Literature DB >> 2903104

Immunocytochemical analysis of the regeneration of myofibrils in long-term cultures of adult cardiomyocytes of the rat.

M E Eppenberger1, I Hauser, T Baechi, M C Schaub, U T Brunner, C A Dechesne, H M Eppenberger.   

Abstract

Dissociated adult rat ventricular cardiomyocytes obtained from hearts by retrograde perfusion with collagenase were investigated in long-term cultures. Myofibril regeneration, isoprotein transition of alpha- and beta-myosin heavy chain (MHC), and M-band localization of M-creatine kinase in the reconstituting heart cells were studied. Myofibril formation was demonstrated by the use of antibodies against either cardiac C-protein or myomesin as early differentiation markers. Four days after plating, small myofibrils could be identified in attached cells in a perinuclear fashion; later in culture the cells displayed various shapes and myofibril distribution. Frequently a patchy distribution of myofibrils within the extending peripheral processes could be observed. Colocalization of sarcomeres and phalloidin-stained F-actin filament bundles was demonstrated by double fluorescence staining and by the use of high intensifying video microscopy and computerized image processing. The immunofluorescence distribution of alpha- and beta-MHC isoproteins in newly isolated and cultured cardiomyocytes changed from 100% alpha-MHC and 70% beta-MHC in rod-shaped cells to about 100% beta-MHC and 70% alpha-MHC in spread out cultured cells. This shift was corroborated by a relative gradual decline in alpha-MHC at the expense of increasing amounts of beta-MHC with time in culture as assessed by sodium dodecyl sulfate gel electrophoresis of total cell homogenates. In addition, whereas rod-shaped newly isolated cardiomyocytes showed a clear M-band association of M-creatine kinase as found in adult heart tissue, adult cultivated spread out cells did not show a cross-striated pattern after incubation with antibody. Taken together, these observations suggest that adult cardiomyocytes not only undergo extensive morphological transitions in long-term cultures, but also generate new myofibrillar structures lacking M-creatine kinase and containing the beta-MHC, thus fitting the characteristics of fetal myofibrils. These results indicate a change from the adult terminally differentiated to a less differentiated state of the cardiac cells in culture.

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Year:  1988        PMID: 2903104     DOI: 10.1016/0012-1606(88)90408-3

Source DB:  PubMed          Journal:  Dev Biol        ISSN: 0012-1606            Impact factor:   3.582


  31 in total

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Review 3.  Cardiomyogenic stem and progenitor cell plasticity and the dissection of cardiopoiesis.

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4.  Remodelling of adult cardiac muscle cells in culture: dynamic process of disorganization and reorganization of myofibrils.

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Journal:  J Muscle Res Cell Motil       Date:  1996-06       Impact factor: 2.698

5.  Immunohistochemical analysis of the adaptation of adult guinea-pig cardiomyocytes in long-term cultures and in cocultures with cardiac neurons: a novel model for studies of myocardial function.

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7.  Cocultures of fetal and adult cardiomyocytes yield rhythmically beating rod shaped heart cells from adult rats.

Authors:  D Weisensee; T Seeger; A Bittner; J Bereiter-Hahn; W Schoeppe; I Löw-Friedrich
Journal:  In Vitro Cell Dev Biol Anim       Date:  1995-03       Impact factor: 2.416

8.  Adult cardiac muscle cells in long-term serum-free culture: myofibrillar organization and expression of myosin heavy chain isoforms.

Authors:  A C Nag; M L Lee; J R Kosiur
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