The protein kinase C (PKC) substrate GAP‐43 is already expressed in neural precursor cells, colocalizes with PKCη and binds calmodulin
- 1 February 1999
- journal article
- research article
- Published by Wiley in European Journal of Neuroscience
- Vol. 11 (2) , 503-516
- https://doi.org/10.1046/j.1460-9568.1999.00455.x
Abstract
Expression of the growth-associated protein of 43-kDa (GAP-43), which is described as a postmitotic, neuron-specific major protein kinase C (PKC) substrate, was investigated in the murine embryonic carcinoma cell line PCC7-Mz1 which develops into a brain-tissue-like pattern of neuronal, fibroblast-like and astroglial cells upon stimulation with all-trans retinoic acid (RA). GAP-43 expression was very low in stem cells, but increased on mRNA and protein level within the 12 h after differentiation was initiated. While the P1 promoter of the GAP-43 gene gave rise to a 1.6-kb mRNA and was already active at a very low level in PCC7-Mz1 stem cells, transcription of the P2 promoter, which resulted in a 1.4-kb mRNA, was completely blocked in stem cells but increased rapidly after RA treatment. Within the first 2 days of neural differentiation, GAP-43 was localized with the cytoplasmic membrane and the Golgi complex of proliferating neural precursor cells. Then, GAP-43 was translocated to the growth cones and neurites, and from day 6, when neurons began to acquire polarity, the protein was found in the axons. GAP-43 was never detected in the non-neuronal PCC7-Mz1 derivatives, i.e. in fibroblasts or glial cells. In the foetal rat brain (prenatal day F11), GAP-43 was expressed in the optic stalk, the lense plakode and in the postmitotic neurons of the marginal zone of the hindbrain. Moreover, in a layer between the ventricular and marginal zone of the hindbrain (F13) and forebrain (F15), GAP-43 was already expressed in mitotic neural precursor cells. In PCC7-Mz1 cultures, 2 days after addition of RA, GAP-43 became phosphorylated upon activation of PKC, and colocalized specifically with the novel PKC isoform η. Phosphorylation of GAP-43 caused a disruption of its complex with calmodulin. These data demonstrate that GAP-43 is already a functional PKC substrate in prolific neuronal precursor cells, and may participate in neuronal cell lineage determination.Keywords
This publication has 75 references indexed in Scilit:
- Cell fate specification in an in vitro model of neural developmentEuropean Journal of Cell Biology, 1998
- The RXR heterodimers and orphan receptorsPublished by Elsevier ,1995
- Structure and Regulation of the Gene Encoding the Neuron-specific Protein Kinase C Substrate Neurogranin (RC3 Protein)Published by Elsevier ,1995
- Bombesin, endothelin and platelet‐derived growth factor induce rapid translocation of the myristoylated alanine‐rich C‐kinase substrate in Swiss 3T3 cellsEuropean Journal of Biochemistry, 1994
- Retinoic acid induces cholinergic differentiation of cultured newborn rat sympathetic neuronsJournal of Neuroscience Research, 1993
- Transient expression of GAP-43 in nonneuronal cells of the embryonic chicken limbDevelopmental Biology, 1992
- Role of the growth-associated protein B-50/GAP-43 in neuronal plasticityMolecular Neurobiology, 1991
- Rapid changes in the distribution of GAP-43 correlate with the expression of neuronal polarity during normal development and under experimental conditions.The Journal of cell biology, 1990
- States of developmental commitment of a mouse embryonal carcinoma cell line differentiating along a neural pathway.The Journal of cell biology, 1989
- A membrane phosphoprotein associated with neural development, axonal regeneration, phospholipid metabolism, and synaptic plasticityTrends in Neurosciences, 1987