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• Taiwan Society for Mitochondrial Research and Medicine  + (The '''Taiwan Society for Mitochondrial Research and Medicine''' (TSMRM) is a member of [[Asian Society for Mitochondrial Research and Medicine|ASMRM]].)
• USB port  + (The '''USB port''' describes the connection between O2k and Computer. With the USB cable connected, select '''USB port''' in the [[Connection window]]. Depending on the O2k series, it is possible to connect with a '''USB port''' or [[Serial port]].)
• Abscissa  + (The '''abscissa''' is the horizontal axis … The '''abscissa''' is the horizontal axis ''x'' of a rectangular two-dimensional graph with the [[ordinate]] ''y'' as the vertical axis. Values ''X'' are placed horizontally from the origin.</br></br>See [[Abscissal X/Y regression |Abscissal ''X''/''Y'' regression]].[[Abscissal X/Y regression |Abscissal ''X''/''Y'' regression]].)
• Accuracy  + (The '''accuracy''' of a method is the degree of agreement between an individual test result generated by the method and the true value.)
• Activity  + (The '''activity''' (relative activity) is … The '''activity''' (relative activity) is a dimensionless quantity related to the concentration or partial pressure of a dissolved substance. The activity of a dissolved substance B equals the [[concentration]], ''c''_B [mol·L^-1], at high dilution divided by the unit concentration, ''c''° = 1 mol·L^-1: </br> ''a''_B = ''c''_B/''c''°</br>This simple relationship applies frequently to substances at high dilutions <10 mmol·L^-1 (<10 mol·m^-3). In general, the concentration of a [[solute]] has to be corrected for the activity coefficient (concentration basis), ''γ''_B,</br> ''a''_B = ''γ''_B·''c''_B/''c''°</br>At high dilution, ''γ''_B = 1. In general, the relative activity is defined by the [[chemical potential]], ''µ''_B</br> ''a''_B = exp[(''µ''_B-''µ''°)/''RT'']potential]], ''µ''_B ''a''_B = exp[(''µ''_B-''µ''°)/''RT''])
• Adenine nucleotide translocase  + (The '''adenine nucleotide translocator''', … The '''adenine nucleotide translocator''', ANT, exchanges [[ADP]] for [[ATP]] in an electrogenic antiport across the inner mt-membrane. The ANT is inhibited by [[atractyloside]], [[carboxyatractyloside|carboxyatractyloside]] and [[bongkrekik acid]]. The ANT is a component of the [[phosphorylation system]].[[phosphorylation system]].)
• Advantage of preprints  + (The '''advantages of preprints''', the excitement and concerns about the role that preprints can play in disseminating research findings in the life sciences are discussed by N Bhalla (2016).)
• Aerobic  + (The '''aerobic''' state of metabolism is d … The '''aerobic''' state of metabolism is defined by the presence of oxygen (air) and therefore the potential for oxidative reactions (ox) to proceed, particularly in [[oxidative phosphorylation]] (OXPHOS). Aerobic metabolism (with involvement of oxygen) is contrasted with [[anaerobic]] metabolism (without involvement of oxygen): Whereas anaerobic ''metabolism'' may proceed in the absence or presence of oxygen (anoxic or oxic ''conditions''), aerobic ''metabolism'' is restricted to oxic ''conditions''. Below the [[critical oxygen pressure]], aerobic ATP production decreases.[[critical oxygen pressure]], aerobic ATP production decreases.)
