Fluorescence of 3-keto-steroids in aqueous solution

The physiologically important 3-keto-steroids are non-fluorescent or only weakly fluorescent in protic as well as in aprotic solvents. In contrast, the 4,6,8(14)-triene-3-one steroids are highly fluorescent in aqueous solution but they do not appreciably fluoresce in other solvents. Evidence is presented that the introduction of double bonds into the skeleton of the 3-keto-steroids leads to a decrease of the energy of the lowest – ^* state, bringing this level into the neighbourhood of the non-fluorescent n – ^* state. As a consequence, for two states of approximately the same energy, relatively small perturbations such as those due to solvent interactions, protein binding and micelle formation, will then determine whether a system will fluoresce ( – ^* state lowest) or not (n – ^* state lowest). When the fluorescent 3-keto-steroids, having three conjugated double bonds, bind to proteins, the fluorescence intensity becomes almost zero, making these compounds useful as probes for steroid-protein interactions. This quenching of the fluorescence is explained by a decrease in energy of the n – ^* state relative to the – ^* state of the steroids due to hydrophobic interactions with the proteins.Abbreviations 6,8-BDT 6,8-bisdehydrotestosterone; DMSO, dimethylsulfoxide - HPLC high pressure liquid chromatography This work was presented in part at the Annual Meeting of the Gesellschaft für Biologische Chemie, September 26–29, 1983, in Göttingen. For an abstract see: Hoppe-Seyler's Z. Physiol. Chem. (1983) 364: 1151–1152Dedicated to Prof. Dr. F.-W. Zilliken on the occasion of his 65th birthday     

Cell-wall tension of the inner tissues of the maize coleoptile and its potential contribution to auxin-mediated organ growth

Plant organs such as maize (Zea mays L.) coleoptiles are characterized by longitudinal tissue tension, i.e. bulk turgor pressure produces unequal amounts of cell-wall tension in the epidermis (essentially the outer epidermal wall) and in the inner tissues. The fractional amount of turgor borne by the epidermal wall of turgid maize coleoptile segments was indirectly estimated by determining the water potential ^* of an external medium which is needed to replace quantitatively the compressive force of the epidermal wall on the inner tissues. The fractional amount of turgor borne by the walls of the inner tissues was estimated from the difference between -^* and the osmotic pressure of the cell sap (_i) which was assumed to represent the turgor of the fully turgid tissue. In segments incubated in water for 1 h, -^* was 6.1–6.5 bar at a _i of 6.7 bar. Both -^* and _i decreased during auxin-induced growth because of water uptake, but did not deviate significantly from each other. It is concluded that the turgor fraction utilized for the elastic extension of the inner tissue walls is less than 1 bar, i.e. less than 15% of bulk turgor, and that more than 85% of bulk turgor is utilized for counteracting the high compressive force of the outer epidermal wall which, in this way, is enabled to mechanically control elongation growth of the organ. This situation is maintained during auxin-induced growth.Abbreviations and Symbols _i osmotic pressure of the tissue - ₀ external water potential - ^* water potential at which segment length does not change - IAA indole-3-acetic acid - ITW longitudinal inner tissue walls - OEW outer epidermal wall - P turgor Supported by Deutsche Forschungsgemeinschaft (SFB 206).     

A novel pollen-specific α-tubulin in sunflower: structure and characterization

We describe here a new -tubulin isoform from sunflower we named -tubulin. -tubulin is the most divergent higher-plant -tubulin described so far, having an unusual deletion in the H1/B2 loop and a glutamine-rich C-terminus. We constructed a three-dimensional model and discuss its implications. Using specific antibodies, we show that -tubulin expression is restricted to the male gametophyte. -tubulin mRNA represents 90% of -tubulin mRNA and a small percentage of total pollen mRNA. Among the plants tested, -tubulin was only detected in sunflower and in Cosmos. Since both plants are Asteraceae, we propose that -tubulin is specific to this family. Our results suggest that -tubulin can inhibit tubulin assembly in pollen. This hypothesis is reinforced by the fact that -tubulin is found in a complex with -tubulin in mature sunflower pollen.     

