Immunofluorescent Patterns of Dissociated Rat Embryo Cerebral Cells during Development in Surface Culture: Distinctive Reactions with Neurite and Perikaryon Cell Membranes

Yavin, Ziva; Yavin, Ephraïm

doi:10.1159/000112550

Cited by 22 publications

(6 citation statements)

References 15 publications

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“…These increases were accompanied by a dramatic shift from simple gangliosides (GM3 and GD3) to more complex species (GM1, GD1a, GD1b, GT1b). A similar increase in the quantity and in the complexity of gangliosides has also been observed during differentiation in cultured neurons of different origin and in mouse neural precursor cells [89,90,[92][93][94][95][96][97]. In humans, the phase of rapid ganglioside increase started from the sixth month of gestation and reached the maximum value at about 5 years of age [91].…”

Section: Role Of Sphingolipids In the Development And Function Of Nersupporting

confidence: 53%

Deregulated Sphingolipid Metabolism and Membrane Organization in Neurodegenerative Disorders

et al. 2010

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Sphingolipids are polar membrane lipids present as minor components in eukaryotic cell membranes. Sphingolipids are highly enriched in nervous cells, where they exert important biological functions. They deeply affect the structural and geometrical properties and the lateral order of cellular membranes, modulate the function of several membrane-associated proteins, and give rise to important intra- and extracellular lipid mediators. Sphingolipid metabolism is regulated along the differentiation and development of the nervous system, and the expression of a peculiar spatially and temporarily regulated sphingolipid pattern is essential for the maintenance of the functional integrity of the nervous system: sphingolipids in the nervous system participate to several signaling pathways controlling neuronal survival, migration, and differentiation, responsiveness to trophic factors, synaptic stability and synaptic transmission, and neuron-glia interactions, including the formation and stability of central and peripheral myelin. In several neurodegenerative diseases, sphingolipid metabolism is deeply deregulated, leading to the expression of abnormal sphingolipid patterns and altered membrane organization that participate to several events related to the pathogenesis of these diseases. The most impressive consequence of this deregulation is represented by anomalous sphingolipid-protein interactions that are at least, in part, responsible for the misfolding events that cause the fibrillogenic and amyloidogenic processing of disease-specific protein isoforms, such as amyloid beta peptide in Alzheimer's disease, huntingtin in Huntington's disease, alpha-synuclein in Parkinson's disease, and prions in transmissible encephalopathies. Targeting sphingolipid metabolism represents today an underexploited but realistic opportunity to design novel therapeutic strategies for the intervention in these diseases.

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Section: Role Of Sphingolipids In the Development And Function Of Nersupporting

confidence: 53%

Deregulated Sphingolipid Metabolism and Membrane Organization in Neurodegenerative Disorders

et al. 2010

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“…The procedure employed for D2 staining of viable cells has been described previously by Yavin and Yavin (1978). In brief, cells grown on polylysine-precoated coverslips were reacted with the antiserum raised against excised D2 precipitates obtained by immunoelectrophoresis.…”

Section: Indirect Immunojluorescence Stainingmentioning

confidence: 99%

Nervous System‐Specific Proteins in Developing Rat Cerebral Cells in Culture

Bock

Yavin

Jørgensen

et al. 1980

Journal of Neurochemistry

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The nervous system-specific proteins; synaptin, D1, D2, D3, glial fibrillary acidic protein (GFA) and 14-3-2, were quantified in dissociated cerebral cells from the foetal rat brain at various times of growth in culture. By approximately 1 week in culture, the neuronal membrane markers synaptin, D1, D2, and D3 could all be demonstrated. A maximum concentration of 10-20% for synaptin, D1, and D3 and 160% for D2, in comparison with the levels in adult forebrain, was attained during the 2nd week in vitro. The astroglial gliofilament marker GFA increased continuously, reaching by 38 days of cultivation an 18-fold higher level than the concentration in adult forebrain. The neuronal cytoplasm marker 14-3-2 could be demonstrated in trace amounts, and only after more than 1 week in vitro. Neuronal cell bodies and processes stained by indirect immunofluorescence using an anti-D2 serum were strongly fluorescent after 1 week in vitro. Immunofluorescence staining for GFA revealed a cytoplasmic filamentous network in perinuclear areas and processes of, presumably, astroblasts.

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“…For example, the total ganglioside content increased several fold from the embryonic stages to the postnatal life in vertebrate brain [2][3][4], as well as during in vitro differentiation of cultured neurons of different origin and in mouse neural precursor cells [2,3,[5][6][7][8][9], with a concomitant shift from simple gangliosides (GM3 and GD3) to more complex species (GM1, GD1a, GD1b, GT1b). Sphingomyelin (SM) content also dramatically increased during in vitro differentiation of rat cerebellar neurons [10].…”

Section: Introductionmentioning

confidence: 99%

Secondary Alterations of Sphingolipid Metabolism in Lysosomal Storage Diseases

et al. 2011

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In several neurodegenerative diseases, sphingolipid metabolism is deeply deregulated, leading to the expression of abnormal membrane sphingolipid patterns and altered plasma membrane organization. In this paper, we review the potential importance of these alterations to the pathogenesis of these diseases and focus the reader's attention on some secondary alterations of sphingolipid metabolism that have been sporadically reported in the literature. Moreover, we present a detailed analysis of the lipid composition of different central nervous system and extraneural tissues from the acid sphingomyelinase-deficient mouse, the animal model for Niemann-Pick disease type A, characterized by the accumulation of sphingomyelin. Our data show an unexpected, tissue specific selection of the accumulated molecular species of sphingomyelin, and an accumulation of GM3 and GM2 gangliosides in both neural and extraneural tissues, that cannot be solely explained by the lack of acid sphingomyelinase.

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Immunofluorescent Patterns of Dissociated Rat Embryo Cerebral Cells during Development in Surface Culture: Distinctive Reactions with Neurite and Perikaryon Cell Membranes

Cited by 22 publications

References 15 publications

Deregulated Sphingolipid Metabolism and Membrane Organization in Neurodegenerative Disorders

Deregulated Sphingolipid Metabolism and Membrane Organization in Neurodegenerative Disorders

Nervous System‐Specific Proteins in Developing Rat Cerebral Cells in Culture

Secondary Alterations of Sphingolipid Metabolism in Lysosomal Storage Diseases

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