the wild type (WT) parent organism,was cultured and subjected to MNNG-induced mutation for lowP requirement while putting MSX as a control in the mutant selectionmedium. The resulting population of mutant Azolla was a normalprototroph with a P requirement as low as 0.75 mM for its ‘WTparent-like’ usual growth and N₂ fixation. Key words: Azolla, phosphorus requirement, mutation     

DIVERSITY AND HOST SPECIFICITY OF AZOLLA CYANOBIONTS1

A unique, hereditary symbiosis exists between the water fern Azolla and cyanobacteria that reside within a cavity in the dorsal leaf‐lobe of the plant. This association has been studied extensively, and questions have frequently been raised regarding the number and diversity of cyanobionts (cyanobacterial symbionts) among the different Azolla strains and species. In this work, denaturating gradient gel electrophoresis (DGGE) and a clone library based on the 16S rRNA gene were used to study the genetic diversity and host specificity of the cyanobionts in 35 Azolla strains covering a wide taxonomic and geographic range. DNA was extracted directly from the cyanobacterial packets, isolated after enzymatic digestion of the Azolla leaves. Our results indicated the existence of different cyanobiont strains among Azolla species, and diversity within a single Azolla species, independent of the geographic origin of the host. Furthermore, the cyanobiont exhibited host‐species specificity and showed most divergence between the two sections of genus Azolla, Azolla and Rhizosperma. These findings are in agreement with the recent redefinition of the taxon Azolla cristata within the section Azolla. With regard to the taxonomic status of the cyanobiont, the genus Anabaena of the Nostocaceae family was identified as the closest relative by this work.     

Effects of Atmospheric NO2 on Azolla-Anabaena Symbiosis

Cultures of the water fern Azolla pinnata R, Br. exposed for1 week to atmospheric NO₂ (50, 100 or 200 nl l^-1) induced additionallevels of nitrate reductase (NaR) protein and nitrite reductase(NiR) activity. At low concentrations of NO₂ (50 nl l^-1), nitratederived from NO₂ provides an alternative N source for Azollabut does not affect rates of acetylene reduction. However, thesymbiotic relationship between Azolla and its endosymbiont,Anabaena azollae is only affected adversely by high concentrations(100 and 200 nl l^-1) of atmospheric NO₂. The resultant decreasesin rate of growth, nitrogen fixation, heterocyst formation,and overall nitrogen cycling are probably due to the additionalaccumulation of N products derived from higher levels of atmosphericNO₂. Parallel increases in levels of polyamines suggest thatAzolla partially alleviates these harmful effects by incorporatingsome of the extra NO₂-induced N into polyamines.Copyright 1994,1999 Academic Press Azolla-Anabaena symbiosis, nitrogen dioxide pollution, nitrogen metabolism, polyamines     

High Concentrations of Ammonium Ions at Low pH Decrease the Number of Cyanobionts in Apical Portions of Azolla

When Azolla plants (Azolla filiculoides vax.japonica) were grownin media with high concentrations of ammonium ions at pH 3.5,numbers of cyanobionts in apical portions were very much reduced.Microscopic observations revealed that cyanobionts in theseplants were preferentially damaged, with resultant death andlysis. (Received August 2, 1991; Accepted December 27, 1991)     

Pyruvate Uptake by Mesophyll and Bundle Sheath Chloroplasts of a C4 Plant, Panicum miliaceum L.

Intact chloroplasts were isolated from mesophyll and bundlesheath protoplasts of a C₄ plant, Panicum miliaceum L., to measurethe uptake of [1-¹⁴C]pyruvate into their sorbitol-impermeablespaces at 4?C by the silicone oil filtering centrifugation method.When incubated in the dark, both chloroplasts showed similarslow kinetics of pyruvate uptake, and the equilibrium internalconcentrations were almost equal to the external levels. Whenincubated in the light, only mesophyll chloroplasts showed remarkableenhancement of the uptake, the internal concentration reaching10–30 times of the external level after 5 min incubation.The initial uptake rate of the mesophyll chloroplasts was enhancedabout ten fold by light and was saturated with increasing pyruvateconcentration; K_m and V_max were 0.2–0.4 mM and 20–40µmol(mg Chl)^–1 h^–1, respectively. The lightenhancement was abolished by DCMU and uncoupling reagents suchas carbonylcyanide-m-chlorophenylhydrazone and nigericin. Theseresults indicate the existence of a light-dependent pyruvatetransport system in the envelope of mesophyll chloroplasts ofP. miliaceum. The uptake activity of mesophyll chloroplastsboth in the light and the dark was inhibited by sulfhydryl reagentssuch as mersalyl and p-chloromercuriphenylsulfonate, but thebundle sheath activity was insensitive to the reagents. Thesefindings are further evidence for the differentiation of mesophylland bundle sheath chloroplasts of a C₄ plant with respect tometabolite transport. (Received July 3, 1986; Accepted October 8, 1986)     

