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    Measurement of Water Transport During Freezing in Mammalian Liver Tissue: Part II—The Use of Differential Scanning Calorimetry

    Source: Journal of Biomechanical Engineering:;1998:;volume( 120 ):;issue: 005::page 559
    Author:
    R. V. Devireddy
    ,
    J. C. Bischof
    DOI: 10.1115/1.2834745
    Publisher: The American Society of Mechanical Engineers (ASME)
    Abstract: There is currently a need for experimental techniques to assay the biophysical response (water transport or intracellular ice formation, IIF) during freezing in the cells of whole tissue slices. These data are important in understanding and optimizing biomedical applications of freezing, particularly in cryosurgery. This study presents a new technique using a Differential Scanning Calorimeter (DSC) to obtain dynamic and quantitative water transport data in whole tissue slices during freezing. Sprague-Dawley rat liver tissue was chosen as our model system. The DSC was used to monitor quantitatively the heat released by water transported from the unfrozen cell cytoplasm to the partially frozen vascular/extracellular space at 5°C/min. This technique was previously described for use in a single cell suspension system (Devireddy, et al. 1998). A model of water transport was fit to the DSC data using a nonlinear regression curve-fitting technique, which assumes that the rat liver tissue behaves as a two-compartment Krogh cylinder model. The biophysical parameters of water transport for rat liver tissue at 5°C/min were obtained as Lpg = 3.16 x 10−13 m3 /Ns (1.9 μm/min-atm), ELp = 265 kJ/mole (63.4 kcal/mole), respectively. These results compare favorably to water transport parameters in whole liver tissue reported in the first part of this study obtained using a freeze substitution (FS) microscopy technique (Pazhayannur and Bischof, 1997). The DSC technique is shown to be a fast, quantitative, and reproducible technique to measure dynamic water transport in tissue systems. However, there are several limitations to the DSC technique: (a) a priori knowledge that the biophysical response is in fact water transport, (b) the technique cannot be used due to machine limitations at cooling rates greater than 40°C/min, and (c) the tissue geometric dimensions (the Krogh model dimensions) and the osmotically inactive cell volumes Vb , must be determined by low-temperature microscopy techniques.
    keyword(s): Freezing , Biological tissues , Differential scanning calorimetry , Liver , Water , Microscopy , Dimensions , Suspension systems , Cooling , Machinery , Cylinders , Ice , Low temperature , Biomedicine , Fittings AND Heat ,
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      Measurement of Water Transport During Freezing in Mammalian Liver Tissue: Part II—The Use of Differential Scanning Calorimetry

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    http://yetl.yabesh.ir/yetl1/handle/yetl/120025
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    • Journal of Biomechanical Engineering

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    contributor authorR. V. Devireddy
    contributor authorJ. C. Bischof
    date accessioned2017-05-08T23:55:51Z
    date available2017-05-08T23:55:51Z
    date copyrightOctober, 1998
    date issued1998
    identifier issn0148-0731
    identifier otherJBENDY-26004#559_1.pdf
    identifier urihttp://yetl.yabesh.ir/yetl/handle/yetl/120025
    description abstractThere is currently a need for experimental techniques to assay the biophysical response (water transport or intracellular ice formation, IIF) during freezing in the cells of whole tissue slices. These data are important in understanding and optimizing biomedical applications of freezing, particularly in cryosurgery. This study presents a new technique using a Differential Scanning Calorimeter (DSC) to obtain dynamic and quantitative water transport data in whole tissue slices during freezing. Sprague-Dawley rat liver tissue was chosen as our model system. The DSC was used to monitor quantitatively the heat released by water transported from the unfrozen cell cytoplasm to the partially frozen vascular/extracellular space at 5°C/min. This technique was previously described for use in a single cell suspension system (Devireddy, et al. 1998). A model of water transport was fit to the DSC data using a nonlinear regression curve-fitting technique, which assumes that the rat liver tissue behaves as a two-compartment Krogh cylinder model. The biophysical parameters of water transport for rat liver tissue at 5°C/min were obtained as Lpg = 3.16 x 10−13 m3 /Ns (1.9 μm/min-atm), ELp = 265 kJ/mole (63.4 kcal/mole), respectively. These results compare favorably to water transport parameters in whole liver tissue reported in the first part of this study obtained using a freeze substitution (FS) microscopy technique (Pazhayannur and Bischof, 1997). The DSC technique is shown to be a fast, quantitative, and reproducible technique to measure dynamic water transport in tissue systems. However, there are several limitations to the DSC technique: (a) a priori knowledge that the biophysical response is in fact water transport, (b) the technique cannot be used due to machine limitations at cooling rates greater than 40°C/min, and (c) the tissue geometric dimensions (the Krogh model dimensions) and the osmotically inactive cell volumes Vb , must be determined by low-temperature microscopy techniques.
    publisherThe American Society of Mechanical Engineers (ASME)
    titleMeasurement of Water Transport During Freezing in Mammalian Liver Tissue: Part II—The Use of Differential Scanning Calorimetry
    typeJournal Paper
    journal volume120
    journal issue5
    journal titleJournal of Biomechanical Engineering
    identifier doi10.1115/1.2834745
    journal fristpage559
    journal lastpage569
    identifier eissn1528-8951
    keywordsFreezing
    keywordsBiological tissues
    keywordsDifferential scanning calorimetry
    keywordsLiver
    keywordsWater
    keywordsMicroscopy
    keywordsDimensions
    keywordsSuspension systems
    keywordsCooling
    keywordsMachinery
    keywordsCylinders
    keywordsIce
    keywordsLow temperature
    keywordsBiomedicine
    keywordsFittings AND Heat
    treeJournal of Biomechanical Engineering:;1998:;volume( 120 ):;issue: 005
    contenttypeFulltext
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