L Rieke scite author profile

L Rieke

3Publications

29Citation Statements Received

7Citation Statements Given

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Gesellschaft für Hochschulforschung

Publications

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Cellular localization of endothelial alkaline phosphatase reaction product and enzyme protein in the myocardium.

Schultz-Hector¹,

Balz²,

Böhm³

et al. 1993

J Histochem Cytochem.

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Myocardial capillary endothelial cells, arteriolar endothelial cells, and the arterial adventitia show positive alkaline phosphatase (AP) enzyme reaction and immunoreactivity in both rat and human heatts. In guinea pigs, however, capillary endothelial staining is discontinuous and arterial adventitia is negative. The ultrastructural correlate of discontinuous capillary staining is a pronounced labeling of pericytes in guinea pig heart and relatively weak endothelial staining. In rat and human heart, enzyme reaction products are localized mainly on plasma membranes and cytotic vesicles of endothelial cells.Comparison of two strains of rat reveals a more dense deposition of enzyme reaction product along the luminal and particularly along the abluminal plasma membrane of SpragueDawley rats than of Wistar rats. Quantitative analysis of immunogold labeled anti-AP antibody density confiims the pronounced polarity of capillary endothelial cell labeling in Sprague-Dawley rats. More than 80% of total endothelial AP protein in Sprague-Dawley rats is localized over the abluminal plasma membrane and basal lamina, as compared with less than 30% in Wistar rats. Moreover, the total endothelial cell labeling is almost sixfold higher in SpragueDawley than in Wistar rats. Total endothelial labeling and proportion of labeling on the abluminal endothelial plasma membrane in human hearts is intermediate between the two strains of rat. The strain and species differences in enzyme distribution could provide important information concerning enzyme function. (JHstochem Cytochem 41:1813-1821, 1993)

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Postembedding Ultrastructural in Situ Hybridization on Ultrathin Cryosections and LR White Resin Sections

Mandry¹,

Murray²,

Rieke³

et al. 1993

Ultrastructural Pathology

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A method was developed for nonisotopic postembedding in situ hybridization (ISH) on ultrathin sections of frozen and of LR White resin-embedded material at the electron microscopic level. The method was successfully applied to detect Epstein-Barr virus (EBV) DNA in the P3HR1 human Burkitt's lymphoma cell line. Each of the steps in the procedure had to be optimized for successful ISH on the frozen and LR White sections. The most important conditions are described. Predigestion with proteinase K was only necessary with the resin sections. Sections were treated with sodium hydroxide to denature target DNA and were hybridized with a biotinylated probe. The probe was best detected with a primary antibody to biotin followed by a gold-conjugated secondary antibody. EBV DNA was detected in the nucleus and/or cytoplasm in 10% to 20% of P3HR1 cells. A similar percentage of cells in thin L-sectioned material prepared by routine methods showed virus particles at different stages of maturation.

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Identification Of The Position Of Selected Cells In Large Sections Of Oriented Material Following Electron Microscopy

Rieke

1986

Stain Technology

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L Rieke

Cellular localization of endothelial alkaline phosphatase reaction product and enzyme protein in the myocardium.

Postembedding Ultrastructural in Situ Hybridization on Ultrathin Cryosections and LR White Resin Sections

Identification Of The Position Of Selected Cells In Large Sections Of Oriented Material Following Electron Microscopy

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