Transcriptional regulation of the pro-apoptotic gene Bnip3 by P65 NF-κB, Histone Deacetylase 1, and E2F-1 in postnatal ventricular myocytes

Shaw, James Alexander

20 August 2009

Apoptotic cell death of cardiac myocytes plays an important pathological role after a myocardial infarction and during heart failure. Apoptotic myocytes are not regenerated because of the restricted ability of terminally differentiated cardiac myocytes to undergo cell division. Because ventricular function is directly related to the number of active muscle cells, the inappropriate loss or premature death of cardiac myocytes results in reduced cardiac performance. Bnip3 was previously identified by Dr. Lorrie Kirshenbaum’s laboratory as a critical mediator of hypoxia-induced apoptosis in the heart. Importantly, his lab established that the cytoprotective actions of NF-κB during hypoxia included the transcriptional repression of Bnip3. However, the mechanism by which NF-κB acted as a transcriptional repressor was undefined. The present work strongly supports the hypothesis that NF-κB-mediated inhibition of Bnip3 transcription is dependent on the recruitment of the corepressor protein HDAC1. Immunoprecipitation experiments revealed that HDAC1 and p65 NF-κB formed protein-protein interactions. ChIP assays demonstrated that HDAC1 and p65 NF-κB associated with the Bnip3 promoter. HDAC1-mediated repression of Bnip3 was lost in cells deficient for p65 NF-κB, and restored upon repletion of p65. A second avenue of investigation described in this work demonstrated that the cell cycle factor E2F-1 directly activated Bnip3 transcription. Earlier work by Dr. Kirshenbaum found that adenovirus-mediated overexpression of E2F-1 in ventricular myocytes induced apoptosis. Herein, it is shown that E2F-1-mediated cell death is largely Bnip3-dependent because functional loss of Bnip3 inhibited E2F-1-induced cell death. Concerning hypoxia, Bnip3 expression is dependent upon the loss of p65/HDAC1-mediated repression, and on the presence of transcriptionally active E2F-1. During hypoxia, overexpression of p65, HDAC1, or Rb, an endogenous inhibitor of E2F-1-dependent transcription, attenuated hypoxia-induced Bnip3 transcription. Based on these findings, future therapies may be designed to repress Bnip3 gene expression after a myocardial infarction, thereby averting cardiac cell death and preserving cardiac function post-infarction.

Bnip3

E2F-1

Apoptosis

Hypoxia

Mitochondria

Myocyte

NF-κB

Cell Culture

HDAC1

Regulation of Neural Precursor Cell Fate by the E2f3a and E2f3b Transcription Factors

Julian, Lisa

29 August 2013

The classical cell cycle regulatory pathway is well appreciated as a key regulator of cell fate determination during neurogenesis; however, the extent of pRB/E2F function in neural stem and progenitor cells is not fully understood, and insight into the mechanisms underlying its connection with cell fate regulation are lacking. The E2F3 transcription factor has emerged as an important regulator of neural precursor cell (NPC) proliferation in the embryonic and adult forebrain, and we demonstrate here that it also influences the self-renewal potential of NPCs. Using knockout mouse models of individual E2F3 isoforms, we demonstrate the surprising result that the classical transcriptional activator E2F3a represses NPC self-renewal and promotes neuronal differentiation, while E2F3b promotes the expansion of the NPC pool and inhibits differentiation. We attribute these opposing activities to a unique mechanism of transcriptional regulation at the Sox2 locus, a key regulator of stem cell pluripotency, whereby E2F3a recruits transcriptional repressors to this site, and E2F3b promotes Sox2 activation. Importantly, E2F3a-mediated Sox2 regulation is necessary for cognitive function in the adult. Additionally, through the determination of genome-wide promoter binding sites for E2f3 isoforms as well as E2F4, another key regulator of NPC self-renewal, we determined that E2Fs are poised to regulate an extensive set of target genes with key roles in regulating diverse cell fate choices in NPCs, including self-renewal, cell death, progenitor expansion, maintenance of the precursor state, and differentiation. Together, these results reveal a diversity of function for E2Fs in the control of neural precursor cell fate, and identify E2F3 isoforms as important regulators of the pluripotency and stem cell maintenance gene Sox2.

