Studies on Plastid-Nuclei (Nucleoids) in Nicotiana tabacum L. I. Isolation of Proplastid-Nuclei from Cultured Cells and Identification of Proplastid-Nuclear Proteins

We have developed a method of isolating morphologically intactproplastid-nuclei (nucleoids) in large quantities from Nicotianatabacum cultured cells (line BY-2) without contamination bymitochondria and cell-nuclei. Fluorescence microscopy using 4',6-diamidino-2-phenylindole(DAPI) revealed that the compact structure of the isolated proplastid-nuclei(pp-nuclei) was disorganized by DNase I, micrococcal nuclease,proteinase K, 2 M NaCl and 2 M KC1, but was not affected byRNase A, suggesting that the pp-nuclei are compactly organizedby an electrostatic interaction between the proplastid- DNA(pp-DNA) and some protein(s). Although SDS-polyacrylamide gelelectrophoresis showed that the isolated pp-nuclear fractionstill contained a number of polypeptides, only four of them(mol wt: 69 kDa, 31 kDa, 30 kDa and 14 kDa) were found to besolubilized by treatments of the pelletable pp-nuclear fractionwith DNase I, micrococcal nuclease and 2 M NaCl. Furthermore,when the supernatant of the pp-nuclei treated with DNase I wasapplied onto a denatured or a native DNA-cellulose affinitycolumn, these four polypeptides were bound to both DNAs andeluted by raising the NaCl concentration. These findings, taken together, show that these proteins areproplastid DNA-binding proteins and strongly suggest that thepp-nuclei are compactly organized by interaction between thepp-DNA and these proteins. ⁴Present address: Department of Biology, Faculty of Science,University of Tokyo, Hongo, Tokyo 113, Japan. ⁵Present address: School of Food and Nutritional Sciences, Universityof Shizuoka, Yata, Shizuoka 422, Japan. (Received August 13, 1987; Accepted November 9, 1987)     

Studies on Plastid-Nuclei (Nucleoids) in Nicotiana tabacum L. IV. Association of Chloroplast-DNA with Proteins at Several Specific Sites in Isolated Chloroplast-Nuclei

When chloroplast-nuclei (cp-nuclei), isolated from tobacco mesophyllprotoplasts, were directly digested by restriction enzymes andanalyzed by agarose gel electrophoresis, the migration of severalrestriction fragments was greatly inhibited during the electrophoresis.When the digested cp-nuclei were treated with SDS and proteinaseK prior to electrophoresis, all the restriction fragments migratednormally and the electrophoretic pattern was the same as thatgenerated by similarly restricted, purified chloroplast-DNA(cp-DNA). Use of a newly developed method, "reciprocal electrophoresis",proved that these fragments were bound so tightly to certainDNA-binding protein(s) that the fragments were trapped in thegel slot. These fragments corresponded to at least four sitesof the cp-DNA. By contrast, when proplastid-nuclei (pp-nuclei)isolated from tobacco cultured cells were analyzed in the sameway, no restriction fragments were trapped in the gel slot.These results, taken together, suggest that a DNA-binding protein(s)is present in cp-nuclei, but not in pp-nuclei, and binds tightlyto the four sites of the cp-DNA. Therefore, the molecular architectureof cp-nuclei is clearly different from that of pp-nuclei. TheDNA-binding protein(s) may have some function(s) specific tocp-nuclei. ⁴ Present address: Department of Biotechnology, Faculty of Technology,Tokyo University of Agriculture and Technology, Nakamachi, Koganei,Tokyo, 184 Japan (Received July 30, 1990; Accepted November 29, 1990)     

Studies on Plastid-Nuclei (Nucleoids) in Nicotiana tabacum L. III. Isolation of Chloroplast-Nuclei from Mesophyll Protoplasts and Identification of Chloroplast DNA-Binding Proteins

We have developed a method of isolating morphologically intactchloroplast-nuclei (nucleoids) in large quantities from mesophyllprotoplasts of Nicotiana tabacum L. cv. Bright Yellow-2. The isolated chloroplast-nuclei (cp-nuclei) were dispersed bythe treatments with proteinase K, 2 M NaCl and 2 M KCL, whichsuggested that the cp-nuclei are compactly organized by an electrostaticinteraction between the chloroplast-DNA and some protein(s).However, the four proplastid DNA-binding proteins identifiedpreviously (Nemoto et al. 1988) were not found in the cp-nuclei,and a different set of DNA-binding proteins (mol wt: 35 kDa,28 kDa and 26 kDa) was detected in the cp-nuclei by a DNA-bindingassay. On the other hand, the chloroplast-DNA was not differentfrom the proplastid-DNA. These findings indicate that the cp-nuclei are constituted fromthe plastid-DNA and the chloroplast-specific DNA-binding proteins.This suggests that the DNA-binding proteins in proplastids aredynamically replaced with the chloroplast DNA-binding proteinsduring the differentiation of plastids from proplastids to chloroplasts.The change of DNA-binding proteins may be involved in the morphologicalchange of plastid-nuclei and/or the regulation of plastid-DNAreplication and gene expression during the differentiation processof plastids. ⁶Present address: Department of Biotechnology, Faculty of Technology,Tokyo University of Agriculture and Technology, Nakamachi, Koganei,Tokyo, 184 Japan ⁷Present address: Department of Biology, Faculty of Science,University of Tokyo, Hongo, Tokyo, 113 Japan (Received April 4, 1990; Accepted May 18, 1990)     

