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1.
The polarotropic response in protonemata of the fern Adiantumis regulated by phytochrome (Kadota et al. 1984); PR and PFRhave been shown to be dichroically oriented parallel and normalto the cell surface, respectively (Kadota et al. 1982). Thischange in the dichroic orientation of phytochrome during photoconversionwas analyzed by a newly-built, polarization plane-rotatabledouble laser flash irradiator. A polarotropic response was effectivelyinduced with a flash of polarized red (640 nm) light (6xl0–7s) having the vibration plane of the electrical vector parallelto the protonemal cell axis. When a flash of polarized far-red(710 nm) light (6xl0–7s) was given 30 sec after the redflash, the red flash-induced response was reversed by a far-redflash vibrating normal to the cell axis but not by one vibratingparallel. However, when given 2 µs or 2 ms after the redflash, the polarotropic response was not reversed by a polarizedfar-red flash vibrating normal to the cell axis but was reversedby a parallel-vibrating flash. These results suggest that theorientation of phototransformation intermediates existing 2µs or 2 ms after a red flash is still parallel to thecell surface, and that the change in the orientation of phytochromemolecules occurs between 2 ms and 30 s after the red flash. (Received February 3, 1986; Accepted April 23, 1986)  相似文献   

2.
This paper reports data and considerations relevant to the question of what determines the polarity of the voltages induced between electrodes in a suspension of chloroplasts when irradiated with a flash of light from a laser or flash-lamp. We found positive polarity (electrode nearest the light source positive) with excitation by ns pulses at 694, 539 and 530 nm wavelength. This and the earlier finding (Meszéna et al. (1988) Studia Biophysica 126:77–86), confirmed in this work, of negative polarity at 420 nm confirm, in part, the action spectrum reported by Gräber and Trissl (1981 FEBS Let 123:95–99) using 50 s flashes. Gräber and Trissl also showed that swelling the chloroplasts can reverse the polarity.Negative polarity is expected on the basis of a simple light-gradient in the sample together with what is known about photosynthetic charge movements. The cause of positive polarities has eluded explanation. Duration of flash was suspected. We tried a random series of short flashes averaging about 10 s apart and found that all simply duplicated the first flash. If there is any effect of light following the first flash it must occur in less than about 10 s.We suggest that the polarity is determined by a complicated interference pattern of the light in the chloroplast which can focus it onto different parts, front or back, depending upon the wavelength of the light and the structure of the chloroplast.Abbreviations DCMU 3-(3, 4-dichlorophenyl)-1, 1 dimethylurea - PSII photosystem II, the oxygen emitting system in green plant photosynthesis - EDTA ethylenediaminetetraacetic acid - Hepes N-2-Hydroxyethylpiperazine-N'-2-ethanesulfonic acid  相似文献   

3.
Photosystem II (PS II) of plants and cyanobacteria, which catalyzes the light-induced splitting of water and the release of oxygen, is the primary source of oxygen in the earth atmosphere. When activated by short light flashes, oxygen release in PS II occurs periodically with maxima after the third and the seventh flashes. Many other processes, including chlorophyll (Chl) t a fluorescence, are also modulated with period of four, reflecting their sensitivity to the activity of Photosystem II. A new approach has been developed for the analysis of the flash-induced fluorescence of Chl t a in plants, which is based on the use of the generalized Stern–Volmer equation for multiple quenchers. When applied to spinach thylakoids, this analysis reveals the presence of a new quencher of fluorescence whose amplitude is characterized by a periodicity of four with maxima after the third and the seventh flashes, in phase with oxygen release. The quencher appears with a delay of 0.5 ms followed by a rise time of 1.2–2 ms at pH 7, also in agreement with the expected time for oxygen evolution. It is concluded that the quencher is a product of the reaction leading to the oxygen evolution in PS II. The same quenching activity, maximal after the third flash, could be seen in dark adapted leaves, and provides the first fully time-resolved measurement of the kinetics of the oxygen evolution step in the leaf. Thus, the non-invasive probe of Chl t a fluorescence provides a new and sensitive method for measuring the kinetics of oxygen evolution with potential for use in plants and cyanobacteria t in vivo.  相似文献   