Identification of a glutathione-S-transferase effector domain for inhibition of jun kinase, by molecular dynamics

We have recently found that the glutathione-S-transferase -isozyme (GST-), a cellular detoxification enzyme, potently and selectively inhibits activation of jun protein by its upstream kinase, jun kinase (JNK). This newly identified regulatory activity of GST- is strongly inhibited by a group of agents that inhibit its enzymatic activity. Since loss of enzymatic activity in general does not correlate with loss of regulatory activity, it is likely that inhibitor binding induces changes in the structure of one or more domains of GST that block its interaction with JNK. To identify regions of GST that change conformation on the binding of inhibitors, we have performed molecular dynamics calculations on GST- to compute its average structure in the presence and absence of the inhibitor, glutathione sulfonate. Superposition of the two average structures reveals that several regions change local structure depending upon whether the inhibitor is bound or not bound. Two of these regions, residues 36–50 and 194–201, are highly exposed. We have synthesized peptides corresponding to these two segments and find that the 194–201 sequence strongly inhibits the ability of GST- to block the in vitro phosphorylation of jun by JNK. These results suggest that this region of GST- is critical to its functioning as a newly discovered regulator of signal transduction.     

Does glutathione S-transferase Pi (GST-Pi) a marker protein for cancer?

Glutathione S-transferases (GSTs, EC 2.5.1.18) are multifunctional and multigene products. They are versatile enzymes and participate in the nucleophilic attack of the sulphur atom of glutathione on the electrophilic centers of various endogenous and xenobiotic compounds. Out of the five, , and , major classes of GSTs, GST- has significance in the diagnosis of cancers as it is expressed abundantly in tumor cells. This protein is a single gene product, coded by seven exons, that is having 24 kDa mass and pI value of 7.0. Four upstream elements such as two enhancers, and one of each of AP-1 site and GC box regulate gene. During chemical carcinogenesis because of jun/fos oncogenes (AP-1) regulatory elements, specifically GST- is expressed in liver. Therefore this gene product could be used as marker protein for the detection of chemical toxicity and carcinogenesis.     

Effects of moisture stress on the multiplication and expansion of cells in leaves of sugar beet

Summary Sugar beets were subjected to moisture stress by decreasing the water potential of the culture solution osmotically with polyethylene glycol by a known amount, , and, alternatively by applying matric potential, , at the plant roots. Lowering the water potential at the root surface less than 200 millibars by either method resulted in significant decreases in the rate of cell multiplication. The final number of cells per leaf at = -372 mb the final was 165% of that at = -473 mb ( = –101 mb); similarly at = –15 mb the final cell number was 198% of that at = –196 mb ( = –181 mb). The mean cell volume of leaves was not significantly affected by these levels of moisture stress.     

Water relations and growth of three grasses during wet and drought years in a tallgrass prairie

Summary The water relations and growth of three tallgrass prairie species Panicum virgatum, Andropogon gerardii and A. scoparius were examined in irrigated and unwatered prairie in eastern Kansas (USA). Measurements of the osmotic potential at full turgor, ¹⁰⁰ , at zero turgor, ⁰, and growth of vegetative and reproductive tillers were made in a year with above-normal precipitation and a drought year to evaluate: 1) the ability of these grasses to osmotically adjust in response to water stress and 2) the effect of drought or supplemental water on growth of these species. Although these grasses adjusted osmotically even in the wet year, the degree of adjustment of ¹⁰⁰ and ⁰ in the drought year was relatively large (0.60–0.78 MPa and 0.88–1.34 MPa, respectively) compared to reports for other species. Seasonal minimum values of ¹⁰⁰ and ⁰ for these grasses in the drought year were lower than in most mesic species and seasonal fluctuations in ¹⁰⁰ and ⁰ were greater than reported for most mesic or xeric species. The relatively frequent occurrence of drought in sub-humid tallgrass prairies may partially explain the greater than expected magnitude of osmotic adjustment in these grasses.Irrigation in the wet year increased reproductive biomass in the mesic grass P. virgatum, but had no effect on A. gerardii or the more xeric grass A. scoparius. However, irrigation in the drought year increased maximum shoot biomass in all three grasses significantly with the largest increase in P. virgatum. Reproduction in P. virgatum was also increased more by irrigation in the drought year compared to the other grasses. Irrigation did not increase season's end production of A. gerardii in the wet year, but in the drought year production was 28% greater in irrigated than unwatered prairie. The combination of these water relations and growth responses of the three grasses to wetter than normal and drought years supports their reported distribution along a moisture gradient in tallgrass prairies.     