• Amount of substance  + (The '''amount of substance''' ''n'' is a b … The '''amount of substance''' ''n'' is a base physical quantity, and the corresponding SI unit is the [[mole]] [mol]. Amount of substance (sometimes abbreviated as 'amount' or 'chemical amount') is proportional to the number ''N''_''X'' of specified elementary entities ''X'', and the universal proportionality constant is the reciprocal value of the [[Avogadro constant]] ([[Bureau International des Poids et Mesures_2019_The International System of Units (SI) |SI]]),</br> ''n''_''X'' = ''N''_''X''·''N''_A^-1</br></br>''n''_''X'' contained in a system can change due to internal and external transformations,</br> d''n''_''X'' = d_i''n''_''X'' + d_e''n''_''X''</br></br>In the absence of nuclear reactions, the amount of any atom is conserved, ''e.g.'', for carbon d_i''n''_C = 0. This is different for chemical substances or ionic species which are produced or consumed during the [[advancement]] of a reaction r, </br>:::: [[File:Amount dn.png|100px]]</br>A change in the amount of ''X''_''i'', d''n''_''i'', in an open system is due to both the internal formation in chemical transformations, d_r''n''_''i'', and the external transfer, d_e''n''_''i'', across the system boundaries. d''n''_''i'' is positive if ''X''_''i'' is formed as a product of the reaction within the system. d_e''n''_''i'' is negative if ''X''_''i'' flows out of the system and appears as a product in the surroundings ([[Cohen 2008 IUPAC Green Book]]).[Cohen 2008 IUPAC Green Book]]).)
• Amplitude  + (The '''amplitude''' of the [[absorbance spectrum]] … The '''amplitude''' of the [[absorbance spectrum]] can be described in terms of the [[absorbance]] differences between the characteristic peaks (absorbance maxima) and troughs (absorbance minima) (see [[absorbance spectrum]]) for substances present in the sample.[[absorbance spectrum]]) for substances present in the sample.)
• Background state  + (The '''background state''' Y (background r … The '''background state''' Y (background rate ''Y_X'') is the non-activated or inhibited respiratory state at background rate, which is low in relation to the higher rate ''Z_X'' in the [[reference state]] Z. The transition from the background state to the reference state is a step change. A [[metabolic control variable]] ''X'' (substrate, activator) is added to the background state to stimulate flux to the level of the reference state. Alternatively, the metabolic control variable ''X'' is an inhibitor, which is present in the background state Y, but absent in the reference state Z. The background state is the baseline of a single step in the definition of the [[flux control efficiency]]. In a sequence of step changes, the common [[baseline state]] is the state of lowest flux in relation to all steps, which can be used as a [[baseline correction]].[[baseline correction]].)
• Baseline state  + (The '''baseline state''' in a sequence of … The '''baseline state''' in a sequence of step changes is the state of lowest flux in relation to all steps, which can be used as a [[baseline correction]]. Correction for [[residual oxygen consumption]], ROX, is an example where ROX is the baseline state. In a single step, the baseline state is equivalent to the [[background state]].[[background state]].)
• Bias  + (The '''bias''' is defined as the difference between the mean of the measurements and the reference value. In general, the measuring instrument calibration procedures should focus on establishing and correcting it.)
• Block temperature  + (The '''block temperature''' of the [[Oroboros O2k]] is the continuously measured temperature of the copper block, housing the two glass chambers of the O2k. The block temperature is recorded by [[DatLab]] as one of the O2k system channels.)
• Body mass excess  + (The '''body mass excess''', BME, is an ind … The '''body mass excess''', BME, is an index of obesity and as such BME is a lifestyle metric. The BME is a measure of the extent to which your actual [[body mass]], ''M'' [kg/x], deviates from ''M''° [kg/x], which is the reference body mass [kg] per individual [x] without excess body fat in the [[healthy reference population]], HRP. A balanced BME is BME° = 0.0 with a band width of -0.1 towards underweight and +0.2 towards overweight. The BME is linearly related to the [[body fat excess]].body fat excess]].)
• Body mass index  + (The '''body mass index''', BMI, is the rat … The '''body mass index''', BMI, is the ratio of body mass to height squared (BMI=''M''·''H''^-2), recommended by the WHO as a general indicator of underweight (BMI<18.5 kg·m^-2), overweight (BMI>25 kg·m^-2) and obesity (BMI>30 kg·m^-2). Keys et al (1972; see 2014) emphasized that 'the prime criterion must be the relative independence of the index from height'. It is exactly the dependence of the BMI on height - from children to adults, women to men, Caucasians to Asians -, which requires adjustments of BMI-cutoff points. This deficiency is resolved by the [[body mass excess]] relative to the [[healthy reference population]].althy reference population]].)
