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A list of all pages that have property "Description" with value "'''Mitochondrial Physiology - Historical Collection''' '''Aims''' The". Since there have been only a few results, also nearby values are displayed.

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List of results

  • Metrology  + ('''Metrology''' is the science of measurement, including all aspects both theoretical and practical with reference to measurements, whatever their uncertainty, and in whatever fields of science or technology they occur [SOURCE: VIM:1993, 2.2].)
  • Microplates  + ('''Microplate''' readers allow large numbe … '''Microplate''' readers allow large numbers of sample reactions to be assayed in well format microtitre plates. The most common microplate format used in academic research laboratories or clinical diagnostic laboratories is 96-well (8 by 12 matrix) with a typical reaction volume between 100 and 200 Β΅L per well. a wide range of applications involve the use of [[fluorescence]] measurements , although they can also be used in conjunction with [[absorbance]] measurements.[absorbance]] measurements.)
  • Microxia  + ('''Microxia''' (deep hypoxia) is obtained when trace amounts of O<sub>2</sub> exert a stimulatory effect on respiration above the level where metabolism is switched to a purely [[anaerobic]] mode.)
  • MitoFit protocols  + ('''MitoFit protocols''' are moderated by t … '''MitoFit protocols''' are moderated by the [[MitoFit moderators]] (MitoFit team), either as protocols with direct reference to publications available to the scientific communicty, or protocols additionally described and made available in Bioblast with full information on authors (including contact details), author contributions, and editor (moderator) in charge. This aims at a comprehensive [[MitoFit data repository]], which will require global input and cooperation.will require global input and cooperation.)
  • MitoFit registered project  + ('''MitoFit registered projects''' are anno … '''MitoFit registered projects''' are announced with reference to [[MitoFit protocols]] as [[publicly deposited protocols]]. Project registration is a two-phase process. Guidelines will be defined. (''1'') Pre-registration of a project requires submission to a MitoFit moderator (editor), including protocol details with reference to MitoPedia protocols, or with submission of protocols for publication (Open Access) in MitoPedia. The MitoFit (Bioblast) editors will edit the submitted protocols (layout) and insert into Bioblast submitted pre-registrations and protocols. (''2'') MitoFit moderators (editors) will set up a [[MitoFit accreditation panel]], in which the registrant will be included (perhaps not in the long run, to avoid conflict of interests) and/or for which the registrant can suggest delegates (compare peer review). Accredited [[MitoFit protocols]] are labelled as [[MitoFit accredited]], and the pre-registered MitoFit project becomes labelled and listed as '''MitoFit registered project''' (MitoFit accredited). This is possible before (advance registration), during progress, and after completion of a study (post-registration). A MitoFit registered project receives a code for feeding data into the [[MitoFit data repository]].[[MitoFit data repository]].)
  • MitoKit-CII/Malonate-nv  + ('''MitoKit-CII/Malonate-nv''' (diacetoxyme … '''MitoKit-CII/Malonate-nv''' (diacetoxymethyl malonate) is a plasma membrane-permeable prodrug (permeable malonate; Mnanv) that diffuses across the plasma membrane. Cleavage of diacetoxymethyl groups is mediated by intracellular esterases, thus releasing [[malonate]] in the intracellular space. Abliva #: 01-161-s2e intracellular space. Abliva #: 01-161-s2)
  • MitoKit-CII/Succinate-nv  + ('''MitoKit-CII/Succinate-nv''' (diacetoxym … '''MitoKit-CII/Succinate-nv''' (diacetoxymethyl succinate) is a plasma membrane-permeable prodrug (permeable succinate; Snv) that diffuses across the plasma membrane. Cleavage of diacetoxymethyl groups is mediated by intracellular esterases, thus releasing [[succinate]] in the intracellular space. Abliva #: 01-118-s4 intracellular space. Abliva #: 01-118-s4)
  • MitoSOX  + ('''MitoSOX<sup>TM</sup>''' is … '''MitoSOX<sup>TM</sup>''' is the version of the [[Dihydroethidium|hydroetidine]] designed to target mitochondria in live cells for the detection of [[superoxide]] (O<sub>2</sub><sup>β€’-</sup>). The oxidation of the compound by O<sub>2</sub><sup>β€’-</sup> is easily detected in the red spectrum. One of the advantages of MitoSOX<sup>TM</sup> is its selectivity for O<sub>2</sub><sup>β€’-</sup> but not for other [[Reactive oxygen species|reactive oxygen species]] or [[Reactive nitrogen species|reactive nitrogen species]]. </br>::::β€’ Readily '''oxidized by superoxide''' but not by other ROS- or RNS-generating systems</br>::::β€’ '''Absorption/emission maxima''': ~510/580 nm</br>::::β€’ Use for '''live cell imaging'''</br>::::β€’ Rapidly and selectively '''targeted to the mitochondria'''</br></br></br>'''MitoSOX<sup>TM</sup>''' has been widely used in life cell imaging but it is not free of problems and should be used cautiously. For example, it has been highlighted that the use of potentiometric dyes which accumulates into the mitochondria due to its moiety with [[Tetraphenylphosphonium]], confers a membrane potential sensitivity that creates a series of artifacts and problems not often considered.hosphonium]], confers a membrane potential sensitivity that creates a series of artifacts and problems not often considered.)
  • Mitochondria  + ('''Mitochondria''' (Greek ''mitos'': threa … '''Mitochondria''' (Greek ''mitos'': thread; ''chondros'': granule) are small structures within cells, which function in cell respiration as powerhouses or batteries. Mitochondria belong to the '''[[bioblasts]]''' of Richard Altmann. Abbreviation: mt, as generally used in mtDNA. Singular: mitochondrion (bioblast); plural: mitochondria (bioblasts).oblast); plural: mitochondria (bioblasts).)
