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1.
Two spatially separate membrane potentials of the parenchymasymplast (7, 8) and the rate of elongation growth were measuredsimultaneously in bean hypocotyl segments. Both the membrane potentials, Vps (electric potential differencebetween parenchyma symplast and organ surface) and Vpx (electricpotential difference between parenchyma symplast and xylem),were rapidly depolarized by anoxia, and were repolarized withre-aeration. Anoxia reduced the growth rate by about 85%, andre-aeration restored it. Changes in the membrane potentialspreceded those in the growth rate by 30–50 sec. About 8 min after the application of aerosol generated from10–3 M indole acetic acid (IAA) solution to the segments,Vps began to hyperpolarize, and the growth rate increased witha delay of several minutes after the potential change and subsequentlybecame ten times the control rate. This hyperpolarization ofVps was due to the increase in the activity of the respiration-dependentelectrogenic ion pump at the outer surface membrane of the parenchymasymplast. A clear correlation was observed between the growthrate and pump activity (Vps) with the change in IAA concentration. (Received December 6, 1979; )  相似文献   

2.
Tracer amounts of atmospheric [13N]-Iabelled ammonia gas, wereabsorbed by leaves of Lupinus albus and Helianthus annuus inboth the light and the dark. Exogenous [13N]-ammonia was onlyabsorbed in the dark when the feeding occurred shortly aftera period of illumination and the tissue was not depleted ofits carbohydrate reserves (e.g. starch). Incorporation of the[13N]-ammonia appeared to occur via the leaf glutamine synthetase/glutamatesynthase (GS/GOGAT) cycle since 2.0 mol m–3 MSX, an inhibitorof the GS reduced uptake in both the light and dark. Photosyntheticincorporation of 11CO2 was not affected by this treatment Therate of movement of [13N]-assimilates in the petiole of attachedleaves of Helianthus and Lupinus was similar to that of the11Cl-photo assimilates. Export of both [13N] and [11C]-Iabelledassimilates from the leaf and movement in the petiole in boththe light and the dark was inhibited by source leaf anoxia (i.e.nitrogen gas). Translocation was re-established at the samerate when the feed leaf was exposed to gas containing more than2% O2 which permitted dark respiration to proceed. After aninitial feeding of either 11CO2 or [13N]-ammonia at ambient(21%) O2 exposure of the source leaf to 2% O2, or 50% O2 didnot alter the rates of translocation, indicating that changesin photosynthetic activity in the source leaf due to photorespiratoryactivity need not markedly alter, at least during the shortperiod, the loading and translocation of either [11C ] or [13N]-labelledleaf products. Key words: Translocation, CO2, NH3, Leaves, Helianthus annuus, Lupinus albus  相似文献   

3.
The cell-membrane resistance (Rm) of Vigna hypocotyls was examined,and the effects of osmotic stress, ionic stress and IAA on Rmwere investigated. Rm decreased by 64 to 77% under osmotic stressin the presence of absorbable solutes (40 mM sorbitol, 15 mMKC1, 30 mM sucrose; or 40 mM sorbitol, 15 mM KC1, 30 mM sucroseplus 10–4 M IAA) or under ionic stress (50 mM NaCl or50 mM KC1). Rm was not changed by perfusion with 10–4M IAA. Therefore, the hyper-polarizations of the membrane potentialobserved in both cases should be ascribed totally to the activationof the electrogenic proton pump. Although Rm showed an increaseof 1.6 fold when the hypocotyls were subjected to osmotic stress(100 mM sorbitol or 100 mM sorbitol plus 10–4 M IAA),83.6% or 92.4% of the hyperpolarization of the membrane potential(Vpx was also the result of the activation of the pump. Theresults, calculated on the basis of the current source model,support the viewpoint that the hyperpolarization of the cellmembrane potential of Vigna hypocotyls under osmotic stress,ionic stress or in the presence of IAA is an expression of theactivation of the proton pump, and is not caused by an increasein Rm. 1 Present address: Researchers and Planners of Natural Environment, Yotsugi Bldg. (2F), 1-5-4 Horinouchi, Suginami-Ku, Tokyo,166 Japan 2 Present address: Graduate School of Integrated Science, YokohamaCity University, 22-2 Seto, Kanazawa-Ku, Yokohama, 236 Japan (Received February 14, 1991; Accepted July 24, 1991)  相似文献   