• Body mass  + (The '''body mass''' ''M'' is the mass ([[kilogram]] … The '''body mass''' ''M'' is the mass ([[kilogram]] [kg]) of an individual (object) [x] and is expressed in units [kg/x]. Whereas the body weight changes as a function of gravitational force (you are weightless at zero gravity; your floating weight in water is different from your weight in air), your mass is independent of gravitational force, and it is the same in air and water.orce, and it is the same in air and water.)
• Bound energy  + (The '''bound energy''' change in a closed … The '''bound energy''' change in a closed system is that part of the ''total'' [[energy]] change that is always bound to an exchange of [[heat]],</br></br> d''B'' = d''U'' - d''A'' [Eq. 1]</br></br> ∆''B'' = ∆''H'' - ∆''G'' [Eq. 2]</br></br>The ''free'' energy change (Helmoltz or Gibbs; d''A'' or d''G'') is the ''total'' energy change (total inner energy or enthalpy, d''U'' or d''H'') of a system minus the ''bound'' energy change.</br></br>Therefore, if a process occurs at [[equilibrium]], when d''G'' = 0 (at constant gas pressure), then d''H'' = d''B'', and at d_e''W'' = 0 (d''H'' = d_e''Q'' + d_e''W''; see [[energy]]) we obtain the definition of the bound energy as the heat change taking place in an equilibrium process (eq),</br></br> d''B'' = ''T''∙d''S'' = d_e''Q''_eq [Eq. 3]rocess (eq), d''B'' = ''T''∙d''S'' = d_e''Q''_eq [Eq. 3])
• Cell count and normalization in HRR  + (The '''cell count''' ''N''_{ce< … The '''cell count''' ''N''_ce is the number of cells, expressed in the abstract [[unit]] [x] (1 Mx = 10⁶ x). The ''elementary entity'' cell ''U''_ce [x] is the real unit, the 'single individual cell'. A cell count is the multitude or number ''N'' of cells, ''N''_ce = ''N''·''U''_ce ([[Gnaiger MitoFit Preprints 2020.4]]). Normalization of respiratory rate by cell count yields oxygen [[flow]] ''I''_O₂ expressed in units [amol·s^-1·x^-1] (=10^-18 mol·s^-1·x^-1).gt;} expressed in units [amol·s^-1·x^-1] (=10^-18 mol·s^-1·x^-1).)
• Chamber volume  + (The '''chamber volume''' of the O2k is 2.0 … The '''chamber volume''' of the O2k is 2.0 mL or 0.5 mL of aqueous medium with or without sample, excluding the volume of the stirrer and the volume of the capillary of the stopper (see: [[Cell count and normalization in HRR]]). A modular extension of the O2k, the [[O2k-sV-Module]], was specifically developed to perform high-resolution respirometry with reduced amounts of biological sample, and all components necessary for the smaller operation volume of 0.5 mL.or the smaller operation volume of 0.5 mL.)
• Charge number  + (The '''charge number''' of an ion ''X'' or … The '''charge number''' of an ion ''X'' or electrochemical reaction with unit stoichiometric number of ''X'' is the [[particle charge]] [C·x^-1] divided by the [[elementary charge]] [C·x^-1]. The particle charge ''Q''_{<u>''N''</u>''X''} is the charge per count of ions ''X'' or per ion ''X'' transferred in the reaction as defined in the reaction equation.ns ''X'' or per ion ''X'' transferred in the reaction as defined in the reaction equation.)
