The Optimal Oxygen Equilibrium Curve: A Comparison Between Environmental Hypoxia and Anemia

SYNOPSIS. Internal hypoxia in vertebrates occurs during anemia,when blood oxygen (0₂) carrying capacity is reduced, or duringexposure to environmental hypoxia. In non-altitude adapted vertebrates,exposure to environmental hypoxia results in a change in bloodO₂ affinity which, in some cases is beneficial to tissue O₂delivery. In contrast, the elevation in blood O₂ carrying capacityobserved in almost all vertebrates is always beneficial to tissueO₂ delivery (assuming no large changes in blood viscosity) andmay be more important than changes in blood O₂ affinity in maintainingtissue O₂ delivery. Experimental anemia in vertebrates results in a decrease inblood O₂ affinity which is always beneficial to tissue O₂ delivery.The reduction in affinity is brought about by an increase inthe organic phosphate to hemoglobin ratio (NTP:Hb) within thered cell. In fish NTP:Hb decreases during environmental hypoxiabut increases during anemia indicating that NTP regulation isquite different between these treatments despite the similarityof these treatments at the tissue level.     

Physiological Adaptations of Crayfish to the Hypoxic Environment

SYNOPSIS. Crayfish routinely encounter waters of reduced oxygentension, resulting in a broad array of behavioral and physiologicalresponses. Many animals when faced with this stress will simplyremove themselves from the irritating environment through voluntarymigration. When an animal, either by choice or through physicalconstraints remains in a hypoxic environment it must compensatefor the reduction in O₂ availability. Many crayfish have theability to maintain oxygen consumption independent of waterPo₂ down to some critical level; below this the animal can nolonger maintain normoxic levels of aerobic metabolism. Regulationof oxygen uptake is thought to be due to a hypoxia-induced hyperventilationalong with an increase in hemocyanin O₂ affinity and an improvementin the ability of the respiratory surfaces to transfer O₂. Crayfishexposed to a reduction in water oxygen also show a strong bradycardia,which is compensated for by an increase in stroke volume, resultingin a maintenance of cardiac output. The adaptive advantage ofthis response is uncertain. As water Po₂ drops crayfish havebeen shown to redistribute cardiac output, presumably throughthe action of the cardioarterial valves. Hemolymph is shuntedto the anterior end of the animal, resulting in a greater perfusionof nervous tissue. The animals' ability to detect changes inwater Po₂ appear to result from O₂ sensitive receptors locatedon the gills or in the branchiocardiac veins. The integratedphysiological response toward environmental hypoxia allows thecrayfish to not only deal with the stress but to maintain activity.     

Reactive oxygen species formation in the transition to hypoxia in skeletal muscle

Many tissues produce reactive oxygen species (ROS) during reoxygenation after hypoxia or ischemia; however, whether ROS are formed during hypoxia is controversial. We tested the hypothesis that ROS are generated in skeletal muscle during exposure to acute hypoxia before reoxygenation. Isolated rat diaphragm strips were loaded with dihydrofluorescein-DA (Hfluor-DA), a probe that is oxidized to fluorescein (Fluor) by intracellular ROS. Changes in fluorescence due to Fluor, NADH, and FAD were measured using a tissue fluorometer. The system had a detection limit of 1 µM H₂O₂ applied to the muscle superfusate. When the superfusion buffer was changed rapidly from 95% O₂ to 0%, 5%, 21%, or 40% O₂, transient elevations in Fluor were observed that were proportional to the rise in NADH fluorescence and inversely proportional to the level of O₂ exposure. This signal could be inhibited completely with 40 µM ebselen, a glutathione peroxidase mimic. After brief hypoxia exposure (10 min) or exposure to brief periods of H₂O₂, the fluorescence signal returned to baseline. Furthermore, tissues loaded with the oxidized form of the probe (Fluor-DA) showed a similar pattern of response that could be inhibited with ebselen. These results suggest that Fluor exists in a partially reversible redox state within the tissue. When Hfluor-loaded tissues were contracted with low-frequency twitches, Fluor emission and NADH emission were significantly elevated in a way that resembled the hypoxia-induced signal. We conclude that in the transition to low intracellular PO₂, a burst of intracellular ROS is formed that may have functional implications regarding skeletal muscle O₂-sensing systems and responses to acute metabolic stress. dihydrofluorescein; tissue fluorometer; ebselen; N-acetylcysteine; rat     