4.
Bunce  James A. 《Annals of botany》1995,75(4):365-368
Previous work has shown that elevated carbon dioxide (CO2) concentrationsin the dark reversibly reduce the rate of CO2 efflux from soybeans.Experiments were performed exposing soybean plants continuallyto concentrations of 350 or 700 cm3 m-3 for 24 h d-1, or to350 during the day and 700 cm3 m-3 at night, in order to determinethe importance of the reduced rate of dark CO2 efflux for plantgrowth. High CO2 applied only at night conserved carbon andincreased dry mass during initial growth compared with the constant350 cm3 m-3 treatment. Long-term net assimilation rate was increasedby high CO2 in the dark, without any increase in daytime leafphotosynthesis. However, leaf area ratio was reduced by thedark CO2 treatment to values equal to those of plants continuallyexposed to the higher concentration. From days 14-21, leaf areawas less for the elevated night-time CO2 treatment than foreither the constant 350 or 700 cm3 m-3 treatments. For the days7-21-period, relative growth rate was significantly reducedby the high night CO2 treatment compared with the 350 cm3 m-3continuous treatment. The results indicate that some functionallysignificant component of respiration was reduced by the elevatedCO2 concentration in the dark.Copyright 1995, 1999 AcademicPress Glycine max L. (Merr.), carbon dioxide, plant growth, respiration  相似文献   

5.
The application of D-glucose to solutions bathing excised maize,wheat, pea and bean roots causes a rapid depolarization of theelectrical potentials between the cut tops of the roots andthe bathing solutions. Similar effects are observed for theplasma membrane potentials of maize lateral roots. A flow cell apparatus was used to demonstrate qualitative andquantitative relations between glucose induced H+ influx andthe transient decrease in current through the root. The currentchanges appear to be due entirely to H+ fluxes. Current andH+ fluxes are strongly influenced by external pH, the optimumpH for glucose induced current change being about 4.0. A similarpH optimum was found for 3-O-methyl-D-glucopyranoside but 1-O-methyl--D-glucopyranosidedid not significantly affect the trans-root potential at anypH, suggesting a significant role for the anomeric hydroxylgroup of glucose. Compounds which depolarize the trans-root potential also inhibitthe glucose induced depolarization. Surface -SH groups are probablynot involved in the glucose/H+ cotransport. Eadie-Hofstee plots relating the depolarization of trans-rootpotential to the concentrations of D-glucose or 3-O-methyl-D-glucopyranosidehave shown that Km values increase with increasing monosaccharideconcentration and are very similar to reported values of 3-O-methyl-D-glucopyranosideuptake in maize root segments. Km values for a similar rangeof D-glucose concentrations do not vary significantly with pHor with membrane depolarization due to a 10-fold increase ofKCl concentration. However, Vmax is lowered by an increase inexternal pH or a decrease in trans-root potential. It appearsthat both proton and electrical gradients can affect glucoseinduced H+ influx. The auxin herbicide, 2, 4-dichlorophenoxyethanoic acid (0.01mM) stimulates the glucose induced depolarizations in a mannerconsistent with an increase in cytoplasmic pH. This is discussedin relation to the reported action of indole-3-acetic acid andfusicoccin on maize root tissue.  相似文献   