Gibberellin Production in Cultured Cells of Nicotiana tabacum

Endogenous gibberellins (GAs) in several kinds of crown gallcells and cultured cells derived from normal tissue of Nicotianatabacum were systematically analyzed by gas chromatography-selectedion current monitoring (GC-SICM) after chromatographic purifications,and GA₁, GA₉, GA₁₉ and GA₂₀ were identified. Agrobacterium tumefaciens,a pathogen of crown gall, was confirmed not to produce GAs inits culture. We also investigated endogenous GAs of mother plant,tobacco, and found the same kinds of GAs as in cultured cells. ³ Present address: College of Agriculture, Chonnam NationalUniversity, Kwangju 500, Korea. (Received May 19, 1982; Accepted July 22, 1983)     

Cytological and Embryological Studies on Haploid Plant Production from Cultured Unpollinated Ovaries of Nicotiana tabacum L.

We obtained mature haploid (n = 24) ovary plants from in vitro cultured unpollinated young ovaries. These ovaries were induced to form embryoids which then developed into plants. The results obtained are summarized as follows: 1. The origin of development of the ovary haploid plants has been followed by light microscopy. Embryological abservations revealed that there are two ways of plantlet production: (1) Ovary haploid plant was derived from the macrospore without an intervening callus phase. (2) Ovary haploid plant was derived directly from the egg cell of mature embryo sac. In addition, Callus derived haploid plant was also obtained from the base and the tip of a bud of the above mentioned haploid plantlet. In same medium embryoids was derived from callus. Finally, plantlet was developed. 2. The exogenous hormones are necessary for high induction frequency of embryoid from unpollinated isolated young ovary, but these are not definitely necessary for induction of embryonic callus to form embryoids which then developed into plant. 3. The induction frequency of embryoid from in vitro cultured ovary and embryonic callus significantly increased when the concentration of thiamine, pyridoxine, ascorbic acid, nicotinic acid, inositol and folic acid was raised.     

Osmotic Adjustment of Cultured Tobacco Cells (Nicotiana tabacum var. Samsum) Grown on Sodium Chloride

Tobacco cell cultures (var. Samsum) were grown on increasing levels of NaCl to select variants for increased salt tolerance. The osmotic adjustment of NaCl-adapted and nonadapted cell lines was studied. Both cell lines were grown on modified Linsmaier and Skoog medium with or without NaCl. Few differences were found in the response of adapted and nonadapted lines to NaCl.     

Characterization of Polypeptides that Accumulate in Cultured Nicotiana tabacum Cells

We characterized the polypeptides that accumulate in photoautotrophicallycultured cells of tobacco. Microsequencing of these polypeptidesaccumulated in large amounts revealed four NH₂-terminal aminoacid sequences that were highly homologous to those of the knownstress proteins, osmotin and chitinase. Further analyses ofour tobacco cell line grown with sucrose in light and in darkness,as well as analyses of newly established cultured cells andregenerating adventitious shoots, clearly showed that all thein vitro cultured cells accumulated these stress proteins. Theaccumulation of these proteins were also observed in old leaves,roots, and leaves infected with Tobacco Mosaic Virus, but notin young healthy leaves. (Received September 27, 1989; Accepted December 4, 1989)     

烟草未授粉子房胚状体诱导的研究

对烟草（Ｎｉｃｏｔｉａｎａ ｔａｂａｃｕｍ Ｌ．）未授粉子房胚状体的诱导进行了研究,结果发现,胚状体是单细胞起源,起源于大孢子或卵细胞,接种发育早期的子房,胚状体起源于大孢子;接种发育晚期的子房,胚状体起源于卵细胞;接种发育中期的子种,胚状多起源于大孢子,少数起源于卵细胞,不同的基因型,蔗糖浓度及光照强度等对胚状体诱导率的影响亦有不同。     

Sperm dimorphism in Nicotiana tabacum L.