4.
The PS II–LHC II supercomplex is a novel type of oxygen evolving Photosystem II (PS II) core particle that contains the light harvesting complex proteins Lhcb1/2/4/5 in addition to the PS II reaction centre, oxygen evolving complex (OEC) and inner antennae [Hankamer et al. (1997) Eur J Biochem 243: 422–429]. The 33 and 23 kDa extrinsic proteins in these particles have been localised by image analysis of electron micrographs and averaging techniques [Boekema et al. (1998) Eur J Biochem 252: 268–276]. To assay the functionality of the water splitting complex, we compared the single flash P680+ reduction kinetics in these supercomplexes with those of PS II-rich granal stack membranes (BBYs). We found that the P680+ reduction kinetics in PS II–LHC II supercomplexes were indistinguishable from those in BBYs. We also examined a number of PS II core particles lacking the Lhcb components. All of these had different P680+ reduction kinetics, which we attributed to partial loss of OEC function before and during the measurements.  相似文献   

5.
Treatment of membranes ofHeliobacillus mobilis with high concentrations of the chaotropic agent urea resulted in the removal of the iron-sulfur centers FA and FB from the reaction center, as indicated by EPR spectra under strongly reducing conditions. In urea-treated membranes, transient absorption measurements upon a laser flash indicated a recombination between the photo-oxidized primary donor P798+ and a reduced acceptor with a time constant of 20 ms at room temperature. Benzylviologen, vitamin K-3 and methylene blue were found to accept electrons from the reduced acceptor efficiently. A differential extinction coefficient of 225–240 mM–1 cm–1 at 798 nm was determined from experiments in the presence of methylene blue. Transient absorption difference spectra between 400 and 500 nm in the presence and absence of artificial acceptors indicated that the electron acceptor involved in the 20 ms recombination has an absorption spectrum similar to that of an iron-sulfur center. This iron-sulfur center was assigned to be analogous to FX of Photosystem I. Our results provide evidence in support of the presence of FX in heliobacteria, which was proposed on the basis of the reaction center polypeptide sequence (Liebl et al. (1993) Proc. Natl. Acad. Sci. USA 90: 7124–7128). Implications for the electron transfer pathway in the reaction center of heliobacteria are discussed.  相似文献   

6.
It is shown that step-scan Fourier transform infrared spectroscopy can be applied to resolve the QA QB QAQB transition in Rhodobacter sphaeroides reaction centres with a 5 µs time resolution. In the mid-infrared region (1900 – 1200 cm–1), transient signals previously assigned to QA/B and QA/B vibrations, respectively (Brudler et al. 1994; Brudler et al. 1995; Breton and Nabedryk 1996), can be resolved with this new technique. In addition, the three small positive bands in the spectral region of the carboxylic C=O stretching modes of acidic amino acid side chains are also resolved at 1730, 1719 and 1704 cm–1. A global fit analysis yields two exponentials with half-times of 150 µs and 1.2 ms in agreement with IR spectroscopic studies at single wavenumbers (Hienerwadel et al. 1995), in the UV/VIS and near IR (Tiede et al. 1996, Li et al. 1996). The establishement of the step-scan technique enables a new approach to elucidate the molecular mechanism of this transition.  相似文献   

7.
The design and circuitry of solid electrodes of the Clark type for the determination of oxygen dissolved in microbial cultures and the suitable techniques are described. For the electrodes a portable battery instrument with an amplifier and recorder was developed. The electrode materials tested were: Au, Pt, Ag (cathode) and Ag/Ag2O and Ag/AgCl (anode). The effect of the presence of carbon dioxide on the course of the polarographic curves was determined. The temperature effect was determined for various membrane materials and its compensation with a thermistor was investigated. The effect of the circuit and design of the electrodes on stability, response time, reproducibility of measurement, durability of the electrodes and applicability in microbiology are discussed.  相似文献   