Oxygen Transport in the Avian Egg at High Altitude

Oxygen transport to avian embryo tissues occurs by three steps,two of which are driven by diffusion. This results in a seriesof stepwise decrements in PO₂ between atmosphere and tissue.The PO₂ decrements for embryos of the domestic fowl incubatedat different altitudes are used here to examine potential adaptationsto hypobanc hypoxia. With exposure to moderate hypoxia embryosof the domestic fowl appear to maintain adequate tissue oxygenation.Adaptive adjustments in the shell, shell membranes and chorioallantoiscomplex were not observed. However, hemoglobin O₂ affinity wasincreased and preliminary evidence suggests a redistributionof blood flow to maintain adequate oxygenation in higher priorityareas of embryonic tissue. At severe hypoxia, embryos of thedomestic fowl show decreased O₂ consumption, embryo mass andlengthened incubition period. Thus at severe hypoxin the embryoof the domestic fowl does not appear to provide a realisticmodel. Evidence from avian embryos of species native to highaltitude suggest that they are able to maintain adequate tissueoxygenation even at severe hypoxia. Preliminary evidence suggeststhat some of the blood vascular system and tissue level adaptationspresent in the chicken embryo are also present in species nativeto high altitude. One of these, an increase in embryonic hemoglobin-O₂affinity which is physiologically mediated in the chicken embryois genetically-based in the embryo of the native high-altitudespecies.     

A system for measuring phytoplankton photosynthesis in a defined light field with an oxygen electrode

A system is described for the precise continuous measurementof oxygen consumption and photo-synthetic oxygen evolution ina well defined light field with a polarographic oxygen electrode.The procedure uses a parallel light beam to irradiate samples,a relatively short pathlength and temperature regulation. Maximalsensitivity of the O₂-mcasurement is 1.4 µmol O₂/mV at20°C. The O₂-chamber and the O₂-amplifier are presentedin full detail together with a typical recorder tracing of aphotosynthesis-irradiance curve.     

Quantifying the sensitivity of barley seed germination to oxygen, abscisic acid, and gibberellin using a population-based threshold model

Barley (Hordeum vulgare L.) seeds (grains) exhibit dormancyat maturity that is largely due to the presence of the glumellae(hulls) that reduce the availability of oxygen (O₂) to the embryo.In addition, abscisic acid (ABA) and gibberellins (GAS) interactwith O₂ to regulate barley seed dormancy. A population-basedthreshold model was applied to quantify the sensitivities ofseeds and excised embryos to O₂, ABA, and GA, and to their interactiveeffects. The median O₂ requirement for germination of dormantintact barley seeds was 400-fold greater than for excised embryos,indicating that the tissues enclosing the embryo markedly limitO₂ penetration. However, embryo O₂ thresholds decreased by anotherorder of magnitude following after-ripening. Thus, increasesin both permeability of the hull to O₂ and embryo sensitivityto O₂ contribute to the improvement in germination capacityduring after-ripening. Both ABA and GA had relatively smalleffects on the sensitivity of germination to O₂, but ABA andGA thresholds varied over several orders of magnitude in responseto O₂ availability, with sensitivity to ABA increasing and sensitivityto GA decreasing with hypoxia. Simple additive models of O₂–ABAand O₂–GA interactions required consideration of theseO₂ effects on hormone sensitivity to account for actual germinationpatterns. These quantitative and interactive relationships amongO₂, ABA, and GA sensitivities provide insight into how dormancyand germination are regulated by a combination of physical (O₂diffusion through the hull) and physiological (ABA and GA sensitivities)factors. Key words: Abscisic acid, barley, germination, gibberellin, Hordeum vulgare L., model, oxygen, sensitivity Received 2 August 2007; Revised 14 November 2007 Accepted 19 November 2007     

