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(Received for publication, October 16,
1995; and in revised form, November 28, 1995) The synapsins are a family of neuron-specific phosphoproteins
that selectively bind to small synaptic vesicles in the presynaptic
nerve terminal. The human synapsin I gene was functionally analyzed to
identify control elements directing the neuron-specific expression of
synapsin I. By directly measuring the mRNA transcripts of a reporter
gene, we demonstrate that the proximal region of the synapsin I
promoter is sufficient for directing neuron-specific gene expression.
This proximal region is highly conserved between mouse and human.
Deletion of a putative binding site for the zinc finger protein,
neuron-restrictive silencer factor/RE-1 silencing transcription factor
(NRSF/REST), abolished neuron-specific expression of the reporter gene
almost entirely, allowing constitutively acting elements of the
promoter to direct expression in a non-tissue-specific manner. These
constitutive transcriptional elements are present as a bipartite
enhancer, consisting of the region upstream (nucleotides -422 to
-235) and downstream (nucleotides -199 to -143) of
the putative NRSF/REST-binding site. The latter contains a motif
identical to the cAMP response element. Both regions are not active or
are only weakly active in promoting transcription on their own and show
no tissue-specific preference. From these data we conclude that
neuron-specific expression of synapsin I is accomplished by a negative
regulatory mechanism via the NRSF/REST binding motif.
Volume 271,
Number 6,
Issue of February 9, 1996 pp. 3317-3323
©1996 by The American Society for Biochemistry and Molecular Biology, Inc.
MAJOR ROLE OF A NEGATIVE REGULATORY MECHANISM
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