6.
Biophysical characterization of zebrafish connexin35 hemichannels   总被引:1,自引:0,他引:1  
A subset of connexins can form unopposed hemichannels in expression systems, providing an opportunity for comparison of hemichannel gating properties with those of intact gap junction channels. Zebrafish connexin35 (Cx35) is a member of the Cx35/Cx36 subgroup of connexins highly expressed in the retina and brain. In the present study, we have shown that Cx35 expression in Xenopus oocytes and N2A cells produced large outward whole cell currents on cell depolarization. Using whole cell, cell-attached, and excised patch configurations, we obtained multichannel and single-channel current recordings attributable to the Cx35 hemichannels (Ihc) that were activated and increased by stepwise depolarization of membrane potential (Vm) and deactivated by hyperpolarization. The currents were not detected in untransfected N2A cells or in control oocytes injected with antisense Cx38. However, water-injected oocytes that were not treated with antisense showed activities attributable to Cx38 hemichannels that were easily distinguishable from Cx35 hemichannels by a significantly larger unitary conductance (hc: 250–320 pS). The hc of Cx35 hemichannels exhibited a pronounced Vm dependence; i.e., hc increased/decreased with relative hyperpolarization/depolarization (hc was 72 pS at Vm = –100 mV and 35 pS at Vm = 100 mV). Extrapolation to Vm = 0 mV predicted a hc of 48 pS, suggesting a unitary conductance of intact Cx35 gap junction channels of 24 pS. Channel gating was also Vm dependent: open time declined with negative Vm and increased with positive Vm. The ability to break down the complex gating of intact intercellular channels into component hemichannels in vitro will help to evaluate putative physiological roles for hemichannels in vivo. connexin; gating; retina  相似文献   

7.
Cratoneuron filicinum, a drought-sensitive moss, and Tortularuralis, a drought-tolerant moss, fix CO2 non-autotrophicallyat a rate of about 1.2 and 2.2 µmol h–1 g–1dry wt. respectively. During drying, T. ruralis fixes CO2 atan undiminished rate until the tissue loses about 60% of theinitial fresh weight. Thereafter, CO2 fixation rapidly declinesto zero. Dark CO2 fixation by C.filicinum declines steadilyduring the dehydration period. On rehydration, dark CO2 fixationis resumed immediately in T. ruralis but not in C.filicinum.When dried T. ruralis is equilibrated with an atmosphere ofnearly 100% relative humidity, its weight increases to about40% of the original fresh weight and dark CO2 fixation resumesat a rate about 60% of the fresh moss. In C.filicinum thereis only a small increase in weight and little CO2 fixation inthe dark. The non-autotrophically fixed carbon, in both mossesstudied, is incorporated into amino acids (more than 60% ofthe total, mainly into aspartate, alanine and glutamate) andorganic acids (less than 40% of the total, mainly into malate).It is suggested that on rehydration immediate availability ofNADPH, known to be produced by transhydrogenation from NADHduring dark CO2 fixation, may be an important factor in therepair of drought-induced cellular damage by reductive biosynthesisof membrane components and other cellular constituents. Key words: Mosses, Dehydration, Rehydration, Dark CO2 fixation, Amino acids, Organic acids, NADPH, Drought tolerance.  相似文献   

8.
Mass spectrometry has been used to investigate the transportof CO2 in the freshwater diatom Navicula pelliculosa. The timecourseof CO2 formation in the dark after addition of 100 mmol m–3dissolved inorganic carbon (DIC) to cell suspensions showedthat no external carbonic anhydrase (CA) was present in thesecells. Upon illumination, cells pre-incubated at pH 75 with100 mmol m–3 DIC, removed almost all free CO2 from themedium at an initial rate of 285 µmol CO2 mg–1Chl h–1. Equilibrium between HCO3 and CO2 in themedium occurred rapidly upon addition of bovine CA, showingthat CO2 depletion resulted from a selective uptake of CO2 ratherthan an uptake of all inorganic carbon species. However, photosyntheticO2 evolution rate remained constant after CO2 had been depletedfrom the medium indicating that photosynthesis is sustainedprimarily by active HCO3 uptake. Treatment of cells with2-iodoacetamide (83 mol m–3) completely inhibited CO2fixation but had little effect on CO2 transport since initialrates of CO2 depletion were about 81% that of untreated cells.Transfer of iodoacetamide-treated cells to the dark caused arapid increase in the CO2 concentration in the medium largelydue to the efflux of the unfixed intracellular DIC pool whichwas found to be about 194 times the concentration of that inthe external medium. These results indicate that Navicula pelliculosaactively takes up molecular CO2 against a concentration gradientby a process distinct from HCO3 transport. Key words: Dissolved inorganic carbon, carbonic anhydrase, bicarbonate transport, CO2 transport, mass spectrometry  相似文献   