Lactate efflux from exercising human skeletal muscle: role of intracellular PO2

It remainscontroversial whether lactate formation during progressive dynamicexercise from submaximal to maximal effort is due to muscle hypoxia. Tostudy this question, we used direct measures of arterial and femoralvenous lactate concentration, a thermodilution blood flow technique,phosphorus magnetic resonance spectroscopy (MRS), and myoglobin (Mb)saturation measured by ¹H nuclearMRS in six trained subjects performing single-leg quadriceps exercise.We calculated net lactate efflux from the muscle and intracellularPO₂ with subjects breathing room airand 12% O₂. Data were obtained at50, 75, 90, and 100% of quadriceps maximalO₂ consumption at each fraction ofinspired O₂. Mb saturation wassignificantly lower in hypoxia than in normoxia [40 ± 3 vs. 49 ± 3% (SE)] throughout incremental exercise to maximalwork rate. With the assumption of aPO₂ at which 50% of Mb-binding sitesare bound with O₂ of 3.2 Torr,Mb-associated PO₂ averaged 3.1 ± 0.3 and 2.3 ± 0.2 Torr in normoxia and hypoxia, respectively. Netblood lactate efflux was unrelated to intracellular PO₂ across the range of incrementalexercise to maximum (r = 0.03 and 0.07 in normoxia and hypoxia, respectively) but linearly related toO₂ consumption(r = 0.97 and 0.99 in normoxia andhypoxia, respectively) with a greater slope in 12%O₂. Net lactate efflux was alsolinearly related to intracellular pH(r = 0.94 and 0.98 in normoxia andhypoxia, respectively). These data suggest that with increasing workrate, at a given fraction of inspiredO₂, lactate efflux is unrelated tomuscle cytoplasmic PO₂, yet theefflux is higher in hypoxia. Catecholamine values from comparablestudies are included and indicate that lactate efflux in hypoxia may bedue to systemic rather than intracellular hypoxia.

     

Effect of 2,4-dinitrophenol on the hypometabolic response to hypoxia of conscious adult rats

Saiki, Chikako, and Jacopo P. Mortola. Effect of2,4-dinitrophenol on the hypometabolic response to hypoxia of conscious adult rats. J. Appl. Physiol. 83(2):537-542, 1997.During acute hypoxia, a hypometabolic response iscommonly observed in many newborn and adult mammalian species. Wehypothesized that, if hypoxic hypometabolism were entirely a regulatedresponse with no limitation in O₂availability, pharmacological uncoupling of the oxidativephosphorylation should raise O₂consumption(O₂) bysimilar amounts in hypoxia and normoxia. Metabolic, ventilatory, andcardiovascular measurements were collected from conscious rats in airand in hypoxia, both before and after intravenous injection of themitochondrial uncoupler 2,4-dinitrophenol (DNP). In hypoxia (10%O₂ breathing, 60% arterialO₂ saturation),O₂, as measured by anopen-flow technique, was less than in normoxia (~80%). SuccessiveDNP injections (6 mg/kg, 4 times) progressively increasedO₂ in both normoxia andhypoxia by similar amounts. Body temperature slightly increased innormoxia, whereas it did not change in hypoxia. The DNP-stimulatedO₂ during hypoxia couldeven exceed the control normoxic value. A single DNP injection (17 mg/kg iv) had a similar metabolic effect; it also resulted inhypotension and a drop in systemic vascular resistance. We concludethat pharmacological stimulation ofO₂ counteracts theO₂ drop determined byhypoxia and stimulates O₂not dissimilarly from normoxia. Hypoxic hypometabolism is likely toreflect a regulated process of depression of thermogenesis, with nolimitation in cellular O₂availability.