Sperm cells of tobacco have been intensively studied as examples of isomorphic gametes in which major cellular and organellar parameters remain statistically indistinguishable in the two sperm cells. An examination of sperm cells late in maturation, however, displays that the sperm cell associated with the vegetative nucleus becomes statistically significantly smaller than the other sperm cell in tobacco. If late divergence occurs in the two sperms of other angiosperms, sperm dimorphism may be more prevalent than has previously been assumed and dimorphism may have a major influence on the pattern of double fertilization. Received: 15 December 2000 / Accepted: 4 May 2001     

Changes in Composition of Soluble Intercellular Proteins Isolated from Healthy and TMV-Infected Nicotiana tabacum L. cv. Xanthi-nc

Changes in ribonucleases (RNases), phosphomonoesterase (PME), phosphodiesterase (PDE), glucose-6-phosphate dehydrogenase (G6P DH), polyphenoloxidases, peroxidases and proteases activity and PR-proteins composition in leaf tissue and intercellular fluid (ICF) isolated from leaf tissue of healthy and TMV-infected hypersensitive tobacco (Nicotiana tabacum L. cv. Xanthi-nc) plants (non-inoculated leaves) were studied. The amount of the proteins and the enzymes of intercellular space was less than 3 % of the total amount of proteins and the enzymes found in homogenate of healthy leaves. The TMV infection did not significantly change this observation. The great increase in the activities of the enzymes was observed in homogenates of the infected leaves, especially of the enzymes involved in biosynthesis of precursors needed for virus multiplication (G6P DH, RNase, PME, PDE). This is in contrast with the activities of the enzymes of ICF, which were only partly increased. The ICF proteins of infected plants were separated by means of ion exchange chromatography on DEAE cellulose. The isozymes of peroxidase, polyphenoloxidase, PME and PDE were identified. Using discontinuous nondenaturating polyacrylamide gel electrophoresis of DEAE cellulose fractions, the detection of isozymes of peroxidases and PR-proteins was performed. By means of SDS-PAGE the molecular masses of PR-proteins were identified: 15 – 16 kDa (group 1), 27 – 28 kDa (group 3: chitinases) and 36 – 40 kDa (group 2a: -1,3-glucanases).     

Visualization of Membrane Calcium and Calmodulin in Embryo Sacs in situ and Isolated from Petunia hybrida L. and Nicotiana tabacum L.

We have used chlorotetracycline (CTC) and fluphenazine (FPZ)as fluorescent probes to visualize the distributional patternsof membrane calcium (mCa²⁺) and the Ca²⁺-receptor protein calmodulin(CaM) in various cell types of unfixed living isolated and unisolatedembryo sacs of Petunia hydrida L. and Nicotiana tabacum L. Ourresults indicate that in the young embryo sacs of Petunia, bothsynergids and the central cell sequester relatively higher amountsof mCa²⁺ and CaM than the egg cell and the antipodals. Much of the mCa²⁺ in the synergids is polarized in its distributionin that the mCa²⁺ is higher towards the micropylar end of thesynergids. Interestingly, in the mature embryo sacs of Petuniaonly one of the two synergids and the egg cell proper manifesta higher level of mCa²⁺. In vivo only one of the synergids inthe young as well as in the mature embryo sacs if Nicotianaconsistently show higher mCa²⁺. In the mature embryo sacs of Petunia the level of CaM is almostuniform in all the cell types except that one of the synergidsand the three antipodal cells show a slightly higher level ofCaM. The possible implications of these findings in the late eventsof vectorial orientation of pollen tube tip, pollen-tube-synergidinteractions and sperm delivery mechanism are discussed.Copyright1993, 1999 Academic Press Membrane-Ca²⁺, calmodulin, living embryo sacs, Petunia, Nicotiana, pollen tube-synergid interaction     

Amino-acid-transport mutant of Nicotiana tabacum L.

The structure of spinach ribulose 1,5-bisphosphate carboxylase/oxygenase (EC 4.1.1.39) has been investigated by tilted-view electron microscopy of negatively stained monolayer crystals and image processing. The structure determined consists of a cylinder of octagonal cross-section with a large central hole. Based on this and other available evidence a model for the arrangement of the large and small subunits is suggested with the eight small subunits arranged equatorially around the core of eight large subunits.Abbreviations LS large subunit - Rubisco ribulose 1,5-bisphosphate carboxylase/oxygenase - SS small subunit     

Cyanide-Resistant Respiration in Suspension Cultured Cells of Nicotiana glutinosa L

The respiration of dark-grown Nicotiana glutinosa L. cells in liquid suspension culture was found to be highly cyanide resistant and salicylhydroxamic acid (SHAM) sensitive, indicative of an active alternative respiratory pathway. This was especially true during the lag and logarithmic phases of the 14-day growth cycle. Mitochondria isolated from logarithmically growing cells exhibited active oxidation of malate, succinate, and exogenous NADH. Oxidation of all three substrates had an optimum pH of 6.5 and all were highly resistant to inhibited by cyanide and sensitive to SHAM. Respiratory control was exhibited by all three substrates but only if SHAM was present to block the alternative pathway and divert electrons to the phosphorylating cytochrome pathway. The cyanide-resistant oxidation of exogenous NADH has previously only been associated with Arum spadix mitochondria. Coemergence during evolution of the alternative respiratory pathway and the exogenous NADH dehydrogenase in plant mitochondria as a possible mechanism for removal of cytoplasmic NADH is proposed. Evidence is presented which suggests that mitochondrial assays should be performed at pH 6.5.     

