Beeinflussung der Anthocyansynthese in Keimlingen von Sinapis alba L. durch α-Methyl-Dl-tryptophan

Summary -methyl-Dl-tryptophan stimulates anthocyanin synthesis in dark grown seedlings of Sinapis alba L. Effective concentrations are between 10^-4 m and 10^-3m. This stimulation is accompanied by an inhibition of root and shoot growth.The induction of anthocyanin synthesis by red light (3×10³ erg cm^-2 sec^-1) is complete after an exposure time of 3 minutes regardless of whether or not the plants were treated with -methyl-Dl-tryptophan.Isonicotinic acid hydrazide inhibits growth of Sinapis alba in a similar manner. It does not affect anthocyanin synthesis.     

Über die Synthese von DNS in den Keimpflanzen von Sinapis alba L.

Summary Seedlings of Sinapis alba were grown under standard conditions. In the hypocotyls and cotyledons DNA synthesis still takes place 36 h after sowing. This synthesis decreases in the following 24 h, but an incorporation of ³H-thymidine was found 108 h after sowing.Autoradiographic studies demonstrate the incorporation of ³H-thymidine into cell nuclei. While some nuclei are homogeneously labelled, in other nuclei the radioactivity appears preferentially or exclusively in the chromocenters.A transfer into the dark of plants previously grown in light (for 24 h or 48 h) does not result in an increase of DNA-synthesis again.     

Sequential control of phytochrome-mediated synthesis de novo of β-amylase in the cotyledons of mustard (Sinapis alba L.) seedlings

In the cotyledons of mustard (Sinapis alba L.) seedlings irradiated from the time of sowing with continuous red light, the photoreversibility of the phytochrome-mediated increase in -amylase activity (EC 3.2.1.2) is lost 36 h after sowing (coupling point). However, the induced increase of -amylase activity cannot be detected before 46 h after sowing (starting point). Density labeling with deuterium oxide shows that the increase of enzyme activity in light and darkness coincides precisely with the synthesis of -amylase protein. Thus, phytochrome mediates an increase of -amylase synthesis de novo. Since there is no turnover detectable by density labeling, it is concluded that -amylase of mustard cotyledons is a physiologically stable enzyme (half-life >5 d). The 10-h time gap between loss of photoreversibility and onset of light-induced -amylase synthesis points to a relatively stable regulatory element within the signal chain (transmitter) which links -amylase synthesis to the primary action of phytochrome. A 12-h lag between the cessation of phytochrome action and the cessation of induced -amylase synthesis indicates a limited lifetime of the transmitter (about 12 h). The effect of this result on the interpretation of the coupling point is discussed.Abbreviations P_r, P_fr red and far-red absorbing forms of phytochrome     

Phytochrome-mediated regulation of β-amylase mRNA level in mustard (Sinapis alba L.) cotyledons

Phytochrome, activated by continuous red light, increases the amount of total polyadenylated RNA during photomorphogenesis of mustard (Sinapis alba L.) cotyledons. In-vitro translation of total polyadenylated RNA in a reticulocyte translation system has shown that the activity of translatable -amylase mRNA is increased by phytochrome about threefold in the 3-d-old cotyledons, based on equal amounts of polyadenylated RNA, and about eightfold on a per-cotyledon basis. Cordycepin prevents the accumulation of translatable -amylase mRNA. It is concluded that the phytochrome-mediated control of -amylase synthesis is exerted on the level of mRNA synthesis. During seedling development in continuous red light, a phytochrome-dependent increase of -amylase mRNA can be observed at least 6 h before the onset of -amylase synthesis. If, after a period of enzyme synthesis, phytochrome action is interrupted by long-wavelength far-red light followed by darkness, -amylase mRNA as well as -amylase synthesis remain at a high level for 8–10 h and then decline sharply. It is concluded that -amylase mRNA, having an apparent lifetime of the order of 8–10 h, can be formed under the influence of phytochrome during early seedling development but it activates -amylase synthesis only after a lag-phase of about 8 h, when the cotyledons acquire competence to synthesize the enzyme. The consequences of these findings for the signal-transduction chain of phytochrome are discussed.Abbreviations EDTA Na₂-ethylenediaminotetraacetic acid - PAGE polyacrylamide gel electrophoresis - poly(A)⁺RNA polyadenylated mRNA - P_r, P_fr red- and far-red-absorbing forms of phytochrome - SDS sodium dodecyl sulfate - Tris 2-amino-2-(hydroxymethyl)-1,3-propanediol     