     

Physiological and hypoxic O2 tensions rapidly regulate NO production by stimulated macrophages

Nitric oxide (NO) production by inducible NO synthase (iNOS) is dependent on O₂ availability. The duration and degree of hypoxia that limit NO production are poorly defined in cultured cells. To investigate short-term O₂-mediated regulation of NO production, we used a novel forced convection cell culture system to rapidly (response time of 1.6 s) and accurately (±1 Torr) deliver specific O₂ tensions (from <1 to 157 Torr) directly to a monolayer of LPS- and IFN-stimulated RAW 264.7 cells while simultaneously measuring NO production via an electrochemical probe. Decreased O₂ availability rapidly (30 s) and reversibly decreased NO production with an apparent K_mO₂ of 22 (SD 6) Torr (31 µM) and a V_max of 4.9 (SD 0.4) nmol·min^–1·10^–6 cells. To explore potential mechanisms of decreased NO production during hypoxia, we investigated O₂-dependent changes in iNOS protein concentration, iNOS dimerization, and cellular NO consumption. iNOS protein concentration was not affected (P = 0.895). iNOS dimerization appeared to be biphasic [6 Torr (P = 0.008) and 157 Torr (P = 0.258) >36 Torr], but it did not predict NO production. NO consumption was minimal at high O₂ and NO tensions and negligible at low O₂ and NO tensions. These results are consistent with O₂ substrate limitation as a regulatory mechanism during brief hypoxic exposure. The rapid and reversible effects of physiological and pathophysiological O₂ tensions suggest that O₂ tension has the potential to regulate NO production in vivo. inducible nitric oxide synthase; substrate limitation; nitric oxide consumption     

Physiological energetics of the protobranch bivalve <Emphasis Type="Italic">Yoldia hyperborea</Emphasis> in a cold ocean environment

Yoldia hyperborea is a deposit-feeding circumpolar protobranch that also inhabits muddy sediments of the cold water boreal system of Conception Bay, Newfoundland, Canada. Little is known about this species, despite its wide distribution and frequent high density in the benthos. The present work deals with oxygen consumption and ammonia excretion under cold ambient conditions. Y. hyperborea showed low basal metabolism [0.051 ml O₂ h^у·(g dry weight)^у, T=у°C] and low ammonia excretion rates [4.212 µg·NH₄-N·h^у·(g dry weight)^у, T=у°C]. Low metabolic activity could prove a useful strategy during periods of low food availability. In addition, Y. hyperborea was able to regulate its O₂ consumption rate at very low pO₂ levels, which may be advantageous for a species that may experience periods of hypoxia.     

Root Respiration and Carbohydrate Status of Two Wheat Genotypes in Response to Hypoxia

To investigate root respiration and carbohydrate status in relationto waterlogging or hypoxia tolerance, root respiration rateand concentrations of soluble sugars in leaves and roots weredetermined for two wheat (Triticum aestivum L.) genotypes differingin waterlogging-tolerance under hypoxia (5% O₂) and subsequentresumption of full aeration. Root and shoot growth were reducedby hypoxia to a larger extent for waterlogging-sensitive Coker9835. Root respiration or oxygen consumption rate declined withhypoxia, but recovered after 7 d of resumption of aeration.Respiration rate was greater for sensitive Coker 9835 than fortolerant Jackson within 8 d after hypoxia. The concentrationsof sucrose, glucose and fructose decreased in leaves for bothgenotypes under hypoxia. The concentration of these sugars inroots, however, increased under hypoxia, to a greater degreefor Jackson. An increase in the ratio of root sugar concentrationto shoot sugar concentration was found for Jackson under hypoxicconditions, suggesting that a large amount of carbohydrate waspartitioned to roots under hypoxia. The results indicated thatroot carbohydrate supply was not a limiting factor for rootgrowth and respiration under hypoxia. Plant tolerance to waterloggingof hypoxia appeared to be associated with low root respirationor oxygen consumption rate and high sugar accumulation underhypoxic conditions.Copyright 1995, 1999 Academic Press Oxygen consumption rate, sugar accumulation, Triticum aestivum L., waterlogging tolerance     