  • MitoOx1  + ('''Mitochondrial respiration medium, MitoOx1,''' used by the Budapest groups for respirometry und Amplex Red trials.)
 ('''Mitochondrial Physiology - Historical Collection''' '''Aims''' The)
  • MiP-Collection  + ('''Mitochondrial Physiology - Historical C … '''Mitochondrial Physiology - Historical Collection'''</br></br>'''Aims'''</br></br>The growing '''''MiP-Collection''''' aims at preserving scientific instruments that are of historical importance in the field of bioenergetics and mitochondrial physiology. The fast turnover of scientific equipment makes obsolete even comparatively recent instrumentation. The Oroboros O2k was the first commercial mitochondrial respirometer using a computer for data acquisition. Today, [[chart recorder]]s are nearly forgotten. Due to limitations of storage space, unused scientific equipment is disposed of, despite its potential historical value. The disposal of some unique apparatus constitutes an irreversible loss to science and society, and to the continued appreciation of the foundations of our scientific discipline. </br></br>You may consider to make items of scientific historical interest in mitochondrial physiology available to the ''MiP-Collection''. These items of the ''MiP-Collection'' may specifically include historically valuable </br> </br>* equipment and accessories,</br>* books and symposium proceedings, </br>* reprint collections,</br>* pictures, slides, documents.ollections, * pictures, slides, documents.)
  • MiP03  + ('''Mitochondrial Preservation Medium, MiP03''', developed for preservation of [[isolated mitochondria]].)
  • Mitochondrial concentration  + ('''Mitochondrial concentration''' is ''C<sub>mtE</sub>'' = ''mtE''Β·''V''<sup>-1</sup> [mtEUΒ·m<sup>-3</sup>]. mt-Concentration is an experimental variable, dependent on sample concentration.)
  • Mitochondrial content  + ('''Mitochondrial content''' per object ''X'' is ''mtE<sub><u>N</u>X</sub>'' = ''mtE''Β·''N<sub>X</sub>''<sup>-1</sup> [mtEUΒ·x<sup>-1</sup>].)
  • Mitochondrial marker enzymes  + ('''Mitochondrial marker enzymes''' are enzymes that are specifically present in mitochondria, in the mt-matrix, the inner mt-membrane, the inter-membrane space, or the outer mt-membrane.)
  • Mitochondrial marker  + ('''Mitochondrial marker'''s are structural … '''Mitochondrial marker'''s are structural or functional properties that are specific for mitochondria. A structural mt-marker is the area of the inner mt-membrane or mt-volume determined stereologically, which has its limitations due to different states of swelling. If mt-area is determined by electron microscopy, the statistical challenge has to be met to convert area into a volume. When fluorescent dyes are used as mt-marker, distinction is necessary between mt-membrane potential dependent and independent dyes. mtDNA or cardiolipin content may be considered as a mt-marker. [[Mitochondrial marker enzymes]] may be determined as molecular (amount of protein) or functional properties (enzyme activities). Respiratory capacity in a defined respiratory state of a mt-preparation can be considered as a functional mt-marker, in which case respiration in other respiratory states is expressed as [[flux control ratio]]s. Β» [[Mitochondrial marker#Mitochondrial markers and expression of mitochondrial respiration| '''MiPNet article''']][Mitochondrial marker#Mitochondrial markers and expression of mitochondrial respiration| '''MiPNet article''']])
  • Mitochondrial competence  + ('''Mitochondrial metabolic competence''' i … '''Mitochondrial metabolic competence''' is the organelle's capacity to provide adequate amounts of ATP in due time, by adjusting the mt-membrane potential, mt-redox states and the ATP/ADP ratio according to the metabolic requirements of the cell.</br></br>The term '''mitochondrial competence''' is also known in a genetic context: Mammalian mitochondria possess a natural competence for DNA import.</br></br>'''''[[MitoCom_O2k-Fluorometer]]''''' is a '''Mitochondrial Competence''' network, the nucleus of which is formed by the K-Regio project ''[[MitoCom_O2k-Fluorometer|MitoCom Tyrol]]''.[[MitoCom_O2k-Fluorometer|MitoCom Tyrol]]''.)
  • Mitochondrial preparations  + ('''Mitochondrial preparations''' (mtprep) … '''Mitochondrial preparations''' (mtprep) are isolated mitochondria (imt), tissue homogenate (thom), mechanically or chemically permeabilized tissue (permeabilized fibers, pfi) or permeabilized cells (pce). In mtprep the plasma membranes are either removed (imt) or mechanically (thom) and chemically permeabilized (pfi), while mitochondrial functional integrity and to a large extent mt-structure are maintained in incubation media optimized to support mitochondrial physiological performance. According to this definition, submitochondrial particles (smtp) are not a mtprep, since mitochondrial structure is altered although specific mitochondrial functions are preserved.fic mitochondrial functions are preserved.)
  • Buffer Z  + ('''Mitochondrial respiration medium, Buffer Z''', described by [http://bioblast.at/index.php/Perry_2011_Biochem_J Perry 2011 Biochem J] For composition and comparison see: [[Mitochondrial respiration media: comparison]])
  • MiR05  + ('''Mitochondrial respiration medium, MiR05 … '''Mitochondrial respiration medium, MiR05''', developed for oxygraph incubations of [[mitochondrial preparations]]. Respiration of [[living cells]] may be assessed in MiR05 by adding pyruvate (P) as an external source. [[MiR06]] = MiR05 + catalase.</br>[[MiR05Cr]] = [[MiR05]] + creatine.[[MiR05]] + creatine.)
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