Pollen—embryogenesis and chromosomal variability in anther culture of Brassica hirta Moench （Sinapis alba L）

The anther cultures of Brassica hirta underwent pollenembryogenesis and callusing,which showed a wide range of chromosome numbers varying from 9 (n=12) to a highly polyploid.For embryogenesis,pretreatment of floral buds in 0.4 M sucrose solution for 72 hrs at 4℃ was superior to freshly cultured anthers.Culture temperature of 30℃ for 14 days before maintenance of cultures at 25℃ was significantly beneficial for embryo yield in comparison to cultures continuously incubated at 25℃.Dark treatment during culture was more effective for pollen-embryo yield.     

Die Wirkung von „Störlicht” auf die Blütenbildung von Sinapis alba L.

Summary The induction of flowering in mustard (Sinapis alba L.) was studied by means of night-breaks (Störlicht). The plants were cultivated under fully controlled conditions: 8000 Lux white light (mixed fluorescent and incandescent) 18°C, 80% relative humidity. Raised under our conditions in short days (8 hours of white light) mustard behaved as a quantitative long-day plant (Fig. 2). Flowering can be promoted by long-day treatment (Fig. 3). The long day (16 hours of white light) can be replaced by a short day plus a night-break. The highest effectiveness of the night-break is found near the middle of the dark period (Figs. 4, 5). —The spectral dependence of flower induction was studied with blue, green, yellow, red (Fig. 1) and far-red light using a 2-hour break near the middle of the dark period. The dose response curves (Fig. 6) and the action spectrum (Fig. 7) indicate a very strong effectiveness in the blue part of the spectrum, a small response in red and yellow light and no response at all in green and far-red light. The participation of phytochrome is indicated (Table 1), but no far-red reversibility could be detected (Table 2). Simultaneous irradiation with red and far-red light yielded significant enhancement effects (Fig. 8). In view of the strong shadowing in the leaves (Figs. 9, 10) these data are interpretable on the basis of phytochrome.     

Mechanism for the Action of λ Exonuclease in Genetic Recombination

Lambda exonuclease degrades in vitro redundant single stranded regions which probably result in λ DNA from genetic recombination in vivo.     

Symmetry-related mutants in the quinone binding sites of the bacterial reaction center – the effects of changes in charge distribution

To probe the structural elements that contribute to the functional asymmetries of the two ubiquinone₁₀ binding pockets in the reaction center of Rhodobacter capsulatus, we targeted the L212Glu–L213Asp (near Q_B) and the M246Ala-M247Ala (near Q_A) pairs of symmetry-related residues for site-specific mutagenesis. We have constructed site-specific mutants that eliminate the sequence differences at these positions (L212Glu–L213AspAla-Ala or M246Ala–M247AlaGlu-Asp), and have reversed that asymmetry by constructing a quadruple-mutant strain, RQ (L212Glu–L213Asp-M246Ala–M247AlaAla-Ala-Gl u-Asp). The mutations were designed to change the charge distribution in the quinone-binding region of the reaction center; none of the strains is capable of photosynthetic growth. In photocompetent phenotypic revertants of the RQ strain, second-site mutations which affect Q_B function are coupled to mutations in the Q_A site which restore an Ala or substitute a Tyr at the M247 site; one strain carries an additional MetLeu substitution at M260 near Q_A. All of the RQ revertants retain the engineered M246AlaGlu mutation in the Q_A site as well as the L212Ala–L213Ala mutations in the Q_B site. Kinetic characterization of the RQ revertants will give us an idea of what structural and functional elements are important for restoring efficiency to electron and proton transfer pathways in the RQ RC, which is far from native. To date, these preliminary results underscore the importance of an asymmetric distribution of polar amino acids in the quinone binding pockets and its influence on the functional properties of the reaction center.     

“Lossless” compression of high resolution mass spectra of small molecules

Fourier transform ion cyclotron resonance (FTICR) provides the highest resolving power of any commercially available mass spectrometer. This advantage is most significant for species of low mass-to-charge ratio (m/z), such as metabolites. Unfortunately, FTICR spectra contain a very large number of data points, most of which are noise. This is most pronounced at the low m/z end of spectra, where data point density is the highest but peak density low. We therefore developed a filter that offers lossless compression of FTICR mass spectra from singly charged metabolites. The filter relies on the high resolving power and mass measurement precision of FTICR and removes only those m/z channels that cannot contain signal from singly charged organic species. The resulting pseudospectra still contain the same signal as the original spectra but less uninformative background. The filter does not affect the outcome of standard downstream chemometric analysis methods, such as principal component analysis, but use of the filter significantly reduces memory requirements and CPU time for such analyses. We demonstrate the utility of the filter for urinary metabolite profiling using direct infusion electrospray ionization and a 15 tesla FTICR mass spectrometer.     