Regeneration of Ribulose 1,5-bisphosphate and Ribulose 1,5-bisphosphate carboxylase/oxygenase Activity Associated with Lack of Oxygen Inhibition of Photosynthesis at Low Temperature

The nature of the lack of oxygen inhibition of C₃-photosynthesisat low temperature was investigated in white clover (Trifoliumrepens L.). Detached leaves were brought to steady-state photosynthesisin air (34 Pa p(CO²), 21 kPa p(O₂), balance N₂) at temperaturesof 20°C and 8°C, respectively. Net photosynthesis, ribulose1,5-bisphosphate (RuBP) and ATP contents, and ribulose 1,5-bisphosphatecarboxylase/oxygenase (RuBPCO) activities were followed beforeand after changing to 2·0 kPa p(O₂). At 20°C, lowering p(O₂) increased net photosynthesis by37%. This increase corresponded closely with the increase expectedfrom the effect on the kinetic properties of RuBPCO. Conversely,at 8°C net photosynthesis rapidly decreased following adecrease in p(O₂) and then increased again reaching a steady-statelevel which was only 7% higher than at 21 kPa p(O₂). The steady-staterates of RuBP and associated ATP consumption were both estimatedto have decreased. ATP and RuBP contents decreased by 18% and33% respectively, immediately after the change in p(O₂) suggestingthat RuBP regeneration was reduced at low p(O₂) due to reducedphotophosphorylation. Subsequently, RuBP content increased again.Steady-state RuBP content at 2·0 kPa p(O₂) was 24% higherthan at 21 kPa p(O₂). RuBPCO activity decreased by 22%, indicatingcontrol of steady-state RuBP consumption by RuBPCO activity. It is suggested that lack of oxygen inhibition of photosynthesisat low temperature is due to decreased photophosphorylationat low temperature and low p(O₂). This may be due to assimilateaccumulation within the chloroplasts. Decreased photophosphorylationseems to decrease RuBP synthesis and RuBPCO activity, possiblydue to an acidification of the chloroplast stroma. Key words: Oxygen inhibition, photosynthesis, ribulose bisphosphate carboxylase/oxygenase     

Depressed ventilatory response to hypoxia in hypothermic newborn piglets: role of glutamate

To evaluatewhether changes in extracellular glutamate (Glu) levels in the centralnervous system could explain the depressed hypoxic ventilatory responsein hypothermic neonates, 12 anesthetized, paralyzed, and mechanicallyventilated piglets <7 days old were studied. The Glu levels in thenucleus tractus solitarius obtained by microdialysis, minute phrenicoutput (MPO), O₂ consumption, arterial blood pressure, heart rate, and arterial blood gases weremeasured in room air and during 15 min of isocapnic hypoxia (inspiredO₂ fraction = 0.10) at braintemperatures of 39.0 ± 0.5°C [normothermia (NT)]and 35.0 ± 0.5°C [hypothermia (HT)]. During NT, MPO increased significantly during hypoxia and remained above baseline. However, during HT, there was a marked decrease in MPOduring hypoxia (NT vs. HT, P < 0.03). Glu levels increased significantly in hypoxia during NT;however, this increase was eliminated during HT(P < 0.02). A significant linearcorrelation was observed between the changes in MPO and Glu levelsduring hypoxia (r = 0.61, P < 0.0001). Changes in pH, arterialPO₂, O₂ consumption, arterial bloodpressure, and heart rate during hypoxia were not different between theNT and HT groups. These results suggest that the depressed ventilatoryresponse to hypoxia observed during HT is centrally mediated and inpart related to a decrease in Glu concentration in the nucleus tractussolitarius.