Cell-Free Synthesis of Rice Prolamin

Polyadenylated RNA was isolated from the protein-body rich fractionof developing rice (Oryza sativa. L) seeds. In a wheat germcell-free system, the isolated polyadenylated RNA produced polypeptideswith the same solubility as prolamin subunits. The electrophoreticmobility of the polypeptides suggested the presence of a signalpeptide. ⁴To whom correspondences should be addressed (Received May 13, 1986; Accepted July 25, 1986)     

Polypeptide Composition of Envelope Membranes Isolated from Chloroplasts of C3, C4, and CAM Plants

Chloroplast envelopes were isolated from chloroplasts purifiedfrom Spinacea oleracea L. (C₃), Panicum miliaceum L. (NAD-malicenzyme-type C₁), Digitaria sanguinalis (L.) Scop. (NADP-malicenzyme-type C₄), Kalanchoe daigremontiana Hamet et Perrier (constitutiveCAM), and from Mesembryanthemum crystallinum L. (inducible CAM)performing either C₃ photosynthesis or Crassulacean acid metabolism(CAM). For each species, methods were developed to isolate chloroplastenvelopes free of thylakoid contamination. The polypeptidesof ribulose bisphosphate (RuBP) carboxylase which has been consistentlyreported in envelope preparations of spinach were not foundin envelope preparations of C₄ mesophyll chloroplasts. Silverstaining of envelope polypeptides resolved electrophoreticallyon sodium dodecylsulfate polyacrylamide gradient slab gels produceda more complex profile than did Coomassie staining which haspreviously been used with C₃ envelope preparations, even thoughsilver reacted poorly with polypeptides corresponding to thesubunits of RuBP carboxylase. All of the plants examined possesseda major polypeptide of 27 to 29 kilodaltons (kD) which was previouslysuggested to be the phosphate translocator in spinach. WithC₃ M. crystallinum, the 29 kD polypeptide stained most intensely.After induction of CAM, a 32 kD polypeptide also stained intensely,giving a profile similar to that obtained with the constitutiveCAM species. A 32 kD polypeptide was also prominent in C₄ envelopepreparations, suggesting that a 32 kD polypeptide may be a translocatorprotein which is required in Crassulacean acid metabolism andC4 photosynthesis, but not in C₃ photosynthesis. (Received April 25, 1983; Accepted July 9, 1983)     

Oligosaccharide profiles of HIV-2 external envelope glycoprotein: dependence on host cells and virus isolates

The glycosylation pattern of the external envelope glycoproteinof human immunodeficiency virus type 2 (HIV-2) was studied independence on host cells and virus isolates. Strains HIV-2_ALT,HIV-2_ROD and HIV-2_D194, differing in their biological propertiesand in the amino acid sequences of their env genes, were propagatedin MOLT4, HUT78 and U937 cells, in human peripheral blood lymphocytesand monocytes/macrophages in the presence of [6-³] glucosamine.Radiolabelled viral glycoproteins were isolated from the cell-freesupernatants and digested with trypsin. Glycans were sequentiallyliberated by endo-ß-N-acetylglucosaminidase H andpeptide-N⁴-(N-acetyl-ß-glucosaminyl) asparagine amidaseF, and fractionated according to charge and size. Comparisonof the oligosaccharide profiles revealed that the envelope glycoproteinsof different virus isolates, propagated in the same host cells,yielded very similar glycan patterns, whereas cultivation ofan isolate in different host cells resulted in markedly divergentoligosaccharide maps. Variations concerned the proportion ofhigh-mannose-, hybrid- and complex-type substituents, as wellas the state of charge and structural parameters of the complex-typespecies. As a characteristic feature, complex-type glycans ofmacrophage-derived viral glycoprotein were almost exclusivelysubstituted by lactosamine repeats. Hence, glycosylation ofthe HIV-2 external envelope glycoprotein seems to be primarilygoverned by host cell-specific factors rather than by the aminoacid sequence of the corresponding polypeptide backbone. envelope glycoprotein glycosylation human immunodeficiency virus type 2     

Structure and Development of Stomata in Some Leptosporangiate Ferns

The structure and development of stomata are described for 17species of leptosporangiate ferns. In these species the maturestomata are anomocytic, diacytic, Pyrrosia(applied), tetracytic,suspended, or floating type. Stomata are present on both surfacesof floating as well as sub merged leaves of Azolla and Marsilea.In a few species twin stomata, arrested development, and persistentstomatal initials are present Floating stomata result from disintegrationof the anticlinal suspending wall in Pleopeltis, and by detachmentand displacement in Azolla pinnata. The development of stomatais haplocheilic, syndetocheilic, or syndetohaplocheilic. InCyathea spinulosa the guard cell nuclei divide amitoticallyand the resulting two daughter nuclei occupy the opposite polesof the guard cells     