• Chemical potential  + (The '''chemical potential''' of a substanc … The '''chemical potential''' of a substance B, ''µ''_B [J/mol], is the partial derivative of Gibbs energy, ''G'' [J], per amount of B, ''n''_B [mol], at constant temperature, pressure, and composition other than that of B,</br> ''µ''_B = (∂''G''/∂''n''_B)_{''T'',''p'',''n<small>j''≠B</small>}</br>The chemical potential of a [[solute]] in solution is the sum of the standard chemical potential under defined standard conditions and a concentration ([[activity]])-dependent term,</br> ''µ''_B = ''µ''_B° + ''RT'' ln(''a''_B)</br>The standard state for the solute is refered to ideal behaviour at standard concentration, ''c''° = 1 mol/L, exhibiting infinitely diluted solution behaviour [1]. ''µ''_B° equals the standard molar Gibbs energy of formation, Δ_f''G''_B° [kJ·mol^-1]. The formation process of B is the transformation of the pure constituent elements to one mole of substance B, with all substances in their standard state (the most stable form of the element at 100 kPa (1 bar) at the specified temperature) [2].on of the pure constituent elements to one mole of substance B, with all substances in their standard state (the most stable form of the element at 100 kPa (1 bar) at the specified temperature) [2].)
• Comparison of respirometric methods  + (The '''comparison of respirometric methods''' provides the basis to evaluate different instrumental platforms and different [[mitochondrial preparations]], as a guide to select the best approach and to critically evaluate published results.)
• Critical oxygen pressure  + (The '''critical oxygen pressure''', ''p''& … The '''critical oxygen pressure''', ''p''_c, is defined as the partial oxygen pressure, ''p''_O2, below which [[aerobic]] catabolism (respiration or oxygen consumption) declines significantly. If [[anaerobic]] catabolism is activated simultaneously to compensate for lower aerobic ATP generation, then the '''[[limiting oxygen pressure]]''', ''p''_l, is equal to the ''p''_c. In many cases, however, the ''p''_l is substantially lower than the ''p''_c.y cases, however, the ''p''_l is substantially lower than the ''p''_c.)
• Cytochrome c control efficiency  + (The '''cytochrome ''c'' control efficiency … The '''cytochrome ''c'' control efficiency''' expresses the control of respiration by externally added [[cytochrome c | cytochrome ''c'']], c, as a fractional change of flux from substrate state CHNO to CHNOc. These fluxes are corrected for ''Rox'' and may be measured in the OXPHOS state or ET state, but not in the LEAK state. In this [[flux control efficiency]], CHNOc is the [[reference state]] with stimulated flux; CHNO is the [[background state]] with CHNO substrates, upon which c is added:</br> ''j''_{cyt ''c''} = (''J''_CHNOc-''J''_CHNO)/''J''_CHNOc.>CHNOc</sub>-''J''_CHNO)/''J''_CHNOc.)

• Data recording interval  + (The '''data recording interval''' is the t … The '''data recording interval''' is the time interval at which data is sampled with an instrument. In [[DatLab]] the data recording interval is set in the [[O2k control]] window. The system default value is 2 s. A lower data recording interval is selected for kinetic experiments, and when the volume-specific oxygen flux is high (>300 pmol O₂·s^-1·ml^-1).<br/>Technically, the O2k instrument (hardware) measures the sensor signal every 10ms (which is NOT the „data recording interval“). By the given data recording interval from DatLab (software) a discrete number of sensor signal points are taken to calculate an average value in the O2k (e.g. a data recording interval of 2 s can take 200 sensor signal points; a data recording interval of 0.5 s can take 50 sensor signal points). This average value is sent to DatLab and is recorded as a raw data point. However, there is a defined threshold: the O2k does not apply more than 200 sensor signal points to calculate the average for the raw data point. For example a data recording interval of 3 s could take 300 sensor signal points but only the 200 most recent sensor signal points are used for averaging.signal points but only the 200 most recent sensor signal points are used for averaging.)
• Dicarboxylate carrier  + (The '''dicarboxylate carrier''' is a transporter which catalyses the electroneutral exchange of [[malate]]^2- (or [[succinate]]^2-) for inorganic [[phosphate]], HPO₄^2-.)
• Energy charge  + (The '''energy charge''' of the adenylate s … The '''energy charge''' of the adenylate system or adenylate energy charge (AEC) has been defined by Atkinson and Walton (1967) as (ATP + ½ ADP)/(AMP + ADP + ATP). Wheather the AEC is a fundamental metabolic control parameter remains a controversial topic.l parameter remains a controversial topic.)
