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Mol. Cell. Biol., Feb 1995, 892-903, Vol 15, No. 2
S Plaza, C Dozier, MC Langlois and S Saule
Using nuclear run-on assays, we showed that the tissue-specific expression
of quail Pax-6 (Pax-QNR) P0-initiated mRNAs is due in part to regulation of
the gene at the transcriptional level. Regulatory sequences governing
neuroretina-specific expression of the P0-initiated mRNAs were
investigated. By using reporter-based expression assays, we characterized a
region within the Pax-QNR gene, located 7.5 kbp downstream from the P0
promoter, that functions as an enhancer in neuroretina cells but not in
nonexpressing P0-initiated mRNA cells (quail embryo cells and quail retinal
pigment epithelial cells). This enhancer element functioned in a position-
and orientation-independent manner both on the Pax-QNR P0 promoter and the
heterologous thymidine kinase promoter. Moreover, this enhancer element
exhibited a developmental stage-specific activity during embryonic
neuroretina development: in contrast to activity at day E7, the enhancer
activity was very weak at day E5. This paralleled the level of expression
of P0- initiated mRNAs observed at the same stages. Using footprinting, gel
retardation, and Southwestern (DNA-protein) analysis, we demonstrated the
existence of four neuroretina-specific nuclear protein-binding sites,
involving multiple unknown factors. In addition we showed that the quail
enhancer element is structurally and functionally conserved in mice. All of
these results strongly suggest that this enhancer element may contribute to
the neuroretina-specific transcriptional regulation of the Pax-6 gene in
vivo.
Copyright © 1995, American Society for Microbiology
Identification and characterization of a neuroretina-specific enhancer element in the quail Pax-6 (Pax-QNR) gene
Laboratoire de differenciation cellulaire et moleculaire, Centre National de la Recherche Scientifique EP 56. Institut Pasteur, Lille, France.
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