8.
A new NMR spin relaxation experiment is described for measuring chemical exchange time constants from approximately 0.5 ms to 5 ms in 15N-labeled macromolecules. The pulse sequence is based on the Carr–Purcell–Meiboom–Gill technique [Carr and Purcell (1954) Phys. Rev., 94, 630–638; Meiboom and Gill (1958) Rev. Sci. Instrum., 29, 688–691; Loria et al. (1999) J. Am. Chem. Soc., 121, 2331–2332], but implements TROSY selection [Pervushin et al. (1997) Proc. Natl. Acad. Sci. USA, 94, 12366–12371] to permit measurement of exchange linebroadening contributions to the narrower component of the 1H-15N scalar-coupled doublet. This modification extends the size limitation imposed on relaxation measurements due to the fast decay of transverse magnetization in larger macromolecules. The new TROSY-CPMG experiment is demonstrated on a [U-98% 15 N] labeled sample of basic pancreatic trypsin inhibitor and a [U-83% 2H, U-98% 15 N] labeled sample of triosephosphate isomerase, a 54 kDa homodimeric protein.  相似文献   

9.
The problem of obtaining very early ratios for the H+/O stoichiometry accompanying succinate oxidation by rat liver mitochondria was attacked using new techniques for direct measurement rather than extrapolations based on data obtained after mixing and the recovery of the electrode from initial injection of O2. Respiration was quickly initiated in a thoroughly mixed O2-containing suspension of mitochondria under a CO atmosphere by photolysis of the CO-cytochrome c oxidase complex-. Fast responding O2 and pH electrodes were used to collect data every 10 ms. The response time for each electrode was experimentally measured in each experiment and suitable corrections for electrode relaxations were made. With uncorrected data obtained after 0.8 s, the extrapolation back to zero time on the basis of single-exponential curve fitting confirmed values close to 8.0 as previously reported (Costa et al., 1984). The data directly obtained, however, indicate an initial burst in H+/O ratio that peaked to values of approximately 20 to 30 prior to 50 ms and which was no longer evident after 0.3 s. Newer information and considerations that place all extrapolation methods in question are discussed.  相似文献   

10.
We have previously reported concerning the existence of a third type of human α-amylase gene, AMY3 [Emi et al., Gene 62 (1988) 229–235; Tomita et al., Gene 76 (1989) 11–18], which is expressed in a lung carcinoid tissue, and differs in nucleotide sequence from the two previously characterized human α-amylase genes coding for salivary and pancreatic isozymes, termed AMY1 and AMY2, respectively.Here, we rename this gene AMY2B to coincide with the designation by Gumucio et al. [Mol. Cell Biol. 8 (1988) 1197–1205] and describe its genetic properties as revealed by sequencing studies. It consists of ten major exons whose sequences are highly homologous to those of AMY1 and AMY2. Not only the exons, but also most of the introns seem to be highly conserved, as judged from physical mapping data. The AMY2B gene identified from mRNA in a lung carcinoid tissue has at least two additional untranslated exons in its 5′ region; hence the promoter lies far upstream relative to the other two AMY genes.  相似文献   

11.
Until recently, polarographic methods for measuring the time course of transient changes in the rate of oxygen consumption (ΔQO2) have been applied only to tissue preparations containing thousands of cells. Here, we describe ΔQO2 measurements on the lateral ocellus of the barnacle (Balanus eburneus) which contains only three photoreceptor cells. The decrement of partial pressure of oxygen (ΔPO2) elicited by an 80 ms flash of light was measured near the cells with a microelectrode and the ΔQO2 was calculated from the ΔPO2 using a model of diffusion with spherical symmetry. As shown by mathematical simulation, the exact shape of the preparation is not crucial for our measurements of the time course of the ΔQO2. For a given ΔQO2, the model describes correctly the attenuation of the ΔPO2 measured at increased distances from the preparation. To know more about the mechanisms controlling the ΔQO2, we compared it with the electrical response of the photoreceptor cells: both responses have a similar spectral dependence, but only the ΔQO2 was abolished by a 10-min exposure to 50 μM dinitrophenol or to 3 mM amytal. We conclude that the ΔQO2 reflects an increase in mitochondrial respiration and that it is initiated by the phototransformation of rhodopsin, as was already found in the honeybee drone retina (Dimitracos and Tsacopoulos, 1985; Jones and Tsacopoulos, 1987).  相似文献   