Pectin Isolated from the Midrib of Leaves of Nicotiana tabacum

A pectin isolated from tobacco midrib contained residues of d-galacturonic acid (83.7%), L-rhamnose (2.2%), l-arabinose (2.4%) and d-galactose (11.2%) and small amounts of d-xylose and d-glucose. Methylation analysis of the pectin gave 2, 3, 5-tri- and 2, 3-di-O-methyl-l-arabinose, 3, 4-di- and 3-O-methyl-l-rhamnose and 2, 3, 6-tri-O-methyl-d-galactose. Reduction with lithium aluminum hydride of the permethylated pectin gave mainly 2, 3-di-O-methyl-d-galactose and the above methylated sugars. Partial acid hydrolysis gave homologous series of β-(1 → 4)-linked oligosaccharides up to pentaose of d-galactopyranosyl residues, and 2-O-(α-d-galactopyranosyluronic acid)-l-rhamnose, and di- and tri-saccharides of α-(1 → 4)-linked d-galactopyranosyluronic acid residues.

These results suggest that the tobacco pectin has a backbone consisting of α-(1 → 4)-linked d-galactopyranosyluronic acid residues which is interspersed with 2-linked l-rhamnopyranosyl residues. Some of the l-rhamnopyranosyl residues carry substituents on C-4. The pectin has long chain moieties of β-(1 → 4)-linked d-galactopyranosy] residues.     

Photometrically Assayable Phytochrome in vivo in Callus Tissue Cultured from Nicotiana tabacum

Phytochrome was photometrically detected in callus tissue cultured from tobacco stem pith. Our previous work with such tissues showed a growth response to red light, and a nullification of the effect of red by far-red light. Tissues that were subcultured for 4 or 20 months were assayed. Tissues of the younger clone had the most detectable phytochrome. Also, tissues cultured in darkness and those exposed to 5 minutes of red light each day bad more detectable phytochrome than tissues grown under 16-hour photoperiods of low intensity white light. We gratefully acknowledge Drs. H. A. Borthwick and J. E. Scheibe for use of facilities and assistance in operating the dual-wavelength photometer at the U.S.Department of Agriculture Pioneering Research Laboratory for Plant Physiology at Beltsville, Maryland.     

烟草小孢子母细胞减数分裂过程中微管分布变化

应用间接免疫荧光标记技术和激光共聚焦扫描显微镜成像技术观察了烟草小孢子母细胞减数分裂过程中微管的分布变化。在减数分裂前期,小孢子母细胞中的微管较短,随机分散在细胞质中。在减数分裂中期,细胞质中微管形成纺锤体,控制染色体的分布。进入减数分裂I后期,部分纺锤体微管将两组染色体拉向两级。在减数分裂Ⅱ中期,细胞中的微管又形成两个纺锤体。在减数分裂Ⅱ后期,纺锤体微管解聚为微管蛋白分散在细胞质中。胞质分裂发生在四个细胞核形成之后,通过细胞核之间的质膜向内缢缩分隔四个细胞核,产生四个小孢子。     

Adenylate Uptake by Proplastids from Cultured Cells of Tobacco {Nicotiana tabacum L. cv. BY2) Indicates That an Adenylate Translocator is Present in All Types of Plastid

The presence of an adenylate translocator in the envelope membranesof proplastids isolated from the cultured cells of tobacco (Nicotianatabacum L. cv. BY2) was examined by means of transport experimentsusing the silicone oil filtering centrifugation technique. Itwas observed that proplastids can import [³H]ATP, [³H]ADP, [³H]AMPand less specifically ADP-[¹⁴C]Glc which can eventually be usedfor starch biosynthesis. The effects of specific inhibitorsof the mitochondrial adenylate translocator, i.e. atractyloside,bongkrekic acid and carboxyatractyloside were tested. Similarto the case of amyloplasts isolated from the cultured cellsof sycamore and chloroplasts isolated from spinach leaves, onlyATP and ADP-Glc uptake were shown to be partially inhibitedby carboxyatractyloside. On the other hand, neither atractylosidenor bongkrekic acid exerted a significant inhibitory effecton adenylate uptake. (Received August 8, 1992; Accepted November 26, 1992)