9.
K+ efflux from tobacco (Nicotiana tabacum L, cv. Samsun NN)leaf discs into the external medium was increased and the membranepotential (Em) changed in the positive direction with a changein pH from 8.0 to 4.0. Em was affected by the external concentrationof KCl, greatly decreasing with a change in concentration from1 mM to 100 mM. The equilibrium potential of the membrane forK+ (Ek) was decreased in a Nernst fashion with increasing externalconcentrations of KCl. Ek is more positive than Em above ca.50 µM KCl. Most of the experiments were carried out underconditions in which the difference between the electrochemicalpotential for K+ on the inside to the outside of the cell (µkis positive. Thus, K+ may passively flow to the outside of thecells accompanied by the depolarization of the membrane. Abscisic acid (ABA) increased the K+ efflux under conditionsof passive transport. K+ efflux was accelerated with an increasingconcentration of ABA, being maximal at 10–4 M–10–3M. This acceleration was due to the enhancement of the potassiummotive force (µk/F) which is the force causing the netpassive transport of K+. The membrane potential was decreasedfrom –205 mV to –170 mV by 2 x 10–4 M ABAwithin 10 min. The depolarization was not transient, being lostfor at least 3 hr. These results show that ABA accelerated passive K+ efflux, whichaccompanied depolarization of the membrane. (Received June 22, 1981; Accepted August 24, 1981)  相似文献   

10.
Phosphate Uptake in the Cyanobacterium Synechococcus R-2 PCC 7942   总被引:4,自引:0,他引:4  
Phosphate uptake rates in Synechococcus R-2 in BG-11 media (anitrate-based medium, not phosphate limited) were measured usingcells grown semi-continuously and in continuous culture. Netuptake of phosphate is proportional to external concentration.Growing cells at pHo 10 have a net uptake rate of about 600pmol m–2 s–1 phosphate, but the isotopic flux for32P phosphate was about 4 nmol m–2 s–1. There appearsto be a constitutive over-capacity for phosphate uptake. TheKm and Vmax, of the saturable component were not significantlydifferent at pHo 7.5 and 10, hence the transport system probablyrecognizes both H2PO4and HPO2–4. The intracellularinorganic phosphate concentration is about 3 to 10 mol m–3,but there is an intracellular polyphosphate store of about 400mol m–3. Intracellular inorganic phosphate is 25 to 50kJ mol–1 from electrochemical equilibrium in both thelight and dark and at pHo 7.5 and 10. Phosphate uptake is veryslow in the dark ( 100 pmol m–2 s–1) and is light-activated(pHo 7.51.3 nmol m–2 s–1, pHo 10600 pmol m–2s–1). Uptake has an irreversible requirement for Mg2+in the medium. Uptake in the light is strongly Na+-dependent.Phosphate uptake was negatively electrogenic (net negative chargetaken up when transporting phosphate) at pHo 7.5, but positivelyelectrogenic at pHo 10. This seems to exclude a sodium motiveforce driven mechanism. An ATP-driven phosphate uptake mechanismneeds to have a stoichiometry of one phosphate taken up perATP (1 PO4 in/ATP) to be thermodynamically possible under allthe conditions tested in the present study. (Received June 16, 1997; Accepted September 4, 1997)  相似文献   

