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J Biol Chem, Vol. 273, Issue 45, 29626-29634, November 6, 1998
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From the Although purinergic compounds are widely involved
in the intra- and intercellular communication of the nervous system,
little is known of their involvement in the growth and regeneration of neuronal connections. In dissociated cultures, the addition of adenosine or guanosine in the low micromolar range induced goldfish retinal ganglion cells to extend lengthy neurites and express the
growth-associated protein GAP-43. These effects were highly specific
and did not reflect conversion of the nucleosides to their nucleotide
derivatives; pyrimidines, purine nucleotides, and membrane-permeable,
nonhydrolyzable cyclic nucleotide analogs were all inactive. The
activity of adenosine required its conversion to inosine, because
inhibitors of adenosine deaminase rendered adenosine inactive.
Exogenously applied inosine and guanosine act directly upon an
intracellular target, which may coincide with a kinase described in
PC12 cells. In support of this, the effects of the purine nucleosides
were blocked with purine transport inhibitors and were inhibited
competitively with the purine analog 6-thioguanine (6-TG). In PC12
cells, others have shown that 6-TG blocks nerve growth factor-induced
neurite outgrowth and selectively inhibits the activity of protein
kinase N, a partially characterized, nerve growth factor-inducible
serine-threonine kinase. In both goldfish and rat retinal ganglion
cells, 6-TG completely blocked outgrowth induced by other growth
factors, and this inhibition was reversed with inosine. These results
suggest that axon outgrowth in central nervous system neurons
critically involves an intracellular purine-sensitive mechanism.
Laboratories for Neuroscience Research in
Neurosurgery,
Department of Biology,
University of Konstanz, Konstanz, D-78434, Germany
Copyright © 1998 by The American Society for Biochemistry and Molecular Biology, Inc.
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