Isolation and characterization of proteinase inhibitor I from etiolated tobacco leaves

Proteinase Inhibitor I was induced to accumulate in tobacco (Nicotiana tabaccum) leaves by placing plants in darkness for 10 days at 27 degrees C. The inhibitor was isolated using ammonium sulfate precipitation, Sephadex G-75 chromatography, heating, and affinity chromatography with a chymotrypsin-Sepharose column. Inhibitor I was purified 232-fold with a yield of 34 mg from 2.5 kg of leaves. Affinity-purified tobacco Inhibitor I was shown to be homogeneous by gel electrophoresis in both nondissociating and dissociating buffers. The inhibitor has a molecular weight of 39,000 +/- 1000 determined by gel filtration and, like its potato and tomato counterparts, is composed of five subunits of molecular weight 8100. The tobacco Inhibitor I strongly inhibits chymotrypsin and weakly inhibits trypsin. The chemical, physical, and immunological properties of tobacco Inhibitor I indicate that it is structurally very similar to potato tuber Inhibitor I and tomato leaf Inhibitor I, although the synthesis and accumulation of the three inhibitors in their respective tissues are all under different developmental or environmental regulation.     

Plant growth inhibiting properties of diterpenes from tobacco

Certain diterpenes, isolated from various tobacco species andcultivars, inhibited the growth of wheat coleoptiles. The mostactive were sclareol, a mixture of sclareol and epi-sclareol, and rß-4,8,13-duvatriene-1,3-diol, abienol, and labdanediol. (Received December 20, 1976; )     

Saccharopine from tobacco leaves

5-Acetoamino-2-hydroxyvaleric acid, (5-AHV) was metabolized to δ-acetylornithine in tobacco leaves. On the other hand, δ-acetylornithine fed to tobacco leaves was metabolized into at least 5 components, one major component being 5-AHV. These results show that tobacco plant has a reversible metabolic pathway between 5-AHV and δ-acetylornithine.     

Polysomes from expanded tobacco leaves

The isolation of intact polysomes from leaves of tobacco (Nicotiana tabacum L.) is dependent on the age and state of development of leaves. Undegraded polysomes from young leaves in the early stages of expansion can be isolated easily by extracting the leaves in ice-cold extraction buffer (200 mM tris(hydroxymethyl)aminomethylmethane(Tris)-HCl, pH 9.0; 400 mM KCl; 200 mM sucrose; 35 mM MgCl₂). Medium-size leaves give best yields of undegraded polysomes when extractions are carried out in the above buffer and in the presence of ethyleneglycol-bis-(β-amino-ethyl ether)-N,N′-tetracetic acid (EGTA) and mercaptoethanol. Isolation of polysomes from large, nearly fully expanded (mature) leaves requires all of the above plus diethyldithiocarbamate (DIECA) in the extraction medium. An extraction medium consisting of 25 mM EGTA, 0.01 M mercaptoethanol, 25 mM DIECA and 0.5% of the nonionic detergent, Nonidet-P40 (NP 40) was found to be very suitable for extraction of polysomes from all developmental stages of leaves. The polysomes extracted in the above medium showed active translation of protein in the wheat-germ in-vitro protein-synthesizing system. The translational products were similar when translations were carried out directly with polysomes or polysomal RNA, or polysomal poly(A)⁺ RNA from tobacco leaves. Poly(A)^? polysomal RNA was a poor template in the in-vitro wheat-germ system.     

Extraction,partial purification,and properties of a mycoplasmal growth inhibitor extracted from cells ofMycoplasma by ultrasonication

Inhibition of growth ofMycoplasma, but notAcholeplasma, by a substance extracted from mycoplasmal cells by ultrasonication (us-Mcin) was demonstrated. All species ofMycoplasma tested having the growth inhibitor also had arginine deiminase and, except forM. fermentans, those without the inhibitor lacked arginine deiminase. The grade of inhibiting activity was in parallel with that of arginine deiminase. However, the us-Mcin entity is not arginine deiminase itself, because us-Mcin was still active after treatment withp-chloromercuribenzoic acid, which is an inhibitor of the enzyme. The effect of us-Mcin on the growth ofMycoplasma is not mycoplasmastatic but mycoplasmacidal. The us-Mcin obtained from cells ofM. salivarium was partially purified by column chromatography after DNase treatment and was characterized as follows: nondialyzable; heat labile; pH stable between 5 and 9; iactivated by methanol, but insensitive to acetone as well as chloroform; completely or partially inactivated by pronase, trypsin, chymotrypsin, and RNase, but insensitive to phospholipase C and DNase; contained no detectable protease or lipase, but did have a detectable amount of arginine deiminase. The molecular weight of partially purified us-Mcin ofM. salivarium determined by SDS-polyacrylamide gel electrophoresis might be 46,000. Differences between the spectra of growth inhibition by growth inhibitors extracted with chloroform (ch-Mcin) and the spectra of inhibition by us-Mcin are discussed.     