Genetics of the “umbrella” branching habit in Capsicum annuum L.

Summary Three inbred lines, MSU 78-101, MSU 79-221 and MSU 74-230 were used to determine the inheritance of the umbrella branching habit in peppers. MSU 79-221, with the umbrella phenotype, was crossed with MSU 78-191 (dwarf) and MSU 74-230 (indeterminate growth habit). Segregating populations were separated on the basis of plant growth habit and fruit bearing habit. Genetic analyses suggested that the umbrella phenotype was controlled by three major recessive genes, ct and dt determining plant habit, and fa determining fruit bearing habit. When the dominant alleles Dt and Ct were in the dominant homozygous or heterozygous condition an indeterminate phenotype was produced. Su, a dominant suppressor gene, apparently acts to suppress the epistatic action of the Ct gene. Modifiers were involved in the control of branching in the umbrella plants. Linkage also was noted between the genes for indeterminate plant habit and non-clustered bearing habit. The information derived from this study will allow the plant breeder to design an efficient breeding program for the development of pepper cultivars suitable for mechanical harvesting systems.Michigan Agricultural Experiment Station Journal Article No. 11073     

Direct evidence of structural changes in reaction centers of Rb. sphaeroides containing suppressor mutations for Asp L213 → Asn: A FTIR study of QB photoreduction

In bacterial reaction centers (RCs), changes of protonation state of carboxylic groups, of quinone-protein interactions as well as backbone rearrangements occuring upon Q_B photoreduction can be revealed by FTIR difference spectroscopy. The influence of compensatory mutations to the detrimental Asp L213 Asn replacement on Q_B ^–/Q_B FTIR spectra of Rb. sphaeroides RCs was studied in three double mutants carrying a Asn M44 Asp, Arg M233 Cys, or Arg H177 His suppressor mutation. The proton uptake by Glu L212 upon Q_B ^– formation, as reflected by the positive band at 1728 cm^–1, is increased in the Asn M44 Asp and Arg H177 His suppressor RCs with respect to native RCs, and remains comparable to that observed in Asp L213 Asn mutant RCs. Only the Arg M233 Cys suppressor mutation affected the 1728 cm^–1 band, reducing its amplitude to near native level. Thus, there is no clear correlation between the apparent extent of proton uptake by Glu L212 and the recovery of the proton transfer RC function. In all of the mutant spectra, several protein (amide I and amide II) and quinone anion (C...O/C...C) modes are perturbed compared to the spectrum of native RCs. These IR data show that all of the compensatory mutations alter the semiquinone-protein interactions and the backbone providing direct evidence of structural changes accompanying the restoration of efficient proton transfer in RCs containing the Asp L213 Asn lesion.     

Cytoplasmic pH of Root Hair Cells of Sinapis alba Recorded by a pH-sensitive Micro-electrode. Does Fusicoccin Stimulate the Proton Pump by Cytoplasmic Acidification?

Bertl, A. and Felle, H. 1985. Cytoplasmic pH of root hair cellsof Sinapsis alba recorded by a pH-sensitive micro-electrode.Does fusicoccin stimulate the proton pump by cytoplasmic acidification?—J. exp. Bot. 36: 1142–1149. pH-sensitive micro-electrodes, filled with ion-exchanger resinhave been fabricated with a turgorinsensitive tip and have beenapplied to test the intracellular pH and changes thereof inroot hair cells of Sinapis alba. (1) The cytoplasmic pH of Sinapisroot hairs was determined to be 7.3 ±0.2 (at neutralexternal pH). (2) 10 mol m^–3 sodium azide depolarizesthe membrane potential by about 100 mV and acidifies the cytoplasmby 0.8 pH-units. (3) The change from 1.0 mol m^–3 to 10mol m^–3 external potassium causes a depolarization ofabout 45 mV, but no change in internal pH. (4) At an externalpH of 5.0, sodium acetate hyperpolarizes the plasmalemma byabout 60 mV and acidifies the cytoplasmic pH by 0.2 to 0.3 units.(5) 2.0 mmol m^–3 fusicoccin (FC) hyperpolarizes the plasmalemmaby 20–25 mV, acidifies the cytoplasm by 0.1 to 0.2 pH-units,and acidifies the external medium by about 0–3 pH-units.It is concluded that cytoplasmic acidification stimulates theelectrogenic proton pump in Sinapis root hairs, and it is suggestedthat the FC-induced effects, viz. hyperpolarization and externalacidification, can also be interpreted in this way. Key words: —Cytoplasmic pH, pH-sensitive micro-electrode, fusicoccin     

