Abstract

The Laboratory of Cardiovascular Science is committed to identifying those gene products that are differentially expressed in embryonic development through exploitation of the cardiac developmental model of embryonic stem and embryonic carcinoma cell differentiation. Serial analysis of gene expression (SAGE) yields a quantitative, representative and comprehensive differential gene expression profile. Using several time points in the precise developmental profile of embryonic stem and carcinoma cell differentiation to cardiomyocytes, SAGE analysis has been used to generate a quantitative transcript assessment that has proven to be much more rapid and economical than other techniques. We used an RT-PCR based technique to determine the time points where a number of mesodermal and cardiac-restricted gene products are expressed in in vitro differentiated EC derived cardiomyocytes. Results show that the earliest contractions occur on Day 5.5 of differentiation (3+2.5 or 4+1.5). Some contractile protein genes (beta MHC) are expressed before the third day of differentiation, but we show that a clear induction of expression of alpha MHC and MLC2V starts relatively later (5+0.5 and 3+1 for alpha MHC and MLC2V respectively). GATA-4, a transcription factor involved in the regulation of cardiac contractile protein gene expression is highly present in the earliest stages of differentiation, and form 3+1.5 days of differentiation, its expression is reduced to the level of adult heart tissue. This indicates that this time period corresponds to an early stage of cardiac differentiation. We have now used the protocols of SAGE to analyze expressed sequence profiles during these time periods. A total of 150,354 tags have been sequenced from three P19 EC cell-based libraries (undifferentiated P19 cells, differentiation Days 3+0.5 and 3+3.0). Ten percent of the 43,432 unique tags matched sequences in the NR GenBank database, while more than 30% of the unique tags did not match any known mouse sequence. Temporally-restricted induction or repression of transcripts at each differentiation stage examined was a common feature of the developmental profiles, suggesting that differentiation-specific processes are necessary for pre- and early cardiac development. Analysis of the normalized tag frequency with differentiation revealed significant changes (p<0.01) in expression of 357 gene products, including the known cardiac differentiation factor Thing1 (HAND1). Temporal analysis of the 97 tags that had a greater than 10-fold change in expression with differentiation revealed four patterns of expression: monotonic-ascending, monotonic-descending, bell-shaped and U-shaped. Transcription factors implicated in cardiac development (e.g., GATA-4, TEF-1, TGF-beta, Hox-7, HAND1) mostly fell in the bell-shaped group, indicating that this profile may be relevant for the identification of cardiac regulatory genes. Many of the gene products showing significant changes in gene expression have now been evaluated by quantitative PCR. Several of the products have shown a cardiac predominance in either fetal or adult heart. These genes are now being evaluated for any functional significance in the induction or differentiation of pluripotent cells to cardiac myocytes. The novel gene products identified in this study provide a framework for the analysis of pre- and early cardiac developmental processes in human and mouse.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute on Aging (NIA)
Type
Intramural Research (Z01)
Project #
1Z01AG000283-04
Application #
6508396
Study Section
(LCS)
Project Start
Project End
Budget Start
Budget End
Support Year
4
Fiscal Year
2001
Total Cost
Indirect Cost

  Institution

Name
Aging
Department
Type
DUNS #
City
State
Country
United States
Zip Code

  Publications

Nikolova, Teodora; Wu, Minyao; Brumbarov, Krassimir et al. (2007) WNT-conditioned media differentially affect the proliferation and differentiation of cord blood-derived CD133+ cells in vitro. Differentiation 75:100-11
Li, Jinliang; Wei, Hong; Chesley, Alan et al. (2007) The pro-angiogenic cytokine pleiotrophin potentiates cardiomyocyte apoptosis through inhibition of endogenous AKT/PKB activity. J Biol Chem 282:34984-93
Wiese, Cornelia; Rolletschek, Alexandra; Kania, Gabriela et al. (2006) Signals from embryonic fibroblasts induce adult intestinal epithelial cells to form nestin-positive cells with proliferation and multilineage differentiation capacity in vitro. Stem Cells 24:2085-97
Boheler, Kenneth R; Tarasov, Kirill V (2006) SAGE analysis to identify embryonic stem cell-predominant transcripts. Methods Mol Biol 329:195-221
Volkova, Maria; Garg, Rahul; Dick, Salihah et al. (2005) Aging-associated changes in cardiac gene expression. Cardiovasc Res 66:194-204
Boheler, Kenneth R; Crider, David G; Tarasova, Yelena et al. (2005) Cardiomyocytes derived from embryonic stem cells. Methods Mol Med 108:417-35
Anisimov, S V; Boheler, K R (2003) Aging-associated changes in cardiac gene expression: large scale transcriptome analysis. Adv Gerontol 11:67-75
Brady, Marc; Koban, Maren U; Dellow, Kimberley A et al. (2003) Sp1 and Sp3 transcription factors are required for trans-activation of the human SERCA2 promoter in cardiomyocytes. Cardiovasc Res 60:347-54
Fijnvandraat, Arnoud C; van Ginneken, Antoni C G; Schumacher, Cees A et al. (2003) Cardiomyocytes purified from differentiated embryonic stem cells exhibit characteristics of early chamber myocardium. J Mol Cell Cardiol 35:1461-72
Anisimov, Sergey V; Tarasov, Kirill V; Riordon, Daniel et al. (2002) SAGE identification of differentiation responsive genes in P19 embryonic cells induced to form cardiomyocytes in vitro. Mech Dev 117:25-74

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