• Ergodynamic efficiency  + (The '''ergodynamic efficiency''', ''ε'' (c … The '''ergodynamic efficiency''', ''ε'' (compare [[thermodynamic efficiency]]), is a power ratio between the output power and the (negative) input power of an energetically coupled process. Since [[power]] [W] is the product of a [[flow]] and the conjugated thermodynamic [[force]], the ergodynamic efficiency is the product of an output/input flow ratio and the corresponding force ratio. The efficiency is 0.0 in a fully uncoupled system (zero output flow) or at level flow (zero output force). The maximum efficiency of 1.0 can be reached only in a fully (mechanistically) coupled system at the limit of zero flow at ergodynamic equilibrium. The ergodynamic efficiency of coupling between ATP production (DT phosphorylation) and oxygen consumption is the flux ratio of DT phosphorylation flux and oxygen flux (P»/O₂ ratio) multiplied by the corresponding force ratio. Compare with the [[OXPHOS-coupling efficiency]].OXPHOS-coupling efficiency]].)
• Extinction coefficient  + (The '''extinction coefficient''' (''ε'') of a substance is the [[absorbance]] of a 1 µmolar concentration over a 1 cm pathlength and is wavelength-dependent.)
• Gain  + (The '''gain''' is an amplification factor applied to an input signal to increase the output signal.)
• Glutamate-aspartate carrier  + (The '''glutamate-aspartate carrier''' cata … The '''glutamate-aspartate carrier''' catalyzes the electrogenic antiport of glutamate^- +H⁺ for aspartate^-. It is an important component of the malate-aspartate shuttle in many mitochondria. Due to the symport of glutamate^- + +H⁺, the glutamate-aspartate antiport is not electroneutal and may be impaired by [[uncoupling]]. [[Aminooxyacetate]] is an [[inhibitor]] of the glutamate-aspartate carrier.[[inhibitor]] of the glutamate-aspartate carrier.)
• Height of humans  + (The '''height of humans''', ''h'', is give … The '''height of humans''', ''h'', is given in SI units in meters [m]. Humans are countable objects, and the symbol and unit of the number of objects is ''N'' [x]. The average height of ''N'' objects is, ''H'' = ''h''/''N'' [m/x], where ''h'' is the heights of all ''N'' objects measured on top of each other. Therefore, the height per human has the unit [m·x^-1] (compare [[body mass]] [kg·x^-1]). Without further identifyer, ''H'' is considered as the standing height of a human, measured without shoes, hair ornaments and heavy outer garments., measured without shoes, hair ornaments and heavy outer garments.)
• Hexokinase  + (The '''hexokinase''' catalyzes the phosphorylation of D-glucose at position 6 by ATP to yield D-glucose 6-phosphate as well as the phosphorylation of many other hexoses like D-fructose, D-mannose, D-glucosamine.)
• Limiting oxygen pressure  + (The '''limiting oxygen pressure''', ''p''& … The '''limiting oxygen pressure''', ''p''_l, is defined as the partial oxygen pressure, ''p''_O2, below which [[anaerobic]] catabolism is activated to contribute to total ATP generation. The limiting oxygen pressure, ''p''_l, may be substantially lower than the '''[[critical oxygen pressure]]''', ''p''_c, below which [[aerobic]] catabolism (respiration or oxygen consumption) declines significantly.[[aerobic]] catabolism (respiration or oxygen consumption) declines significantly.)
• Membrane-bound ET pathway  + (The '''membrane-bound [[electron transfer pathway]] … The '''membrane-bound [[electron transfer pathway]] (mET pathway)''' consists in mitochondria mainly of [[respiratory complexes]] CI, CII, electron transferring flavoprotein complex (CETF), glycerophosphate dehydrogenase complex (CGpDH), and choline dehydrogenase, with [[convergent electron flow]] at the [[Q-junction]] (Coenzyme Q), and the two downstream respiratory complexes connected by cytochrome ''c'', CIII and CIV, with oxygen as the final electron acceptor. The mET-pathway is the terminal (downstream) module of the mitochondrial [[ET pathway]] and can be isolated from the ET-pathway in [[submitochondrial particles]] (SmtP).[[submitochondrial particles]] (SmtP).)