     

System-specific O2 sensitivity of the tandem pore domain K+ channel TASK-1

Hypoxic inhibition of TASK-1, a tandem pore domain background K⁺ channel, provides a critical link between reduced O₂ levels and physiological responses in various cell types. Here, we examined the expression and O₂ sensitivity of TASK-1 in immortalized adrenomedullary chromaffin (MAH) cells. In physiological (asymmetrical) K⁺ solutions, 3 µM anandamide or 300 µM Zn²⁺ inhibited a strongly pH-sensitive current. Under symmetrical K⁺ conditions, the anandamide- and Zn²⁺-sensitive K⁺ currents were voltage independent. These data demonstrate the functional expression of TASK-1, and cellular expression of this channel was confirmed by RT-PCR and Western blotting. At concentrations that selectively inhibit TASK-1, anandamide and Zn²⁺ were without effect on the magnitude of the O₂-sensitive current or the hypoxic depolarization. Thus TASK-1 does not contribute to O₂ sensing in MAH cells, demonstrating the failure of a known O₂-sensitive K⁺ channel to respond to hypoxia in an O₂-sensing cell. These data demonstrate that, ultimately, the sensitivity of a particular K⁺ channel to hypoxia is determined by the cell, and we propose that this is achieved by coupling distinct hypoxia signaling systems to individual channels. Importantly, these data also reiterate the indirect O₂ sensitivity of TASK-1, which appears to require the presence of an intracellular mediator. hypoxia; background K⁺ channels; TASK-1; MAH cells     

Native, not nitrated, cytochrome c and mitochondria-derived hydrogen peroxide drive osteoclast apoptosis

Two unresolved aspects of the role of mitochondria-derived cytochrome c in apoptosis are whether there is a separate pool of cytochrome c within mitochondria that participates in the activation of apoptosis and whether a chemically modified cytochrome c drives apoptosis. These questions were investigated using osteoclasts, because they are rich in mitochondria and because osteoclast apoptosis is critical in bone metabolism regulation. H₂O₂ production was increased during culture, preceding cytochrome c release; both processes occurred anterior to apoptosis. With the addition of a mitochondrial uncoupler, H₂O₂ production and apoptosis were blocked, indicating the prominent role of mitochondria-derived H₂O₂. Trapping H₂O₂-derived hydroxyl radical decreased apoptosis. Cytosolic cytochrome c was originated from a single mitochondrial compartment, supporting a common pool involved in respiration and apoptosis, and it was chemically identical to the native form, with no indication of oxidative or nitrative modifications. Protein levels of Bcl-2 and Bc-xL were decreased before apoptosis, whereas expression of wild-type Bcl-2 repressed apoptosis, confirming that cytochrome c release is critical in initiating apoptosis. Cytosolic cytochrome c participated in activating caspase-3 and -9, both required for apoptosis. Collectively, our data indicate that the mitochondria-dependent apoptotic pathway is one of the major routes operating in osteoclasts. reactive oxygen species; nitric oxide; free radicals; caspase     

Dormancy in Seeds of Charlock: IV. INTERRELATIONSHIPS OF GROWTH, OXYGEN SUPPLY AND CONCENTRATION OF INHIBITOR

Respiration measurements were made over a period of 24 h at25 °C on seeds and excised embryos maintained in Warburgflasks with partial pressures of oxygen ranging from 0 to 1atm. In the initial phase (0 to 4 h), the rate of oxygen uptake(Q_O2 of excised embryos increased linearly with external oxygenconcentration (C_O from 0 to 0.1 atm O₂ from 0.1 to 0.2 atm O₂the relation was curvilinear, and from 0.2 to 1.0 atm O₂ uptakewas independent of concentration. In later stages the relationbetween Q_O2 and C_o changed, and from 20 to 24 h the rate ofoxygen uptake increased with concentration to 1.0 atm O₂. Thechanges with time were associated with increase in rate of respiration,increase in cell size and cell number, and the oxidation offats. The decline in concentration of oxygen from the surfaceto the centre of embryos was calculated to be relatively smallat each external oxygen concentration. Althugh the rate of diffusionfailed to keep pace with consumption, the main parameters whichdetermined the internal oxygen status of the embryos were thesurface concentrations and the permeability of the seed coat.The resistance of the seed coat to diffusion of oxygen was foundto be very high, the coefficient of diffusion being about 10^–7mm² s^–1. The concentration of oxygen and in air were estimatedto be approximately 0.04 and 0.02 atm O₂, respectively. Sincea smaller concentration of oxygen (0.012 atm O₂) in the tissueswas found to be sufficient for growth, the dormancy of the seedswas not due to lack of oxygen. Dormancy appeared to be due tothe activity of growth-inhibiting substances, the concentrationof which increased with decrease in oxygen supply; below 0.1atm O₂ their rate of production increased with decrease in theoxygen concentration of the tissues. They accumulated withinthe testas of dormant seeds and prevented cell elongation. Extractsof the inhibitory substances were partially purifield by partitioningthe aqueous fraction with ether and separating chromatographically.The active principle(s) was not abscisic acid ((+)—AbscisinII, ‘Dormin’) or the mustard oil, allylisothiocyanate.     