UV-Spektren und Elektronenstrukturen von Monoamino-Acridinium-Kationen

Zusammenfassung Es wurden die UV-Spektren und die Fluoreszenzanisotropie der 1-, 2-, 3- und 4-Amino-Acridinium-Kationen gemessen und mit Hilfe nach PPP berechneter Anregungsenergien, Übergangsmomente und Polarisationen gedeutet. Die Rechnungen liefern die Elektronenstrukturen der Grund- und Anregungszustände (-Bindungsordnungen und -Elektronendichten). Die Elektronenanregungen der Kationen sind über diejenigen der nicht ionisierten Basen mit denen des Kohlenwasserstoffs Anthracen als Grundkörper zu korrelieren. Der Einfluß von Wasserstoffbrückenbindungen auf die Spektren wird diskutiert. Wir danken der D. F. G. und den Rechenzentren in Darmstadt und Freiburg.

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UV-spectra and -electronic structures of monoamino-acridinium cations

Summary The electronic-excitation and polarisation-spectra of 1-, 2-, 3- and 4-amino-acridinium cations were measured. Transition energies, -electronic densities and -bond orders have been calculated by a -variable SCF-method within the general PPP-framework; the effect of H-bond formation upon their electronic spectra is examined and attempts are being made to correlate the computed transitions of the monoamino-acridinium cations with those of the corresponding non-ionized bases and with anthracene.

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Wir danken der D. F. G. und den Rechenzentren in Darmstadt und Freiburg.     

Vacuolar and cytoplasmic pH,ion composition,and turgor pressure in Lamprothamnium as a function of external pH

Ionic responses to alteration in external and internal pH were examined in an organism from a marine-like environment. Vacuolar pH (pH^v) is about 4.9–5.1, constant at external pH (pH^o) 5–8, while cytoplasmic pH (pH^c) increases from 7.3 to 7.7. pH^c regulation fails above pH^o 9, and this is accompanied by failure of turgor regulation. Na⁺ increases above pH^o 9, while K⁺ and Cl^– decrease. These changes alone cannot however explain the alterations in turgor. Agents known to affect internal pH are also tested for their effect on ion relations.Abbreviations C_i ion concentration - CCCP carbonyl cyanide m-chlorophenyl hydrazone - DCCD dicyclohexylcarbodiimide - DES diethylstilbestrol - DMO 5,5-dimethyloxazolidine-2,4-dione - DNP 2,4-dinitrophenol - pH^o external pH - pH^c cytoplasmic pH - pH^v vacuolar pH - ⁱ osmotic pressure - turgor pressure     

Kinetics of growth and lactic acid production in continuous and batch culture

Summary In a lactic acid fermentation by Streptococcus faecalis, the specific consumption rate of glucose (v) and the specific production rate of lactic acid () were represented by the following simple equations as functions of the specific growth rate (): 1/=(1/) + 1/ = (1/) + By use of data from a batch culture, these two equations were derived from enzyme kinetics of the product inhibition. These equations were successfully applied to the results of batch culture and chemostat culture. In addition, calculation of ATP yield by these equations agreed with the experimental results better than the conventional Leudeking-Piret type equation, which includes two terms associated with growth and not with growth. Correspondence to: H. Ohara     

Expression in Saccharomyces cerevisiae of a gene associated with cytoplasmic male sterility from maize: Respiratory dysfunction and uncoupling of yeast mitochondria

Summary The replication initiation protein of the Escherichia coli plasmid R6K is a dual regulator in the control of plasmid copy number, functioning both as a specific initiator and inhibitor of replication. While the biochemical basis of these activities is not known, initiator activity requires binding of the protein to the seven 22 by direct repeats within the -origin region. By deleting C-terminal segments of the coding region, we have found that the N-terminal polypeptides of that are produced, corresponding to the first 117 and 164 amino acids, respectively, retain the negative activity of the bifunctional protein, i.e. these truncated proteins specifically inhibit R6K replication in vivo. These negatively acting polypeptides, however, are incapable of initiating replication in vivo and fail to bind to the -origin of the R6K DNA in vitro. A correspondence between the observed negative activity of the N-terminal peptide and the negative regulatory activity of the intact protein is supported by the finding that point mutations introduced into the 164 amino acid N-terminal peptide that result in a decrease in its inhibitory activity also produce a plasmid high-copy phenotype when these mutations are incorporated into the full-length protein. These findings demonstrate that the negative domain of resides in the N-terminal segment of the protein. Furthermore, the data obtained suggest that inhibition of R6K replication by does not require direct binding to DNA.     