11.
The effects of night-time temperature, leaf-to-air vapour pressuredeficit (VPD) and water stress on CO2 recycling in Bromeliahumilis Jacq. grown under two light and nitrogen regimes wereinvestigated. At night-time temperatures above 30°C, integratednet dark CO2 uptake was severely reduced and CO2 for malatesynthesis was mainly derived from dark respiration. At 35°C,up to 84% of the CO2 liberated by dark respiration was refixedinto malic acid. Below 30 °C only nitrogen deficient plantsshowed significant recycling. No significant differences wereobserved between high and low light grown plants in CO2 recycling.A doubling of leaf-to-air VPD from 7-46 Pa kPa–1 to 15.49Pa kPa–1 resulted in a 2- to 20-fold decrease in leafconductance and about 50 to 65% reduction in integrated darkCO2 uptake. However, about twice as much CO2 was recycled atthe higher VPD as in the lower. Ten days of water stress resultedin 80 to 100% recycling of respiratory CO2. Under high VPD andwater stress treatments, the amount of water potentially savedthrough recycling of CO2 reached 2- to 6-fold of the actualtranspiration. In general, nitrogen deficient plants had higherper cent recycling of respiratory CO2 in response to high night-timetemperature, increased VPD or water stress. The results emphasizethe ecological relevance of carbon recycling in CAM plants. Key words: Bromelia humilis, CAM, PPFD, dark respiration, temperature, VPD, water stress  相似文献   

12.
Insulin secretion is dependent on coordinated pancreatic islet physiology. In the present study, we found a way to overcome the limitations of cellular electrophysiology to optically determine cell membrane potential (Vm) throughout an islet by using a fast voltage optical dye pair. Using laser scanning confocal microscopy (LSCM), we observed fluorescence (Förster) resonance energy transfer (FRET) with the fluorescent donor N-(6-chloro-7-hydroxycoumarin-3-carbonyl)-dimyristoylphosphatidyl-ethanolamine and the acceptor bis-(1,3-diethylthiobarbiturate) trimethine oxonol in the plasma membrane of essentially every cell within an islet. The FRET signal was approximately linear from Vm –70 to +50 mV with a 2.5-fold change in amplitude. We evaluated the responses of islet cells to glucose and tetraethylammonium. Essentially, every responding cell in a mouse islet displayed similar time-dependent changes in Vm. When Vm was measured simultaneously with intracellular Ca2+, all active cells showed tight coupling of Vm to islet cell Ca2+ changes. Our findings indicate that FRET-based, voltage-sensitive dyes used in conjunction with LSCM imaging could be extremely useful in studies of excitation-secretion coupling in intact islets of Langerhans. pancreatic -cell; optical electrophysiology; islet electrical coupling  相似文献   

13.
Published data suggest that the neuropeptide calcitonin gene-related peptide (CGRP) can stimulate osteoblastic bone formation; however, interest has focused on activation of cAMP-dependent signaling pathways in osteogenic cells without full consideration of the importance of cAMP-independent signaling. We have now examined the effects of CGRP on intracellular Ca2+ concentration ([Ca2+]int) and membrane potential (Em) in preosteoblastic human MG-63 cells by single-cell fluorescent confocal analysis using fluo 4-AM-fura red-AM and bis(1,3-dibarbituric acid)-trimethine oxanol [DiBAC4(3)] bis-oxonol assays. CGRP produced a two-stage change in [Ca2+]int: a rapid transient peak and a secondary sustained increase. Both responses were dose dependent with an EC50 of 0.30 nM, and the maximal effect (initially 3-fold over basal levels) was observed at 20 nM. The initial phase was sensitive to inhibition of Ca2+ mobilization with thapsigargin, whereas the secondary phase was eliminated only by blocking transmembrane Ca2+ influx with verapamil or inhibiting cAMP-dependent signaling with the Rp isomer of adenosine 3',5'-cyclic monophosphorothioate (Rp-cAMPS). These data suggest that CGRP initially stimulates Ca2+ discharge from intracellular stores by a cAMP-independent mechanism and subsequently stimulates Ca2+ influx through L-type voltage-dependent Ca2+ channels by a cAMP-dependent mechanism. In addition, CGRP dose-dependently polarized cellular Em, with maximal effect at 20 nM and an EC50 of 0.30 nM. This effect was attenuated with charybdotoxin (–20%) or glyburide (glibenclamide; –80%), suggesting that Em hyperpolarization is induced by both Ca2+-activated and ATP-sensitive K+ channels. Thus CGRP signals strongly by both cAMP-dependent and cAMP-independent signaling pathways in preosteoblastic human MG-63 cells. osteoblastic cells; calcium; membrane potential; potassium channels; adenosine 3',5'-cyclic monophosphate  相似文献   

