Abstract

Megakaryopoiesis is the process by which hematopoietic stem cells in the bone marrow differentiate into mature megakaryocytes. The expression of megakaryocytic genes during megakaryopoiesis is controlled by specific transcription factors. Fli-1 and GATA-1 transcription factors are required for development of megakaryocytes and promoter analysis has defined in vitro functional binding sites for these factors in several megakaryocytic genes, including GPIIb, GPIX, and C-MPL. Herein, we utilize chromatin immunoprecipitation to examine the presence of Ets-1, Fli-1, and GATA-1 on these promoters in vivo. Fli-1 and Ets-1 occupy the promoters of GPIIb, GPIX, and C-MPL genes in both Meg-01 and CMK11-5 cells. Whereas GPIIb is expressed in both Meg-01 and CMK11-5 cells, GPIX and C-MPL are only expressed in the more differentiated CMK11-5 cells. Thus, in vivo occupancy by an Ets factor is not sufficient to promote transcription of some megakaryocytic genes. GATA-1 and Fli-1 are both expressed in CMK11-5 cells and co-occupy the GPIX and C-MPL promoters. Transcription of all three megakaryocytic genes is correlated with the presence of acetylated histone H3 and phosphorylated RNA polymerase II on their promoters. We also show that exogenous expression of GATA-1 in Meg-01 cells leads to the expression of endogenous c-mpl and gpIX mRNA. Whereas GPIIb, GPIX, and C-MPL are direct target genes for Fli-1, both Fli-1 and GATA-1 are required for formation of an active transcriptional complex on the C-MPL and GPIX promoters in vivo. In contrast, GPIIb expression appears to be independent of GATA-1 in Meg-01 cells.

Highlights

  • Ets family members each contain a conserved winged helixloop-helix DNA binding (ETS) domain that allows recognition of purine-rich DNA sequences with a core GGA(A/T) consensus, designated EBS1 (Ets binding sequence) [1,2,3]

  • We show that exogenous expression of GATA-1 in Meg-01 cells leads to the expression of endogenous c-mpl and gpIX mRNA

  • To better understand how Ets and GATA-1 proteins regulate the transcription of megakaryocytic target genes, we examined the in vivo binding of Fli-1, Ets-1, and GATA-1 proteins to the endogenous GPIIb, GPIX, and C-MPL promoters

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Summary

Primer sequences

5Ј-TAGCACAGATACAGAGGCTGAGTT-3Ј 5Ј-CATCCTCCCTTCAGGAAGCTG-3Ј 5Ј-GTGCTTAACACACGGCAGC-3Ј 5Ј-CCATCCAGACCACACTGG-3Ј 5Ј-TGCTGTTGCTCCTGGTCTACA-3Ј 5Ј-CAGCCATGCTGTCGTATGCTC-3Ј 5Ј-GAACCAATAGGACATGG-3Ј 5Ј-CATCTTCCTTCTTCCAC-3Ј 5Ј-GCACTGACTGCACTGCTG-3Ј 5Ј-GCTGTGGTGCTTTGTGAC-3Ј 5Ј-GCACTCCTCCTCTTCCGCTTAC-3Ј 5Ј-TGCTACAGCCCTAGAGACTACC-3Ј 5Ј-GAGATGTGGTTCTGTGCC-3Ј 5Ј-TGCTGGGTAATACGGAGG-3Ј 5Ј-ACTTGGTAGAGGCTCTGCTT-3Ј 5Ј-CTGGCTGAGCACACCATGGT-3Ј 5Ј-GCGAGCGTCTTCGATGC-3Ј 5Ј-CTCAGCTCCTTACATGGGC-3Ј 5Ј-CCAGCCAGGGGAACTTC-3Ј 5Ј-GCTTTGGTCCATCTTGCC-3Ј 5Ј-AGGCATGATCTGCTGGTGGGCGCT-3Ј 5Ј-ATTGTAGCCATCCCGGTCGAGGT-3Ј 5Ј-AGCTGCAGACCCTCGATGTGACGC-3Ј 5Ј-GACCAGCGCCACGTCCCACAAG-3Ј 5Ј-TAAGGTGGCTGAATCCTCTGCATC-3Ј 5Ј-CCGTCTTCAAGGTGTCCAAGAACGT-3Ј 5Ј-GGTTTACCGATGGACGGGACTATTAAG-3Ј 5Ј-CCTGATCAAAGAAGCTTCTAGTAGTAG-3Ј. Over 200 Ets target genes have been identified by the presence of functional EBS [5], based upon transient transfection studies. Few of these have been characterized on chromatin templates in vivo. To better understand how Ets and GATA-1 proteins regulate the transcription of megakaryocytic target genes, we examined the in vivo binding of Fli-1, Ets-1, and GATA-1 proteins to the endogenous GPIIb, GPIX, and C-MPL promoters. The differential expression of these genes in megakaryocytic cell lines allowed us to correlate Ets factor occupancy, histone acetylation status, and/or presence of phosphorylated RNA polymerase II with transcription from these promoters. We demonstrate for the first time that simultaneous in vivo promoter occupancy by these factors is directly correlated with the transcriptional status of specific megakaryocytic genes

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