Respiratory plasticity in response to changes in oxygen supply and demand

Aerobic organisms maintain O₂ homeostasis by responding to changesin O₂ supply and demand in both short and long time domains.In this review, we introduce several specific examples of respiratoryplasticity induced by chronic changes in O₂ supply (environmentalhypoxia or hyperoxia) and demand (exercise-induced and temperature-inducedchanges in aerobic metabolism). These studies reveal that plasticityoccurs throughout the respiratory system, including modificationsto the gas exchanger, respiratory pigments, respiratory muscles,and the neural control systems responsible for ventilating thegas exchanger. While some of these responses appear appropriate(e.g., increases in lung surface area, blood O₂ capacity, andpulmonary ventilation in hypoxia), other responses are potentiallyharmful (e.g., increased muscle fatigability). Thus, it maybe difficult to predict whole-animal performance based on theplasticity of a single system. Moreover, plastic responses maydiffer quantitatively and qualitatively at different developmentalstages. Much of the current research in this field is focusedon identifying the cellular and molecular mechanisms underlyingrespiratory plasticity. These studies suggest that a few keymolecules, such as hypoxia inducible factor (HIF) and erythropoietin,may be involved in the expression of diverse forms of plasticitywithin and across species. Studying the various ways in whichanimals respond to respiratory challenges will enable a betterunderstanding of the integrative response to chronic changesin O₂ supply and demand.     

Effect of reduced oxygen tension on chondrogenesis and osteogenesis in adipose-derived mesenchymal cells

Recent studies have demonstrated that adipose-derived mesenchymal cells (AMCs) offer great promise for cell-based therapies because of their ability to differentiate toward bone, cartilage, and fat. Given that cartilage is an avascular tissue and that mesenchymal cells experience hypoxia during prechondrogenic condensation in endochondral ossification, the goal of this study was to understand the influence of oxygen tension on AMC differentiation into bone and cartilage. In vitro chondrogenesis was induced using a three-dimensional micromass culture model supplemented with TGF-1. Collagen II production and extracellular matrix proteoglycans were assessed with immunohistochemistry and Alcian blue staining, respectively. Strikingly, micromasses differentiated in reduced oxygen tension (2% O₂) showed markedly decreased chondrogenesis. Osteogenesis was induced using osteogenic medium supplemented with retinoic acid or vitamin D and was assessed with alkaline phosphatase activity and mineralization. AMCs differentiated in both 21 and 2% O₂ environments. However, osteogenesis was severely diminished in a low-oxygen environment. These data demonstrated that hypoxia strongly inhibits in vitro chondrogenesis and osteogenesis in AMCs. cartilage; bone     

Variation in the Specificity Factor of C3 Higher Plant Rubiscos Determined by the Total Consumption of Ribulose-P2

The specificity factors for ribulose 1, 5-bisphosphate carboxylase/oxygenase(rubisco) from six species of photosynthetic organisms are compared.The values were determined by measuring the oxygen uptake duringthe total consumption of ribulose-P₂ in the presence of variousconcentrations of O₂ and CO₂. The specificity factors determinedin this way were similar to values previously published; smallbut significant differences were found between the specificityfactors of rubisco from C₃ higher plant species. Key words: Specificity factor, total consumption, partitioning, carboxylase oxygenase ratios, ribulose bisphosphate carboxylase, rubisco