• Meter  + (The '''meter''', symbol m, is the SI unit … The '''meter''', symbol m, is the SI unit of the SI base quantity [[length]] ''l''. It is defined by taking the fixed numerical value of the speed of light ''c'' in vacuum to be 299 792 458 when expressed in the unit m·s⁻¹, where the second is defined in terms of the caesium frequency Δ''ν''_Cs.in terms of the caesium frequency Δ''ν''_Cs.)
• Mitochondrial ATP-sensitive K+ channel  + (The '''mitochondrial ATP-sensitive K⁺ channel''' (mtK_ATP or mitoK_ATP).)
• Mitochondrial free radical theory of aging  + (The '''mitochondrial free radical theory o … The '''mitochondrial free radical theory of aging''' goes back to Harman (1956) and ranks among the most popular theories of aging. It is based on postulates which are not unequivocally supported by observation (Bratic, Larsson 2013):</br>(i) Mitochondrial ROS production increases with age caused by progressive mitochondrial dysfunction;</br>(ii) antioxidat capacity declines with age;</br>(iii) mutations of somatic mtDNA accumulate during aging;</br>(iv) a vicious cycle occurs of increased ROS production caused by mtDNA mutations and degenerated mt-function, and due to ROS-induced ROS production.on, and due to ROS-induced ROS production.)
• Mitochondrial inner membrane  + (The '''mitochondrial inner membrane''' mtI … The '''mitochondrial inner membrane''' mtIM is the structure harboring the membrane-bound [[electron transfer system]] ETS including the respiratory complexes working as [[hydrogen ion pump]]s, the mt-[[phosphorylation system]] including the hydrogen ion pump [[ATP synthase]], several substrate transporters involved in the [[electron transfer pathway]], and a variety of other ion pumps that carry [[proton]] charge (Ca²⁺, Mg²⁺). The [[protonmotive force]] is the electrochemical potential difference across the mtIM generated by the [[hydrogen ion pumps]] of the .[[hydrogen ion pumps]] of the .)
• Mitochondrial matrix  + (The '''mitochondrial matrix''' (mt-matrix) … The '''mitochondrial matrix''' (mt-matrix) is enclosed by the mt-inner membrane mtIM. The terms mitochondrial matrix space or mitochondrial lumen are used synonymously. The mt-matrix contains the enzymes of the [[tricarboxylic acid cycle]], [[fatty acid oxidation]] and a variety of enzymes that have cytosolic counterparts (e.g. [[glutamate dehydrogenase]], [[malic enzyme]]). Metabolite concentrations, such as the concentrations of fuel substrates, adenylates (ATP, ADP, AMP) and redox systems (NADH), can be very different in the mt-matrix, the mt-intermembrane space, and the cytosol. The finestructure of the gel-like mt-matrix is subject of current research. mt-matrix is subject of current research.)
• Mitochondrial membrane potential  + (The '''mitochondrial membrane potential''' … The '''mitochondrial membrane potential''' difference, mtMP or Δ''Ψ''_p⁺ = Δ_el''F''_{<u>''e''</u>p⁺}, is the electric part of the protonmotive [[force]], Δp = Δ_m''F''_{<u>''e''</u>H⁺}.</br></br>:::: Δ_el''F''_{<u>''e''</u>p⁺} = Δ_m''F''_{<u>''e''</u>H⁺} - Δ_d''F''_{<u>''e''</u>H⁺}</br>:::: Δ''Ψ''_p⁺ = Δp - Δ''µ''_H+·(''z''_H⁺·''F'')^-1</br></br>Δ''Ψ''_p⁺ is the potential difference across the mitochondrial inner membrane (mtIM), expressed in the electric unit of volt [V]. Electric force of the mitochondrial membrane potential is the electric energy change per ‘motive’ charge or per charge moved across the transmembrane potential difference, with the number of ‘motive’ charges expressed in the unit coulomb [C].t;p⁺</sub> is the potential difference across the mitochondrial inner membrane (mtIM), expressed in the electric unit of volt [V]. Electric force of the mitochondrial membrane potential is the electric energy change per ‘motive’ charge or per charge moved across the transmembrane potential difference, with the number of ‘motive’ charges expressed in the unit coulomb [C].)