12.
Oscillations of photosynthesis induced in leaves of Vicia faba L. were accompanied by oscillations not only in the pH of the chloroplast stroma, but also by pH oscillations in the cytosol and in the vacuole of leaf mesophyll cells. Cytosolic pH oscillations were in phase with stromal oscillations, but antiparallel to vacuolar pH oscillations. During maxima of photosynthesis, the cytosolic pH exhibited maxima and the vacuolar pH minima. Vacuolar acidification is interpreted to be the result of energized proton transport from the cytosol into the vacuole. Since the ratio of dihydroxyacetone phosphate to phosphoglycerate is maximal during the peaks of photosynthesis (Stitt et al., 1988, J. Plant Physiol. 133, 133–143; Laisk et al., 1991, Planta 185, 554–562), while the activity of NADP-malic dehydrogenase is highest during minima of photosynthesis (Scheibe and Stitt, 1988, Plant Physiol. Biochem. 26, 473–481), the present data indicate in agreement with earlier observations (Yin et al., 1991, Planta 184, 30–34) that light-dependent cytosolic energization is brought about by the oxidation of dihydroxyacetone phosphate rather than of malate. They also indicate that the over-reduction of the electrontransport chain observed during minima of photosynthesis is relieved not predominantly by oxaloacetate reduction and export of the resulting malate from the chloroplasts but by another reaction, presumably oxygen reduction.Abbreviations CDCF 5-(and 6-)carboxy-2,7-dichlorofluorescein  相似文献   

13.
In conflict with the Z-scheme of photosynthesis, it has recently been reported [Greenbaum et al. Nature (1995) 376: 438–441; Lee et al. Science (1996) 273: 364–367] that Photosystem II can drive ferredoxin reduction and photoautotrophic growth in some mutants of Chlamydomonas lacking detectable Photosystem I reaction centre, P700. Using the same mutants, B4 and F8, here we report that action spectra and parameters of flash yields of different photoreactions show the operation in ferredoxin-dependent H2 photoproduction and CO2 fixation of a fraction (at least 5% compared to wild- type) of the only Photosystem I complexes.  相似文献   

14.
The electrophoretic deposition of glucose oxidase from water using asymmetrical alternating voltages is investigated. Using asymmetric voltages, glucose oxidase layers with a thickness of 7 μm could be deposited on a platinum electrode in 20 min time as verified with a microbalance, carbon analysis and scanning electron microscopy. In contrast, if a symmetrical alternating signal is used under the same conditions, a layer of 0.5 μm is formed. We believe the deposition is due to two effects: the electrophoretic migration of the enzyme towards the deposition electrode and the pH induced precipitation of the enzyme near the deposition electrode. The electrophoretic migration is due to the non-linear dependence of the electrophoretic mobility on the electric field caused by the asymmetry of the applied alternating current signal. In addition, pH changes near the deposition electrode drive the enzyme towards its point of zero charge (PZC), perhaps causing the precipitation of GOx on the substrate. The effect of amplitude, frequency, deposition time and GOx concentration on the deposition rate was studied. An amplitude of 160 Vp–p and a frequency of 30 Hz was found to be optimal for the formation of thick enzyme layers, which excludes a big part of the interferences.  相似文献   