Limitation of C3–CAM shift in the common ice plant under high irradiance

In the halophytic plant Mesembryanthemum crystallinum salinity or drought can change the mode of photosynthesis from C₃ to crassulacean acid metabolism (CAM). These two stress factors are linked to oxidative stress, however, the induction of CAM by oxidative stress per se is not straightforward. Treatment with high light (HL) did not lead to the induction of CAM, as documented by a low night/day difference in malate level and a low expression of the CAM-related form of phosphoenolcarboxylase (Ppc1), despite causing some oxidative damage (elevated MDA level, malondialdehyde). In contrast to the action of high salinity (0.4 M NaCl), HL treatment did not activate neither the cytosolic NADP-malic enzyme nor the chloroplastic form of NADP-dependent malate dehydrogenase (NADP-MDH). In plastids of HL-treated plants a huge amount of starch was accumulated. This was associated with a weak stimulation of hydrolytic and phosphorolytic starch-degrading enzymes, in contrast to their strong up-regulation under high salinity. It is concluded that HL alone is not able to activate starch degradation necessary for CAM performance. Moreover, in the absence of salinity in C₃M. crystallinum plants an age-dependent increase in energy dissipation from PSII was documented under high irradiance, as illustrated by non-photochemical quenching (NPQ). Obtained data suggest that in this halophytic species several photoprotective strategies are strictly salinity-dependent.     

“Primäre” und “Sekundäre” Differenzierung im Zusammenhang mit der Photomorphogenese von Keimpflanzen (Sinapis alba L.)

Zusammenfassung Die Anthocynsyanthese des Senfkeimlings ist phytochromabhängig. Lediglich zwei Gewebe, die Epidermis der Cotyledonen und die Subepidermis des Hypocotyls sind zu dieser Anthocyansynthese fähig. Erst 24 Std nach Aussaat ist Anthocyansynthese möglich und bereits etwa 60 Std nach Aussaat (25° C; Standardbedingungen vgl. Methoden) erlischt dei Fähigkeit zur Anthocyansynthese weitgehend und zwar unabhängig von der Menge des synthetisierten Anthocyans. Die höchste Empfindlichkeit für Licht besitzt das Anthocyan bildende System etwa 36 Std nach Aussaat. — Teilt man den Keimling unmittelbar vor der Anthocyanmessung in 4 Segmente auf (Abb. 9) und mißt den Anthocyangehalt der Segmente getrennt, so stellt sich heraus, daß die Fähigkeit zur Anthocyansynthese im mittleren und basalen Bereich des Hypocotyls rapide verloren geht. Im oberen Hypocotylabschnitt hingegen und in den Cotyledonen nimmt diese Fähigkeit erst zu, und die Abnahme ist langsamer. —Es werden Argumente für die Auffassung entwickelt, daß das spezifische und dynamische Zellmuster, das man hinsichtlich der P₇₃₀-abhängigen Anthocyansynthese vorfindet, ein Ausdruck der primären Differenzeierung sei (vgl. Abb. 4). P₇₃₀ hingegen, so stellen wir uns vor, wirkt unspezifisch im Rahmen einer sekundären Differenzierung, indem es potentiell aktive Gene (P₇₃₀) in Funktion setzt. Welche Gene in den einzelnen Zellen des Dunkelkeimlings potentiell aktiv sind, legt die primäre Differenzierung fest. — Diese Vorstellungen werden durch den Befund gestützt, daß eine Applikation von Actinomycin D zu einer zeitlich sehr viel ausgedehnteren Anthocyansynthese führt; offenbar deshalb, weil die genetisch kontrollierte Entwicklung des primären Differenzie-rungsmusters gebremst wird. Eine Folge wäre, daß die Inaktivierung der zur Anthocyansynthese benötigten Gene, die normalerweise etwa 60 Std nach Aussaat erfolgt, weit hinausgezögert wird.