Chloroplast acclimation to low osmotic potential

Photosynthetic potential of isolated chloroplasts was investigated during in situ water deficits. An eight day stress cycle imposed on spinach plants reduced leaf _w by 0.57MPa, and leaf by 0.50MPa, resulting in partial turgor maintenance during the stress cycle. Pressure/volume curves confirmed the occurrence of osmotic adjustment. Leaf depression was associated with an altered response of chloroplasts to low in vitro. Optimum reaction medium for photosynthesis shifted from –1.04 to –1.57MPa, and low was not as inhibitory to photosynthesis of plastids pre-exposed to stress in situ. These data indicate that chloroplasts acclimate to low external in response to leaf water deficits. This response was still evident four days after a stress cycle ended, but was nearly reversed eight days after stress. Repeated stress cycles in situ did not increase the degree of chloroplast acclimation to low in vitro. Fast dehydration of leaves did not induce this apparent chloroplast acclimation.Abbreviations osmotic potential - _w water potential - PEG polyethylene glycol 8000 - MPa megapascals     

Pre-clinical studies of the negative pi-meson beam at TRIUMF

Summary The ^– flux from the biomedical channel at TRIUMF increases with increasing channel momentum, while the contaminating electron flux decreases. Since the electrons appear to result from conversion of the high energy-rays produced by ⁰ decay in the production target, the electron contamination can be reduced further by target configurations which minimize gamma conversion.The attenuation of ^– beams by in-flight interactions was found to decrease from an initial value of 1.67 ± 0.02 % per g/cm² at zero depth to 1.48 ± 0.02 % per g/cm² near the stopping peak.The inactivation of cultured CHO cells by an extended-peak ^– dose distribution has been measured using the gel technique. The survival data have been fitted by a model which characterizes the physical quality of the dose profile by means of measured star densities. This model provides a convenient method of analysis for large sets of survival data and may be useful for prediction of the biological effect of new ^– dose distributions.The RBE value for 50% survival measured at the centre of a 7 cm extended peak was found to be approximately 1.4, in reasonable agreement with recent values obtained at LAMPF and SIN.     

The double ππ5.6 helix of gramicidin a predominates in unsaturated lipid membranes

The structure of the channel-forming polypeptide gramicidin A (GA) incorporated into phosphatidylcholine (PC) liposomes has been studied as a function of the degree of unsaturation of the acyl chains of PC. The initial conformational state of GA in reconstituted bilayers is determined by the solvent in which the peptide and the lipid are initially co-dissolved, whereas the equilibrium conformational state (after heat incubation) is affected by the lipid structure rather than by the nature of the solvent. The conformational equilibrium of GA has been studied in liposomes prepared from PC having a variable number of double bonds in the fatty acid moiety, by circular dichroism and Fourier transform infrared. Liposomes were prepared from trifluoroethanol or ethanol solutions and incubated at 68°C. GA was shown to retain the conformation of the right-handed .3 .3 helix in PC with saturated acyl chains and with one double bond, whereas in dilinoleoyl-PC, having two double bond in each chain, the thermodynamically preferred structures are left-handed antiparallel and parallel double 5.6 helices. Natural soybean PC also favours left-handed 5.6 helical structures of GA (75%). This finding is discussed in terms of the role of PC unsaturation in the dynamic properties of the lipid matrix. Differences between observed FTIR spectra of the =5.6 helix in solution (and to a larger extent in the membrane) and the calculated IR spectra can be interpreted as resulting from deviation of the real structure from the theoretically derived ideal helix. The data obtained provide grounds for better understanding of a GA channel functioning in lipids of variable degrees of unsaturation.Abbreviations GA gramicidin A - CD circular dichroism - FTIR Fourier transformed infrared - 2D-NMR two-dimensional nuclear magnetic resonance - DSPC distearoylphosphatidylcholine (di-C18:0) - DPPC dipalmitoyl-PC (di-C16:0) - DMPC dimiristoyl-PC (di-C14:0) - POPC palmitoyloleyl-PC (C16:0-C18:1) - DOPC dioleyl-PC (di-C18:1) - DLPC dilinoleoyl-PC (di-C18:2) - TFE trifluorethanol - SDS sodium dodecylsulfate - TMA-DPH 1-[4(trimethylammonio)-phenyl]-6-phenyl-1,3,5-hexatriene - HPLC high-performance liquid chromatography Correspondence to: V.T. Ivanov     

1H-filtered correlation experiments for assignment and determination of coupling constants in backbone labelled proteins

The implementation of [¹³C,¹³C,¹⁵N,²H] labelled amino acids into proteins allows the acquisition of high resolution triple resonance experiments. We present for the first time resonance assignments facilitated by this new labelling strategy. The absence of ¹J_C,C couplings enables us to measure ¹J_C,C scalar and ¹D_C,C residual dipolar coupling constants using modified HNCA experiments which do not suffer from sensitivity losses characteristic for ¹³C constant time experiments.     