15.
Phosphorylation of thylakoid membrane proteins results in a partial inhibition (approximately 15–20%) of the light-saturated rate of oxygen evolution. The site of inhibition is thought to be located on the acceptor side of photosystem 2 (PS2) between the primary, QA, and secondary, QB, plastoquinone acceptors (Hodges et al. 1985, 1987). In this paper we report that thylakoid membrane phosphorylation increases the damping of the quaternary oscillation in the flash oxygen yield and increases the extent of the fast component in the deactivation of the S2 oxidation state. These results support the proposal that thylakoid membrane protein phosphorylation decreases the equilibrium constant for the exchange of an electron between QA and QB. An analysis of the oxygen release patterns using the recurrence matrix model of Lavorel (1976) indicates that thylakoid membrane phosphorylation increases the probability that PS2 miss a S-state transition by 20%. This is equivalent, however, to an insignificant inhibition (approximately 2.4%) of the light-saturated oxygen evolution rate. If a double miss in the S-state transitions is included when the PS2 centres are in S2 the fit between the experimental and theoretical oxygen yield sequences is better, and sufficient to account for the 15–20% inhibition in the steady-state oxygen yield. A double miss in the S-state transition is a consequence of an increased population of PS2 centres retaining QA : not only will these PS2 centres fail to catalyse photochemical charge transfer until QA is reoxidized, but the re-oxidation reaction will also result in the deactivation of S2 to S1.Abbreviations Chl Chlorophyll - PS2 Photosystem 2 - Si The oxidation states of PS2 (where i can be from 0 to 4) - QA and QB the anionic semiquinone forms of the primary and secondary plastoquione acceptors of PS2  相似文献   

16.
The influence of muscle activation and the time allowed for torque generation on the angle-specific torque-velocity relationship of the triceps surae was studied during plantar flexion using supramaximal electrical stimulation and a release technique on six male subjects [mean (SD) age 25 (4) years]. Torque-velocity data were obtained under different levels of constant muscle activation by varying the stimulus frequency and the time allowed for isometric torque generation prior to release and isokinetic shortening. To eliminate the effects of the frequency response on absolute torque the isokinetic data were normalized to the maximum isometric torque values at 0.44 rad. There were no significant differences in the normalized torques generated at any angular velocity using stimulus frequencies of 20, 50 or 80 Hz. When the muscle was stimulated at 50 Hz the torques obtained after a 400 ms and 1 s pre-release isometric contraction did not differ significantly. However, with no pre-release contraction significantly less torque was generated at all angular velocities beyond 1.05 rad · s–1 when compared with either the 200, 400 ms or 1 s condition. With a 200 ms pre-release contraction significantly less torque was generated at angular velocities beyond 1.05 rad · s–1 when compared with the 400 ms or 1 s conditions. It would seem that the major factor governing the shape of the torque-velocity curve at a constant level of muscle activation is the time allowed for torque generation.  相似文献   

17.
Amperometric estimation of BOD by using living immobilized yeasts   总被引:4,自引:0,他引:4  
Summary A microbial electrode consisting of immobilized living whole cells of yeasts, porous membrane and an oxygen electrode was prepared for continuous estimation of biochemical oxygen demand (BOD). Immobilized Trichosporon cutaneum was employed for the microbial electrode sensor for BOD. When a sample solution containing the equivalent amount of glucose and glutamic acid was injected into the sensor system, the current of the electrode decreased markedly with time until steady state was reached. The response time was within 18 min. A linear relationship was observed between the current decrease and the concentration below 41 mg l of glucose and 41 mg l glutamic acid (5-day BOD 60 mg l ). The current decrease was reproducible within ± 6% of the relative error when a sample solution containing 27 mg l of glucose and 27 mg l of glutamic acid (5-day BOD 40 mg l ) was employed. The microbial electrode sensor was applied to untreated waste waters from a fermentation factory. Good comparative results were obtained between BOD estimated by the microbial electrode and that determined by the conventional 5-day method (regression coefficient was 1.2). Furthermore, the effect of various compounds on BOD estimation was also examined. The current output of the microbial electrode sensor was almost constant for 17 d and 400 tests.  相似文献   