14.
Polyamines are essential for cell migrationduring early mucosal restitution after wounding in the gastrointestinaltract. Activity of voltage-gated K+ channels (Kv) controlsmembrane potential (Em) that regulates cytoplasmicfree Ca2+ concentration([Ca2+]cyt) by governing thedriving force for Ca2+ influx. This study determinedwhether polyamines are required for the stimulation of cell migrationby altering K+ channel gene expression,Em, and[Ca2+]cyt in intestinal epithelialcells (IEC-6). The specific inhibitor of polyamine synthesis,-difluoromethylornithine (DFMO, 5 mM), depleted cellularpolyamines (putrescine, spermidine, and spermine), selectivelyinhibited Kv1.1 channel (a delayed-rectifier Kv channel) expression,and resulted in membrane depolarization. Because IEC-6 cells did notexpress voltage-gated Ca2+ channels, the depolarizedEm in DFMO-treated cells decreased [Ca2+]cyt as a result of reduceddriving force for Ca2+ influx through capacitativeCa2+ entry. Migration was reduced by 80% in thepolyamine-deficient cells. Exogenous spermidine not only reversed theeffects of DFMO on Kv1.1 channel expression, Em,and [Ca2+]cyt but also restoredcell migration to normal. Removal of extracellular Ca2+ orblockade of Kv channels (by 4-aminopyridine, 1-5 mM) significantly inhibited normal cell migration and prevented the restoration of cellmigration by exogenous spermidine in polyamine-deficient cells. Theseresults suggest that polyamine-dependent intestinal epithelial cellmigration may be due partially to an increase of Kv1.1 channelexpression. The subsequent membrane hyperpolarization raises[Ca2+]cyt by increasing the drivingforce (the electrochemical gradient) for Ca2+ influx andthus stimulates cell migration.

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15.
Madsen, T. V. 1987. Sources of inorganic carbon acquired throughCAM in Littorella uniflora (L.) Aschers.—J. exp. Bot.38: 367–377. The CO2 dynamics of the lacunal air and the relative contributionof external and internal CO2 sources to dark CO2 assimilationwas examined in the submerged aquatic CAM species Littorellauniflora (L.) Aschers. Refixation of internal CO2, released by dark respiration, constitutedabout 30–35% of the total dark CO2 assimilation. At aCO2 concentration of 0·2 mol m–3 around the leavesthe external CO2 uptake through the roots increased from 45%of the total CO2 uptake at 0·7 mol m–3 CO2 to 100%at 1·6 mol m–3 and 3·1 mol m–3 CO2around the roots. The negligible importance of leaf CO2 uptakeat high CO2 concentrations around the roots was the result ofa causative high CO2 concentration in the leaf lacunae. The CO2 permeability of Littorella leaves was high relativeto root permeability. This has at least two ecological implications:(1) it enhances the potential diffusive release of CO2 fromthe sediment C02-pool via the lacunal system of the plants.This loss of CO2, however, was found to be greatly reduced byCAM activity of the plants. (2) The high permeability of theleaf surface to CO2 exchange allows the plants to assimilateCO2 from the water surrounding the leaves when the concentrationis high, i.e. during extensive epiphyte dark respiration. Thus,CAM tends to facilitate retension of a high CO2 pool in thesediment-plant system and at the same time allows the plantsto exploit the water column CO2 source when it is abundant.This result is in accordance with the general idea that CAMin aquatics constitute a carbon conserving mechanism. Key words: Aquatic macrophytes, dark CO2 assimilation, inorganic carbon sources  相似文献   