Chloroplastic glutamine synthetase from tobacco leaves: a glycosylated protein

The amino acid and carbohydrate content of chloroplastic glutamine synthetase from tobacco leaves has been analysed. The enzyme subunit contanins 5% carbohydrate, mainly represented by glucosamine, galactosamine, glucose, galactose and mannose residues. The enzyme subunit displayed a single band of molecular mass 44000 Da after sodium dodecyl sulphate (SDS) electrophoresis. However, when isoelectrofocussing electrophoresis was performed, four subunits were evident differing by their charge. Furthermore, the four different subunits stained positively when tested with periodic acid Shiff reagent, showing that sugars and amino sugars were present within all the subunits.     

Plant regeneration from immature embryos of peanut

Plant regeneration from immature embryos of peanut (Arachis hypogaea L.) can be accomplished through somatic embryogenesis. The highest frequency of somatic embryo formation occurred on B5 medium plus 0.5–1.0 mg/l picloram. Shoots and plants developed from the somatic embryos only after extended culture on basal medium. Shoots were excised from thick embryonic roots and rerooted on Murashige and Skoog medium containing half the normal concentration of inorganic salts. This technique should be useful for the production of interspecific hybrid plants from immatureArachis embryos.     

烤后不同霉变程度烟叶际真菌群落组成与多样性分析

【目的】为了解烤后不同霉变程度烟叶真菌群落组成与多样性。【方法】基于IlluminaMiSeq高通量测序平台对烤后烟叶叶柄和叶片叶际样品的真菌群落组成进行了分析。【结果】霉变重烟叶叶片(BQ)、霉变重烟叶叶柄(BZ)、霉变轻烟叶叶片(JQ)、霉变轻烟叶叶柄(JZ) 4类样品真菌分布于子囊菌门(Ascomycota)、担子菌门(Basidiomycota)、接合菌门(Zygomycota)等7个菌门、27个纲、58个目、104个科、171个属的360个真菌分类单元(OTUs)。不同霉变程度烟叶叶际真菌群落组成、分类单元的相对丰度及优势分类单元皆存在不同程度差异。在属的水平上,霉变重烟叶叶片(BQ)的优势菌属为Aspergillus (89.64%)、Myrothecium (2.54%)、Rhodotorula (2.48%)、Gibberella (1.49%);霉变重烟叶叶柄(BZ)的优势菌属为Aspergillus(96.93%)和Alternaria(1.92%);霉变轻烟叶叶片(JQ)的优势菌属为Aspergillus(40.13%)、Rhodotorula(31.81%)、Alternaria(16.75%);霉变轻烟叶叶柄(JZ)的优势菌属为Aspergillus (62.77%)、Alternaria (9.74%)、Rhodotorula (5.20%)。【结论】霉变轻烟叶叶片样品真菌群落的多样性最高,霉变轻烟叶叶柄的真菌群落丰富度最高。霉变重烟叶样品的叶片部位的真菌群落丰富度和多样性均高于叶柄。烟叶霉烂为烤房常见病害,其病原真菌种类多样,且广泛分布于烟叶和环境中。该研究结果为烤房烟叶霉烂病的防治可根据不同发病程度的不同部位的真菌群落构成特征,制定相应的防治方案提供了参考依据。     

Potassium requirement of pyruvate kinase extracted from leaves of halophytes

Pyruvate kinase enzymes were partially purified from leaves of halophytes, Atriplex gmelini C. A. Mey., Chenopodium acuminatum Wild, and Spergularia salina J. et C. Presl., grown hydroponically in the presence of 250 m M NaCl in a greenhouse, to determine their K_m values for potassium. The values were all ca 10⁻³ M , as also reported for the glycophyte enzymes. However, the K_m values were reduced by 60 to 70% by the addition of betaine to a concentration of 1 M .     