18.
This paper is concerned with the definition of the standard conditions required for optimum operation of the bare platinum electrode with photosynthetic samples. Experimental evidence shows the following: 1) Polarization circuits should have zero resistance; 2) The electrolyte layer between the electrodes should have a conductance higher than 54×10–6 –1 per mm2 of platinum electrode area; 3) The electrodes should be polarized just before taking the measurements. All these facts can be interpreted in terms of phenomena occurring on the electrode: The adsorption of hydrogen on the electrode imposes the need for low resistances in the system, and oxygen consumption by the electrode is minimized by polarizing the electrodes as late as possible. This investigation increases the reliability of the bare platinum electrode and gives a basis for a comparison of the results from different experiments. Demonstrations of the pertinence of these conditions are made in our lab with the algae Dunaliella Tertiolecta.  相似文献   

19.
Oxygen and glucose biosensors have been designed, fabricated, characterized and optimized for real-time continuous monitoring on a new smart catheter for use in patients with traumatic brain injury (TBI). Oxygen sensors with three-electrode configuration were designed to achieve zero net oxygen consumption. Glucose sensors were based on the use of platinum nanoparticle-enhanced electrodes that were modified with polycation and glucose oxidase immobilized by chitosan matrix. An iridium oxide electrode was developed to work as a biocompatible reference electrode with enhanced durability and stability in the biological solutions. A study of the effect of temperature on oxygen sensor performance, and both temperature and oxygen effects on glucose sensor performance were accomplished to enhance their operative stability and provide useful information for in vivo applications. A new methodology for automatic correction of the temperature and oxygen dependence of biosensor outputs is demonstrated through programmed LabView™ software. In vitro experiments in both physiological and pathophysiological ranges (oxygen: 0–60 mmHg; glucose: 0.1–10 mM; temperature: 25–40 °C) with clinical samples of cerebrospinal fluid obtained from TBI patients have demonstrated stable measurements with enhanced accuracy, indicating the feasibility of the sensors for a real-time continuous in vivo monitoring.  相似文献   

20.
Summary During the European Polarstern Study (EPOS leg 1 and leg 2) measurements of temperature, salinity, inorganic nutrients, chlorophyll-a, oxygen and total inorganic carbon dioxide were performed from October to January 1988–1989 in north-south sections at 47–49 °E in the NW Weddell Sea from approximately 58 °S to 63 °S (Hempel 1989; Hempel et al. 1989). In order to explain parts of the obtained data, a time-dependent ecological model was constructed by Svansson (1991). He found that a moderate mixing with a constant diffusion coefficient from sea surface downwards resulted in good agreement between computed and measured chlorophyll. In this paper we introduce the gas fluxes, mainly oxygen but also carbon dioxide, into the model work. It turns out that air-sea fluxes are necessary to explain the vertical oxygen distribution. The annual development of chlorophyll, phosphate, oxygen and total inorganic carbon dioxide are computed. Hours of day-light, losses and the eddy diffusion coefficient are allowed to vary during the year with the condition that the mean total chlorophyll at 14 selected leg 1 stations was nearly double the magnitude of that of 18 selected leg 2 stations. This yields variations consistent with the observations. Different steady-state solutions after 91 days are also tested to show effects of one selected variation at a time, for example the eddy diffusion coefficient or the loss rate. The oxygen air-sea flux, of about 90 mmol m–2 day–1 in the time variable model computation, is compared to estimated fluxes by a gas transfer formula. The formula used gives a flux which is about 5 times smaller than the model flux. Some of the 91 days solutions give results of fluxes which are less than 90 mmol m–2 day–1 but still higher than the transfer formula result. Fluxes of total inorganic carbon dioxide in the model computation are always directed from air to sea.Data presented here were collected during the European Polarstern Study (EPOS) sponsored by the European Science Foundation  相似文献   

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