Amyloid precursor protein fragment and acetylcholinesterase increase with cell confluence and differentiation in a neuronal cell line

Bronfman F.C.; Inestrosa, N. C.; Fernandez, H. L.

Keywords: growth, neurons, differentiation, adhesion, mouse, amyloid, animals, protein, cell, peptide, mice, tumor, fragments, nerve, acetylcholinesterase, cholinesterase, beta-protein, inhibitors, article, precursor, neuroblastoma, butyrylcholinesterase, controlled, animal, study, priority, nonhuman, journal, Animalia, Cells,, Cultured, bucladesine

Abstract

This study addresses the developmental regulation of amyloid precursor protein (APP) fragments comprising the amyloid-? peptide (A?) and the amyloid-p promoting factor acetyicholinesterase (ACHE) in a mouse neuronal cell line (Neuro-2a). Results indicated that a 35-kDa amyloidogenic fragment of APP and the major molecular forms of AChE (G~1 and G~4) in Neuro-2a cells significantly increase with increasing levels of cell confluence. The foregoing molecules undergo further increases when neuroblastoma cells differentiate in the presence of dibutyryl cAMP. In contrast, a 17-kDa fragment of APP and butyrylcholinesterase were not affected by cell confluence or differentiation. These findings are the first to indicate that a selective A?-containing fragment of APP is subject to develop mental regulation. Moreover, our data show that the 35-kDa fragment and AChE forms respond in parallel to the same developmental stimuli, i.e., cell confluence and differentiation. This points to the existence of a functional relationship between both molecules, a notion that is consistent with the potential role that has been ascribed to AChE in both APP processing and the formation of amyloid deposits in Alzheimer's brains.

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Título de la Revista: EXPERIMENTAL CELL RESEARCH
Volumen: 229
Número: 1
Editorial: ELSEVIER INC
Fecha de publicación: 1996
Página de inicio: 93
Página final: 99
URL: http://www.scopus.com/inward/record.url?eid=2-s2.0-0030601933&partnerID=q2rCbXpz
DOI:

10.1006/excr.1996.0347

Notas: ISI