Polyribosomes in protoplasts isolated from tobacco leaves

Polyribosomes (polysomes), active in an amino acid incorporation system in vitro, were isolated from tobacco leaf protoplasts. A comparison of polysome profiles indicated that the polysome/monosome ratio is greatly decreased in isolated protoplasts as compared to the intact leaf. In isolated protoplasts, a marked accumulation of ribosomal subunits was also found. The division of protoplasts, as investigated in the 8-cell and callus stages, was associated with a(n) (at least) partial regeneration of polysome profiles characteristic for leaves. Plasmolysis of leaves attached to the plant had no great effect on the polysome profile. However, leaf excision per se resulted in a dramatic loss of polysomes, even when the leaf tissue was floated on water. It is concluded that the isolation of the cell from its normal environment, and not the osmotic stress and associated increase in RNase activity, is the most important factor responsible for the loss of polysomes in isolated protoplasts.Abbreviations EGTA ethylene glycol bis (2-aminoethyl ether)-tetraacetic acid - HEPES N-2-hydroxyethylpiperazine-N-2-ethanesulfonic acid - mRNA messenger ribonucleic acid - RNase ribonuclease - Tris tris(hydroxymethyl)aminomethane - TCA trichloroacetic acid     

A cytokinin-binding protein complex from tobacco leaves

A cytokinin binding protein complex (CBP130) has been purified from tobacco leaves (Nicotiana sylvestris). It contains two protein species of 57 and 36 kDa (CBP57 and CBP36). The cDNAs encoding CBP57 have been isolated from a tobacco cDNA library. Their predicted amino acid sequences showed significant homology between CBP57 and S-adenosyl-L-homocysteine (SAH) hydrolase, which catalyzes the reversible hydrolysis of SAH, a methyltransferase inhibitor. A combination of gel filtration an western blot analysis revealed that both CBP57 and benzyladenine (BA)-binding activity were eluted at a peak of 130 kDa. A purified CBP130 fraction contains SAH hydrolase activity. We discuss possible CBP57 as a cytokinin receptor subunit and its possible role as a regulator of methylation.     

Isolation and characterization of a protease inhibitor from spinach leaves

An acid-stable and heat-labile proteinous protease inhibitor which was found in spinach leaves but not in seeds was isolated by sequential chromatography and preparative isoelectric focusing. The isoelectric point of this inhibitor was 4.5. The inhibitor had a M_r of ca 18 000 and was rich in aspartic acid and glycine; it had 4 half-cystine, 2 tryptophan and no methionine residues. Its extinction coefficient (E|_cm^%) was 13.7 at 280 nm. The inhibition was competitive and the dissociation constant was 3.32 × 10^?13 M. The inhibitor was specific to serine proteases and strongly inhibited trypsin and weakly inhibited α-chymotrypsin and kallikrein.     

Plasma cholesterol-lowering effect on rats of dietary fiber extracted from immature plants

Crude dietary fiber samples were prepared from beet, cabbage, Japanese radish, onion and mung bean sprouts (BF, CF, RF, OF and MF, respectively). These samples contained total dietary fiber at the levels of 814, 699, 760, 693 and 666 g/kg, respectively. To examine the effect of these dietary fiber sources on the plasma cholesterol concentration, male Sprague-Dawley rats were fed on a fiber-free (FF) diet or on an FF diet supplemented with 5% or 10% dietary fiber. Dietary fiber extracted from vegetables, wood cellulose (CL), pectin (PE) and guar gum (GG) were used as the fiber sources. Compared with the rats fed on the FF diet, a significant reduction in the plasma cholesterol concentration was observed in the rats fed on BF, CF, RF, MF, PE or GG after a 21-d feeding period. Cecal acetate, n-butyrate and total short-chain fatty acids were significantly higher in the rats fed on these dietary fibers, except for CF, than in those fed on the FF diet. A negative correlation was apparent between the total dietary fiber content, hemicellulose content and pectin content of each dietary fiber source and the plasma cholesterol concentration. These results suggest that some vegetable fibers exert a plasma cholesterol-lowering effect through cecal fermentation of these fibers.