Isolation of Chloroplasts from Poteriochromonas malhamensis with the Capacity for Translation

An improved method for the isolation of chloroplasts from Poteriochromonasmalhamensis is described. Poteriochromonas cells were brokenby passage through a nylon mesh with pores of 6µ in diameterat a flow rate of about 5 ml/15 s. After centrifugation thecrude chloroplast fraction was purified by centrifugation ina step gradient of Percoll. The isolated chloroplasts were enclosedby envelope membranes and were still surrounded in part by cytoplasmicresidues. The chloroplasts had the capacity for translation,which was both chloramphenicol-sensitive and cycloheximide-insensitive.The properties of these isolated chloroplasts from Poteriochromonasare discussed in relation to experiments on the transport intothe chloroplasts of nucleus-encoded proteins. ² Present address: Bundesgesundheitsamt, Zulassungsstelle furGentechnologie, Columbiadamm 3, D-1000 Berlin, F.R.G. (Received July 24, 1990; Accepted March 15, 1991)     

Symbiotic algal nitrogenase activity and heterocyst frequency in sevenAzolla species after phosphorus fertilization

Seven species ofAzolla (A. caroliniana, A. microphylla, A. nilotica, A. filiculoides, A. mexicana, A. rubra, A. pinnata the last from both Malaysia and India) grown in pots of flooded soil were subjected to three different treatments with respect to P: none, single application, split application. The experiments were carried out under greenhouse conditions. Heterocyst frequency inAnabaena azollae and acetylene reducing activity (ARA) were studied in successiveAzolla leaves. Both variables increased from the first leaf (shoot apex) to the last one (before branch) in all species in the presence or absence of P. However, heterocyst frequency, ARA andAzolla biomass were all less in the treatment lacking P. Heterocyst frequency inA. azollae, ARA and biomass ofAzolla were higher when P was applied in split doses than in the other treatments.Azolla plants exhibited more ARA than the isolated leaves.     

Effect of Inhibitors of ADP-ribosyltransferase on the Differentiation of Tracheary Elements from Isolated Mesophyll Cells of Zinnia elegans

The effect of m-aminobenzamide (m-ABm) and nicotinamide, inhibitorsof ADP-ribosyltransferase (ADP-RT), on the differentiation oftracheary elements was investigated using isolated mesophyllcells of Zinnia elegans. Both compounds inhibited differentiationwithout affecting cell division, a result which suggests theinvolvement of ADP-RT. The effects of thymidine, a potent inhibitorof ADP-RT and isomers of m-ABm were also examined. (Received September 1, 1986; Accepted January 29, 1987)     

Ferredoxin Isolated from Plant Non-Photosynthetic Tissues. Purficaition and Characterization

A ferredoxin was isolated from non-photosynthetic tissues ofthe lower storage root of radish (Raphanus sativus L. var. acantiformiscultivar Miyashige) in a pure form by conventional means. Itshowed the characteristic features in its absorption spectrumof chloroplast-type ferredoxin. However, amino acid compositionand amino (N)- terminal sequence were different from those ofradish leaf ferredoxin. Root ferredoxin was able to transferelectrons from dithionite to nitrite reductase [EC 1.7.7.1 [EC] ]isolated from mung bean seedling roots and also to mediate NADP⁺photoreduction in spinach broken chloroplasts. It therefore is suggested that a set of distinctive molecularspecies of ferredoxin is present in non-photosynthetic tissuesand functions as a redox mediator in ferredox-independent enzymesystems. (Received October 18, 1985; Accepted January 16, 1986)     

Isolation of Chloroplast DNA from Pinus

Chloroplast DNA isolated from Japanese black pine [Pinus thunbergii)was digested with three restriction endonucleases. The sizeof this DNA was estimated to be 120 kbp. Chloroplast DNA fromJapanese red pine (P. densiflora) could be distinguished fromthat of P. thunbergii by BamHI restriction patterns. ³Present address: Kanto Forest Tree Breeding Institute, Kasahara,Mito, Ibaraki 310, Japan. (Received December 10, 1985; Accepted March 8, 1986)     

TheAzolla-Anabaena association: Historical perspective,symbiosis and energy metabolism