16.
The maximum rate of photosynthetic 14CO2 fixation (Vmax) aswell as the concentration of CO2 at which the rate of photosynthetic14CO2 fixation attains one-half its maximum velocity (Km) inChlorella vulgaris 11h cells was strongly dependent on the concentrationof CO2 continuously provided during the algal growth. The Vmax (µmoles 14CO2 fixed/ml pcv?min) and Km (% CO2)of the algal cells which had been grown in air containing 4%CO2 (by volume) were ca. 10 and 0.15–0.17, while thosein the cells which had been grown in ordinary air (containing0.04% CO2) were 7 and 0.05–0.06, respectively. When the concentration of CO2 in the bubbling gas was loweredfrom 4 to 0.04% during the algal growth, their photosynthetickinetics attained the respective lower steady levels after 5–10hr. On the other hand, when the photosynthetic kinetics weredetermined 24 hr after raising the concentration of CO2 from0.04 to 4%, the Vmax and Km-values were found to have alreadyattained the respective higher levels. (Received October 15, 1976; )  相似文献   

17.
Two methods were used to estimate construction costs for leaves,stems, branches and woody roots of yellow-poplar (LiriodendrontulipiferaL.) trees grown at ambient (35 Pa) and elevated (65Pa) CO2for 2.7 years and trees of white oak (Quercus albaL.)grown at these same CO2partial pressures for 4 years. Samplecombustion in a bomb calorimeter combined with measurementsof ash and nitrogen content provided the primary method of estimatingtissue construction costs (WG; g glucose g-1dry mass). Thesevalues were compared with a second, simpler method in whichcost estimates were derived from tissue ash, carbon and nitrogencontent (VG). Estimates of WGwere lower for leaves, branchesand roots of yellow-poplar and for leaves of white oak grownat elevated compared with ambient CO2partial pressures. TheseCO2-induced differences in WGranged from 3.7% in yellow-poplarroots to 2.1% in white oak leaves. Only in the case of yellow-poplarleaves, however, were differences in VGobserved between CO2treatments.Leaf VGwas 1.46 g glucose g-1dry mass in ambient-grown treescompared with 1.41 g glucose g-1dry mass for CO2-enriched trees.Although paired-estimates of WGand VGclustered about a 1:1 linefor leaves and branches, estimates of VGwere consistently lowerthan WGfor stems and roots. Construction costs per unit leafarea were 95 g glucose m-2for yellow-poplar trees grown at ambientCO2and 106 g glucose m-2for trees grown at elevated CO2partialpressures. No differences in area-based construction costs wereobserved for white oak. Whole-plant energy content was 1220g glucose per tree in ambient-grown white oak compared with2840 g glucose per tree for those grown at elevated CO2partialpressures. These differences were driven largely by CO2-inducedchanges in total biomass. We conclude that while constructioncosts were lower at elevated CO2partial pressures, the magnitudeof this response argues against an increased efficiency of carbonuse in the growth processes of trees exposed to CO2enrichment. Bomb calorimeter; construction costs; elevated CO2; energy allocation; global change; growth respiration; heat of combustion; respiration; Liriodendron tulipifera; Quercus alba  相似文献   