---

Primary and secondary differentiation in connection with photomorphogenesis of seedlings (Sinapis alba L.)

Summary Anthocyanin synthesis of the mustard seedling (Sinapis alba L.), a typical phytochrome-dependent photoresponse has been further investigated. — It has been found that only two types of tissue can synthesize anthocyanin under the influence of active phytochrome (=P₇₃₀), namely, the epidermis of the votyledons and the subepidermal layer in the hypocotyl (Fig. 2, 3). — Under our standard conditions (25° C; cf. methods) phytochrome-potentiated anthocyanin synthesis is only possible 24 hours after sowing and it ceases about 60 hours after sowing, independent of the amount of anthocyanin which has been accumulated (Fig. 5, 6). On the basis of the whole seedling the highest sensitivity of the anthocyanin producing system to light is around 36 hours after sowing (Fig. 8). Within the tissues which are capable of forming anthocyanin there is a characteristic shift of the ability to respond to P₇₃₀ as the seedling ages. If we devide the seedling into 4 segments (Fig. 9) it turns out that in the basal and middle part of the hypocotyl the ability to form anthocyanin is rapidly lost whereas in the upper part of the hypocotyl and in the cotyledons this ability even increases at first. The following decrease is slower than in the basal parts (Fig. 10, 11).It is argued that this specific and dynamic cellular pattern of responsiveness to P₇₃₀ can be regarded as a manifestation of a primary differentiation in the course of which the genotype of each individual cell in the dark-grownt seedling is devided into 3 functional types of genes: active, inactive, and potentially active genes (P₇₃₀) (Fig. 4). — In connection with anthocyanin synthesis P₇₃₀ is thought to act exclusively at the level of secondary differentiation, i.e., it is thought to initiate the action of potentially active genes via a signal-chain. The action of P₇₃₀ is non-specific. The specificity of the photoresponse of an individual cell is determined by the status of its primary differentiation (Fig. 4).If the process of differentiation is slowed down (e.g. by the application of low doses of Actiomycin D) anthocaynin synthesis can continue much longer than under our standard conditions where it ceases around 60 hours after sowing (Fig. 12). This fact seems to indicate that the loss of the ability to form anthocyanin is due to an inactivation of pertinent genes by the process of primary differentiation, which is itself, as one would expect, under the control of genes.

     

Volume changes and electrostriction in the primary photoreactions of various photosynthetic systems: estimation of dielectric coefficient in bacterial reaction centers and of the observed volume changes with the Drude–Nernst equation

Photoacoustics (PA) allows the determination of enthalpy and volume changes of photoreactions in photosynthetic reaction centers on the 0.1–10 μs time scale. These include the bacterial centers from Rb. sphaeroides, PS I and PS II centers from Synechocystis and in whole cells. In vitro and in vivo PA data on PS I and PS II revealed that both the volume change (–26 A³) and reaction enthalpy (–0.4 eV) in PS I are the same as those in the bacterial centers. However the volume change in PS II is small and the enthalpy far larger, –1 eV. Assigning the volume changes to electrostriction allows a coherent explanation of these observations. One can explain the large volume decrease in the bacterial centers with an effective dielectric coefficient of ∼4. This is a unique approach to this parameter so important in estimation of protein energetics. The value of the volume contraction for PS I can only be explained if the acceptor is the super- cluster (Fe₄S₄)(Cys₄) with charge change from –1 to –2. The small volume change in PS II is explained by sub-μs electron transfer from Y_Z anion to P₆₈₀ cation, in which charge is only moved from the Y_Z anion to the Q_A with no charge separation or with rapid proton transfer from oxidized Y_Z to a polar region and thus very little change in electrostriction. At more acid pH equally rapid proton transfer from a neighboring histidine to a polar region may be caused by the electric field of the P₆₈₀ cation. This revised version was published online in June 2006 with corrections to the Cover Date.     

Use of protoplasts in the improvement of filamentous microorganisms. I. Action of N-methyl-N′-nitro-N-nitrosoguanidine on protoplasts of Streptomycetes

Summary The effects of N-methyl-N–nitro-N-nitroso-guanidine (NTG) on protoplasts of Streptomycetes are markedly different from its action on spores, showing high mutagenic activity even at concentrations having no marked effect on protoplast survival. Strain improvement, eg in chlorotetracycline-producing strains of S. aureofaciens, was most effective when protoplasts were subjected to prolonged treatment (2 h) with low concentrations of NTG (50 /ug/ml).