• Mitochondrial outer membrane  + (The '''mitochondrial outer membrane''' is … The '''mitochondrial outer membrane''' is the incapsulating membrane which is osmotically not active and contains the cytochrome ''b''₅ enzyme similar to that found in the endoplasmatic reticulum, the translocases of the outer membrane, monoaminooxidase, the palmitoyl-CoA synthetase and carnytil-CoA transferase 1.lmitoyl-CoA synthetase and carnytil-CoA transferase 1.)
• Motive unit  + (The '''motive unit''' [MU] is the variable … The '''motive unit''' [MU] is the variable SI unit in which the [[motive entity]] (transformant) of a transformation is expressed, which depends on the energy transformation under study and on the chosen [[format]]. Fundamental MU for electrochemical transformations are:</br></br>* MU = x, for the particle or molecular format, <u>''N''</u></br>* MU = mol, for the chemical or molar format, <u>''n''</u></br>* MU = C, for the electrical format, <u>''e''</u>; </br></br>For the [[protonmotive force]] the motive entity is the proton with charge number ''z''=1. The protonmotive force is expressed in the electrical or molar format with MU J/C=V or J/mol=Jol, respectively. The conjugated flows, ''I'', are expressed in corresponding electrical or molar formats, C/s = A or mol/s, respectively.</br></br>The [[charge number]], ''z'', has to be considered in the conversion of motive units (compare Table below), if a change not only of units but a transition between the entity [[elementary charge]] and an entity with charge number different from unity is involved (''e.g.'', O₂ with ''z''=4 in a redox reaction). The ratio of elementary charges per reacting O₂ molecule (''z''_{O<small>2</small>}=4) is multiplied by the elementary charge (''e'', coulombs per proton), which yields coulombs per O₂ [C∙x^-1]. This in turn is multiplied with the [[Avogadro constant]], ''N''_A (O₂ molecules per mole O₂ [x∙mol^-1]), thus obtaining for ''zeN''_A the ratio of elementary charges [C] per amount of O₂ [mol^-1]. The conversion factor for O₂ is 385.94132 C∙mmol^-1., thus obtaining for ''zeN''_A the ratio of elementary charges [C] per amount of O₂ [mol^-1]. The conversion factor for O₂ is 385.94132 C∙mmol^-1.)
• Ordinate  + (The '''ordinate''' is the vertical axis ''y'' of a rectangular two-dimensional graph with the [[abscissa]] ''x'' as the horizontal axis. Values ''Y'' are placed vertically from the origin. See [[Ordinary Y/X regression |Ordinary ''Y''/''X'' regression]].)
• Oxycaloric equivalent  + (The '''oxycaloric equivalent''' is the the … The '''oxycaloric equivalent''' is the theoretically derived enthalpy change of the oxidative catabolic reactions per amount of oxygen respired, Delta_k''H''_O2, ranging from -430 to -480 kJ/mol O₂. The oxycaloric equivalent is used in [[indirect calorimetry]] to calculate the theoretically expected metabolic heat flux from the respirometrically measured metabolic oxygen flux. [[Calorespirometric ratio|Calorimetric/respirometric ratios]] (CR ratios; heat/oxygen flux ratios) are experimentally determined by [[calorespirometry]]. A CR ratio more exothermic than the oxycaloric equivalent of -480 kJ/mol indicates the simultaneous involvement of aerobic and anaerobic mechanisms of energy metabolism.ltaneous involvement of aerobic and anaerobic mechanisms of energy metabolism.)