A method for the investigation of those transformations under which the visual recognition of a given object is invariant

An experiment is described which shows in operation the program set out in Foster (1972a) for the investigation of the invariance transformations of visual recognition. The concern in the present study is with the Lie group of rotations SO(2), and a certain centrally located foveal Landolt ring. By presenting to the visual system this Landolt ring and a rotated image in rapid succession, one attempted to induce a specified rotation-type phi-motion. Two subjects were employed. Both reported the existence of the required type of phi-motion for rotations ₀ of the Landolt ring about the visual axis with -2/72/7. By appealing to the basic Proposition 2 of Foster (1972 a), the conclusion is reached that the visual system appears capable of effecting upon a certain centrally located foveal annulus the local 1-parameter group of rotations about the visual axis ₀, [–2/7,2/7].     

Visualization ofπ − andπ + stopping density distributions in one and two dimensions

Summary A technique suitable for mapping ^± stopping density distributions in patients or phantoms is described. As a position sensitive detector a multiwire proportional chamber with a slit or a hole collimator in front was applied. Results using a water and a Rando phantom are presented for various momenta and momentum band widths of the ^± beam. To our knowledge the two-dimensional visualization of a ^– stopping density distribution was realized for the first time.     

Diagnosing lactic acid fermentation based on specific rates of growth,substrate consumption and product formation

The on-line calculated specific rates of growth, substrate consumption and product formation were used to diagnose microbial activities during a lactic acid fermentation. The specific rates were calculated from on-line measured cell mass, and substrate and product concentrations. The specific rates were more sensitive indicators of slight changes in fermentation conditions than such monitored data as cell mass or product concentrations.List of Symbols 1/h specific rate of cell growth - 1/h specific rate of substrate consumption - 1/h specific rate of product formation - ^* dimensionless specific rate of cell growth - ^* dimensionless specific rate of substrate consumption - ^* dimensionless specific rate of product formation - _max 1/h maximum specific rate of cell growth - _max 1/h maximum specific rate of substrate consumption - _max 1/h maximum specific rate of product formation - X g/l cell mass concentration - S g/l substrate concentration - S ^* dimensionless substrate concentration - S ₀ g/l initial substrate concentration - P g/l product concentration     

A two-dimensional gas of interacting electric dipoles with hard cores: Van der Waals isotherms and their possible application in lipid phase transitions

We calculate the thermodynamic properties of a two-dimensional fluid of hard disks with embedded dipoles. Our attention is centered on the isotherms in the neighborhood of the critical point. Evaluating the canonical partition function by the "factor cluster expansion", we exhibit the Van der Waals loops obtained considering the exact two-body clusters and the "hard core" contribution of the three-body clusters. The Van der Waals isotherms can be scaled as universal functions of the parameter =p²/4r ₀ ³ kT, where p, r₀, , are the dipole moment, hard core radius, and permittivity which characterize the interaction. The model is applied to the lipid phase transition found in natural and synthetic membranes. The typical critical parameters (T_c300K, _C50 dyne/cm) reflect a physically reasonable value for the dipole moment of a polar head group of a lipid but a much-too-small value for the hard core radius.     

Study of the involvement of osmotic adjustment and H<Superscript>+</Superscript>-ATPase activity in the resistance of <Emphasis Type="Italic">Catharanthus roseus</Emphasis> suspension cells to salt stress

The salt-induced H⁺-ATPase activity and osmotic adjustment responses of Catharanthus roseus (L.) G. Don suspension cultures were studied. Cells were treated with 0, 50 or 100mM NaCl for 7days or were maintained for 8 months with 50 mM NaCl (50T cells). Growth, osmotic potential (), ions content, soluble sugars, proline and total amino acids were determined in the sap of control and salt-treated cells. Salinity reduced cell growth and . The higher decrease in the in salt-treated cells was due to higher accumulation of Na⁺ and Cl^–. The levels of organic solutes, such as soluble sugars, free proline and total amino acids, increased with salt treatment. These results suggest that salt-tolerant cells are able to osmotically adjust. Salinity treatments stimulated H⁺-ATPase activity. Immunodetection of the enzyme showed that the increased activity was due to an increased amount of protein in the plasmalemma. The induction by NaCl, especially at 100 mM NaCl and for 50T cells, could account for the K⁺ and Cl^– uptake but not for higher or lower tolerance.