The heterosporous water-fern genusAzolla is one of the few symbioses with a cyanobacterium in the genusAnabaena. TheAzolla-Anabaena association includes six extant speciesof Azolla, which are widely distributed in relatively placid tropical and/or temperate freshwater environments. The earliest mention of the plant seems to be in an ancient Chinese dictionary that appeared about 2000 years ago.Azolla was used in about the 11th century in Vietnam. By 1980 renewed interest in this symbiotic association was shown by the demand for a less fossil energy-dependent agricultural technology. The importation of a variety ofA. filiculoides may have been a most significant breakthrough for the improvementof Azolla cultivation in China. The history of research may be divided into three periods and a new biotechnological stageof Azolla research has recently begun. Each mature dorsal leaf lobe has an ellipsoid cavity which containsAnabaena azollae throughout its development. HeterocystousA. azollae from sixAzolla species share identical and highly specific antigens.Azolla and its endophyte exhibit a coordinated pattern of differentiation and development. Epidermal hair cells of the host are probably interactive with the symbiont. The interior surface of a mature leaf cavity is lined with an envelope and covered by a mucilaginous layer.A. azollae shares the cavity with small populations of the bacteriaPseudomonas andAzotobacter. Endophyte-freeAzolla may rarely occur in nature and can be generated by aseptic techniques.Anabaena azollae can be isolated fromAzolla fronds by gentle pressure and by enzymatic digestion. The free living cultures derived from theAnabaena so obtained differ in some respects, however, from the freshly extracted symbiont, and might better be called the presumptive isolate. BothAzolla andAnabaena contain specific photosynthetic pigments. The optimum conditions for photosynthesis have been measured.Azolla is a C₃ plant and has high net photosynthesis. PSII activity in the symbiont is low. Nitrogenase is localized in the heterocysts of the symbiont and has some advantages compared with free-living cyanobacteria. SymbioticA. azollae has a high frequency of heterocysts. Unidirectional hydrogenase occurs in the symbiont and recycles electrons and ATP. Simultaneous measurements of N₂ fixation and photosynthesis show the dependence of nitrogenase on photosynthetically captured radiation for energy by an indirect dependence on CO₂ fixation. The host contains most of the total GS and GDH activities, and the symbiont excretes a substantial portion of its newly fixed nitrogen as ammonium. The two partners in the association exhibit a comparable developmental gradient and a mechanism of cooperative integration for their energy metabolism, thus improving the efficiency of solar energy conversion and presenting a unique model for biotechnology.     

Cell-Free Synthesis of the Rice Glutelin Precursor

Polyadenylated RNA was directly isolated from developing rice(Oryza sativa. L) seeds. The major translation product of theisolated polyadenylated RNA in a rabbit reticulocyte cell-freesystem was about 2 kDa larger than the in vivo labeled 57 kDaglutelin precursor, and was immunoprecipitated by antiserumagainst the glutelinprolamin fraction of mature seeds. (Received January 27, 1986; Accepted June 23, 1986)     

Cytochrome c' Isolated from Achromobacter xylosoxidans GIFU 1055

Cytochrome c' has been isolated from Achromobacter xylosoxidansGIFU 1055. The absorption spectra of the oxidized and the reducedforms are almost the same as those of cytochromes c' found sofar. The reduced form combines with CO and NO. The hemoproteinis a basic protein and consists of two identical subunits witha molecular weight of 14,000. It is readily autooxidizable withmidpoint redox potential of + 111 mV at pH 7.2. (Received December 2, 1985; Accepted February 20, 1986)     

Some Biochemical Changes Related to Starch Breakdown Induced by Blue Light Illumination and by Addition of Ammonia to Chlorella Cells

Illumination with blue light enhanced the production of ammoniaby cells of C. vulgaris 11h, while no such effect was inducedby red light illumination. Addition of ammonia caused increasesin ATP levels and decreases in Pi and ADP levels. When 5 mMNH₄Cl was added to phosphorylase and amylase isolated from thecells of C. vulgaris 11h, their activities increased about 5–15%and 40–100%, respectively. (Received June 21, 1986; Accepted December 23, 1986)     

The chloroplast envelope of Phaseolus vulgaris L. II. Enzymic characteristics

The isolated chloroplast envelope of Phaseolus vulgaris L. wasfound to synthesize galactolipids when supplied with exogenousUDP galactose. The rate of total galactose incorporation variedwithin the range 0.4-50 nmole g protein^–1 sec^–1with age of the tissues. The activities of NADH dehydrogenase,malate dehydrogenase and Mg²⁺-ATPase in the envelope fractionwere also investigated. The use of a positive "marker" activityfor the isolated chloroplast envelope is considered. ¹Present address: Boyce Thompson Institute, Tower Road, CornellUniversity, Ithaca, NY 14853, USA. (Received March 24, 1980; )