Tissue culture of human neurocytomas induces the expression of glial fibrilary acidic protein.

M Westphal; H Meissner; Jakob Matschke; H D Herrmann

Tissue culture of human neurocytomas induces the expression of glial fibrilary acidic protein.

Standard

Tissue culture of human neurocytomas induces the expression of glial fibrilary acidic protein. / Westphal, M; Meissner, H; Matschke, Jakob; Herrmann, H D.

in: J NEUROCYTOL, Jahrgang 27, Nr. 11, 11, 1998, S. 805-816.

Publikationen: SCORING: Beitrag in Fachzeitschrift/Zeitung › SCORING: Zeitschriftenaufsatz › Forschung › Begutachtung

Harvard

Westphal, M, Meissner, H, Matschke, J & Herrmann, HD 1998, 'Tissue culture of human neurocytomas induces the expression of glial fibrilary acidic protein.', J NEUROCYTOL, Jg. 27, Nr. 11, 11, S. 805-816. <http://www.ncbi.nlm.nih.gov/pubmed/10451427?dopt=Citation>

APA

Westphal, M., Meissner, H., Matschke, J., & Herrmann, H. D. (1998). Tissue culture of human neurocytomas induces the expression of glial fibrilary acidic protein. J NEUROCYTOL, 27(11), 805-816. [11]. http://www.ncbi.nlm.nih.gov/pubmed/10451427?dopt=Citation

Vancouver

Westphal M, Meissner H, Matschke J, Herrmann HD. Tissue culture of human neurocytomas induces the expression of glial fibrilary acidic protein. J NEUROCYTOL. 1998;27(11):805-816. 11.

Bibtex

@article{6c6407e2280943e5aa38e2082fc3ae92,

title = "Tissue culture of human neurocytomas induces the expression of glial fibrilary acidic protein.",

abstract = "Cell cultures were established from three human neurocytoma specimens (primary and recurrent). The phenotypic evolution was analyzed by immunocytology in different culture conditions in the presence and absence of serum including the addition of epidermal growth factor, rat caudate extract, retinoic acid, and N-acetyl cystein. The cells were grown on glass cover slides or an extracellular matrix (ECM) from bovine corneal endothelial cells. Immunostainings were performed after overnight incubation and were repeated after 5 and 10 days of culture. The cultures were compared to an oligoastrocytoma also arising at the foramen of Monro and an ependymoma of the frontal lateral ventricle, two tumors supposedly originating from the same tissue matrix as the neurocytoma. After overnight incubation, 90% of the neurocytoma cells were positive for A2B5 and synaptophysin. GFAP reactivity appeared in the periphery of cell processes in less than 1% of the cells. The staining patterns and morphology were nearly identical under the different culture conditions. After 5 days, almost all cells were strongly positive for GFAP, while the number of cells remaining positive for synaptophysin and A2B5 was unchanged from the earlier time point. Again, there were no fundamental differences between the incubation conditions. At this point, cultures maintained on ECM were compared to their counterparts on untreated glass cover slides with identical staining results, although many fewer cells had attached. An identical immuno-reactive pattern was found on day 10. In contrast to the neurocytoma cultures, there was an immediate strong GFAP signal in both the mixed glioma and the ependymoma. A2B5 was also positive, but synaptophysin was absent. Because the neurocytoma specimens were synaptophysin positive but GFAP negative by immunohistochemistry, it is concluded that neurocytomas may represent a human neuronoglial precursor tumor that switches its phenotype in culture to astroglial differentiation despite very diverse culture conditions.",

author = "M Westphal and H Meissner and Jakob Matschke and Herrmann, {H D}",

year = "1998",

language = "Deutsch",

volume = "27",

pages = "805--816",

number = "11",

}

RIS

TY - JOUR

T1 - Tissue culture of human neurocytomas induces the expression of glial fibrilary acidic protein.

AU - Westphal, M

AU - Meissner, H

AU - Matschke, Jakob

AU - Herrmann, H D

PY - 1998

Y1 - 1998

N2 - Cell cultures were established from three human neurocytoma specimens (primary and recurrent). The phenotypic evolution was analyzed by immunocytology in different culture conditions in the presence and absence of serum including the addition of epidermal growth factor, rat caudate extract, retinoic acid, and N-acetyl cystein. The cells were grown on glass cover slides or an extracellular matrix (ECM) from bovine corneal endothelial cells. Immunostainings were performed after overnight incubation and were repeated after 5 and 10 days of culture. The cultures were compared to an oligoastrocytoma also arising at the foramen of Monro and an ependymoma of the frontal lateral ventricle, two tumors supposedly originating from the same tissue matrix as the neurocytoma. After overnight incubation, 90% of the neurocytoma cells were positive for A2B5 and synaptophysin. GFAP reactivity appeared in the periphery of cell processes in less than 1% of the cells. The staining patterns and morphology were nearly identical under the different culture conditions. After 5 days, almost all cells were strongly positive for GFAP, while the number of cells remaining positive for synaptophysin and A2B5 was unchanged from the earlier time point. Again, there were no fundamental differences between the incubation conditions. At this point, cultures maintained on ECM were compared to their counterparts on untreated glass cover slides with identical staining results, although many fewer cells had attached. An identical immuno-reactive pattern was found on day 10. In contrast to the neurocytoma cultures, there was an immediate strong GFAP signal in both the mixed glioma and the ependymoma. A2B5 was also positive, but synaptophysin was absent. Because the neurocytoma specimens were synaptophysin positive but GFAP negative by immunohistochemistry, it is concluded that neurocytomas may represent a human neuronoglial precursor tumor that switches its phenotype in culture to astroglial differentiation despite very diverse culture conditions.

AB - Cell cultures were established from three human neurocytoma specimens (primary and recurrent). The phenotypic evolution was analyzed by immunocytology in different culture conditions in the presence and absence of serum including the addition of epidermal growth factor, rat caudate extract, retinoic acid, and N-acetyl cystein. The cells were grown on glass cover slides or an extracellular matrix (ECM) from bovine corneal endothelial cells. Immunostainings were performed after overnight incubation and were repeated after 5 and 10 days of culture. The cultures were compared to an oligoastrocytoma also arising at the foramen of Monro and an ependymoma of the frontal lateral ventricle, two tumors supposedly originating from the same tissue matrix as the neurocytoma. After overnight incubation, 90% of the neurocytoma cells were positive for A2B5 and synaptophysin. GFAP reactivity appeared in the periphery of cell processes in less than 1% of the cells. The staining patterns and morphology were nearly identical under the different culture conditions. After 5 days, almost all cells were strongly positive for GFAP, while the number of cells remaining positive for synaptophysin and A2B5 was unchanged from the earlier time point. Again, there were no fundamental differences between the incubation conditions. At this point, cultures maintained on ECM were compared to their counterparts on untreated glass cover slides with identical staining results, although many fewer cells had attached. An identical immuno-reactive pattern was found on day 10. In contrast to the neurocytoma cultures, there was an immediate strong GFAP signal in both the mixed glioma and the ependymoma. A2B5 was also positive, but synaptophysin was absent. Because the neurocytoma specimens were synaptophysin positive but GFAP negative by immunohistochemistry, it is concluded that neurocytomas may represent a human neuronoglial precursor tumor that switches its phenotype in culture to astroglial differentiation despite very diverse culture conditions.

M3 - SCORING: Zeitschriftenaufsatz

VL - 27

SP - 805

EP - 816

IS - 11

M1 - 11

ER -