18.
The utilization of inorganic carbon and role of the coccolithswere investigated in intact cells and protoplasts of a marineunicellular calcareous alga, Emiliania huxleyi. Protoplastswith high photosynthetic activity were obtained by artificialdecalcification with 50 mM MES-NaOH (pH5.5). (1) The kineticsof the photosynthetic evolution of O2 at various concentrationsof externally added NaHCO3 were the same for intact cells andprotoplasts, indicating that the kinetic properties with respectto dissolved inorganic carbon (DIC) were not affected by thepresence or absence of the coccoliths on the cell surface. Double-reciprocalplots and plots of the concentration of substrate divided byvelocity (s/v) against the concentration of substrate (s) werebiphasic in the case of both intact cells and protoplasts. TheCO2-utilization reaction was, therefore, considered to involvetwo processes with different values of Km and Vmax. From thekinetic analyses, Km and Vmax [µmoles O2 (ml PCV)–1h–1] were deduced to be 92 µM and 76.3 for a "low-Km"reaction and 4.1 mM and 252 for a "high-Km" reaction, respectively.(2) In short-term (40-min) experiments, time courses of thetotal uptake of 14C-DIC and the incorporation of 14C into acid-stableproducts of photosynthesis and the internal pool of DIC, determinedas acid-labile compounds, under CO2-limiting conditions (80µM) were very similar for intact cells and protoplasts.However, incorporation of 14C into CaCO3 apparently occurredmore slowly in protoplasts than in intact cells. (3) In longterm (24-h) experiments, patterns of incorporation of 14C werealmost same for intact cells and protoplasts, with the exceptionthat the amount of 14C incorporated into CaCO3 was much smallerin the former than the latter. The production of Ca14CO3 increasedduring the course of 10 h after a 4-h lag. However, after 10h the level of Ca14CCO3 started to decrease. The decrease wasaccompanied by an increase in 14C in the products of photosynthesis,suggesting that CaCO3 was reutilized for the photosyntheticfixation of CO2 and, therefore, that the coccoliths functionas sites of storage of DIC. However, the internal level of DICremained at the same level even after the supply of externalDIC has been almost completely depleted. (Received July 25, 1995; Accepted December 11, 1995)  相似文献   

19.
The effect of ABA on the membrane potential of barley (Hordeumvulgare cv. Himalaya) aleurone protoplasts was studied by measuringthe distribution of the lipophilic cation tetraphenylphosphonium(TPP+). The resting membrane potential (Em) according to ourmeasurements with TPP+ is about –53 mV and is in agreementwith membrane potential values as measured with intracellularmicroelectrodes (about –55 mV). The TPP+-measurementscould demonstrate a clear dependence of the resting Em on theexternal pH (pHe). Stimulation of the protoplasts with ABA induced a transienthyperpolarization of the membrane to –62 mV as measuredwith TPP+. The hyperpolarization was ABA-concentration dependent. Inhibition of the H+-ATPases with the specific proton pump inhibitorsdiethylstilbestrol (DES) or Micanozole effectively preventedhyperpolarization. This indicates that the hyperpolarizationis consistent with the activation of plasma membrane H+-ATPases.The K+-inward rectifier inhibitor BaCl2 was able to prolongthe hyperpolarization. This result suggests that the hyperpolarizationcauses the opening of K+-channels. The ABA-induced proton-pump activation may be involved in ABA-inducedgene-expression, as DES was able to inhibit this gene expression.BaCl2 did only show a slight inhibitory effect on ABA-inducedgene-expression. (Received January 4, 1994; Accepted April 12, 1994)  相似文献   

20.
Insulin enhancesNa+-K+ pump activity in various noncardiactissues. We examined whether insulin exposure in vitro regulates Na+-K+ pump function in rabbit ventricularmyocytes. Pump current (Ip) was measured using thewhole-cell patch-clamp technique at test potentials(Vms) from 100 to +60 mV. When theNa+ concentration in the patch pipette([Na]pip) was 10 mM, insulin caused aVm-dependent increase in Ip.The increase was ~70% when Vm was at nearphysiological diastolic potentials. This effect persisted afterelimination of extracellular voltage-dependent steps and whenK+ and K+-congeners were excluded from thepatch pipettes. When [Na]pip was 80 mM, causingnear-maximal pump stimulation, insulin had no effect, suggesting thatit did not cause an increase in membrane pump density. Effects oftyrphostin A25, wortmannin, okadaic acid, or bisindolylmaleimide I inpipette solutions suggested that the insulin-induced increase inIp involved activation of tyrosine kinase,phosphatidylinositol 3-kinase, and protein phosphatase 1, whereasprotein phosphatase 2A and protein kinase C were not involved.

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