• Oxygen signal  + (The '''oxygen signal''' of the [[Oroboros O2k]] … The '''oxygen signal''' of the [[Oroboros O2k]] is transmitted from the electrochemical polarographic oxygen sensor ([[OroboPOS]]) for each of the two O2k-chambers to [[DatLab]]. The primary signal is a current [µA] which is converted into a voltage [V] (raw signal), and calibrated in SI units for amount of substance concentration [µmol·L^-1 or µM]. For technical reasons, the raw signal is given in [V] (DatLab 7 and previous) or [µA] (DatLab 8). The value of the raw signal is the same, independent of the displayed unit ([V] or [µA]). In the following sections, only [µA] is used for information on the raw signal, but the same values in [V] apply for the raw signal when using DL7 or previous versions.or the raw signal when using DL7 or previous versions.)
• Oxygen solubility factor  + (The '''oxygen solubility factor''' of the … The '''oxygen solubility factor''' of the incubation medium, ''F''_M, expresses the effect of the salt concentration on [[oxygen solubility]] relative to pure water. In mitochondrial respiration medium [[MiR05]], [[MiR05-Kit]] and [[MiR06]], ''F''_M is 0.92 (determined at 30 and 37 °C) and in culture media is 0.89 (at 37 °C). ''F''_M varies depending on the temperature and composition of the medium. To determine the FM based on the oxygen concentration, specific methods and equipment are needed (see references Rasmussen HN, Rasmussen UF 2003 in [https://wiki.oroboros.at/index.php/MiPNet06.03_POS-calibration-SOP MiPNet06.03]). For other media, ''F''_M may be estimated using Table 4 in [https://wiki.oroboros.at/index.php/MiPNet06.03_POS-calibration-SOP MiPNet06.03]. For this purpose KCl based media can be described as "seawater" of varying salinity. The original data on sucrose and KCl-media (Reynafarje et al 1985), however, have been critizesed as artefacts and the ''F''_M of 0.92 is suggested in the temperature range of 10 °C to 40 °C as for MiR05._M of 0.92 is suggested in the temperature range of 10 °C to 40 °C as for MiR05.)
• Oxygen solubility  + (The '''oxygen solubility''', ''S''<sub& … The '''oxygen solubility''', ''S''_O₂ [µM/kPa] = [(µmol·L^-1)/kPa], expresses the oxygen concentration in solution in equilibrium with the [[oxygen pressure]] in a gas phase, as a function of temperature and composition of the solution. The inverse of oxygen solubility is related to the [[activity]] of dissolved oxygen. The oxygen solubility in solution, ''S''_O₂(aq), depends on temperature and the concentrations of solutes in solution, whereas the dissolved oxygen concentration at equilibrium with air, ''c''_O₂^*(aq), depends on ''S''_O₂(aq), barometric pressure and temperature. ''S''_O₂(aq) in pure water is 10.56 µM/kPa at 37 °C and 12.56 µM/kPa at 25 °C. At standard [[barometric pressure]] (100 kPa), ''c''_O₂^*(aq) is 207.3 µM at 37 °C (19.6 kPa partial oxygen pressure) or 254.7 µM at 25 °C (20.3 kPa partial oxygen pressure). In [[MiR05]] and serum, the corresponding saturation concentrations are lower due to the [[oxygen solubility factor]]: 191 and 184 µM at 37 °C or 234 and 227 µM at 25 °C.lubility factor]]: 191 and 184 µM at 37 °C or 234 and 227 µM at 25 °C.)
• PH  + (The '''pH value''' or pH is the negative o … The '''pH value''' or pH is the negative of the base 10 logarithm of the [[activity]] of [[proton]]s (hydrogen ions, H⁺). A [[pH electrode]] reports the pH and is sensitive to the activity of H⁺. In dilute solutions, the hydrogen ion activity is approximately equal to the hydrogen ion [[concentration]]. The symbol pH stems from the term ''potentia hydrogenii''.[[concentration]]. The symbol pH stems from the term ''potentia hydrogenii''.)