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J Biol Chem, Vol. 273, Issue 14, 8278-8286, April 3, 1998
From the CRC Department of Gene Regulation, Paterson Institute for
Cancer Research, Christie Hospital NHS Trust, Wilmslow Road,
Manchester M20 9BX, United Kingdom
Accumulating evidence implicates functions of the
Id family of helix-loop-helix proteins in the regulation of cell growth and differentiation in metazoa. Within the mammalian hematopoietic organ, expression of the Id3 gene is restricted to the lymphoid cell
compartment. We show here that in non-lymphoid hematopoietic cells,
repression of transcription is correlated with hypermethylation of
sequences in the vicinity of the upstream regulatory region of the Id3
gene, suggestive of a strict developmental control of expression of
this gene in lymphoid versus non-lymphoid hematopoietic cells. Enforced ectopic expression of Id3 in K562 erythroid progenitor cells promotes erythroid differentiation and is correlated with a
quantitative/qualitative shift in the profile of interacting TAL1 and E
protein heterodimers that bind to a consensus E box sequence in
in vitro band shift assays, consistent with selective targeting of E2A E protein(s) by Id3 and suggesting a possible mechanism involving TAL1-mediated differentiation. By using a Gal
4-VP16 two-hybrid competition assay and an E box-dependent reporter assay, we demonstrate directly that the E2A protein E47 preferentially associates with Id3 in vivo. These
observations provide a paradigm for understanding how overlapping but
distinct specificities of individual Id proteins may constitute a
developmentally regulated program underlying cell determination in
diverse lineages.
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