Neural stem cell

E2f

Transcription

Sox2

Neurogenesis

Gene regulation

Brain development

Macrophage mediated prevention of islet loss and diabetes during pancreatitis /

Tessem, Jeffery Sivert.

January 2007

Thesis (Ph.D. in Molecular Biology) -- University of Colorado Denver, 2007. / Typescript. Includes bibliographical references (leaves 162-196). Free to UCD affiliates. Online version available via ProQuest Digital Dissertations;

The role of impaired cellular fitness in leukemia promotion /

Bilousova, Ganna.

January 2007

Thesis (Ph.D. in Biochemistry) -- University of Colorado Denver, 2007. / Typescript. Includes bibliographical references (leaves 137-161). Free to UCD affiliates. Online version available via ProQuest Digital Dissertations;

Regulation of Neural Precursor Cell Fate by the E2f3a and E2f3b Transcription Factors

Julian, Lisa

January 2013

The classical cell cycle regulatory pathway is well appreciated as a key regulator of cell fate determination during neurogenesis; however, the extent of pRB/E2F function in neural stem and progenitor cells is not fully understood, and insight into the mechanisms underlying its connection with cell fate regulation are lacking. The E2F3 transcription factor has emerged as an important regulator of neural precursor cell (NPC) proliferation in the embryonic and adult forebrain, and we demonstrate here that it also influences the self-renewal potential of NPCs. Using knockout mouse models of individual E2F3 isoforms, we demonstrate the surprising result that the classical transcriptional activator E2F3a represses NPC self-renewal and promotes neuronal differentiation, while E2F3b promotes the expansion of the NPC pool and inhibits differentiation. We attribute these opposing activities to a unique mechanism of transcriptional regulation at the Sox2 locus, a key regulator of stem cell pluripotency, whereby E2F3a recruits transcriptional repressors to this site, and E2F3b promotes Sox2 activation. Importantly, E2F3a-mediated Sox2 regulation is necessary for cognitive function in the adult. Additionally, through the determination of genome-wide promoter binding sites for E2f3 isoforms as well as E2F4, another key regulator of NPC self-renewal, we determined that E2Fs are poised to regulate an extensive set of target genes with key roles in regulating diverse cell fate choices in NPCs, including self-renewal, cell death, progenitor expansion, maintenance of the precursor state, and differentiation. Together, these results reveal a diversity of function for E2Fs in the control of neural precursor cell fate, and identify E2F3 isoforms as important regulators of the pluripotency and stem cell maintenance gene Sox2.

Neural stem cell

E2f

Transcription

Sox2

Neurogenesis

Gene regulation

Brain development

Modulation of Ferroptosis by the Classical p53/p21/CDK/RB/E2F Pathway

Kuganesan, Nishanth

15 June 2023

No description available.

Biology

Cellular Biology

Molecular Biology

The Retinoblastoma Tumor Suppressor Modifies the Therapeutic Response of Breast Cancer

Bosco, Emily E.

16 May 2006

No description available.

Retinoblastoma Tumor Suppressor

Breast Cancer

E2F

Tamoxifen

anti-estrogen resistance

DNA damage

cell cycle checkpoint

Role of the RB-E2F pathway in embryonic development: implications for paradigms of cell cycle control

Wenzel, Pamela L.

10 July 2007

No description available.

Rb

E2F

Transcription factors

Development

Placenta

Trophoblast

Stem cells

Lens

Apoptosis

Differentiation

Proliferation

Cell cycle

Biological function of E2F7 and E2F8 is essential for embryo development

Li, Jing

02 September 2009

No description available.

Genetics

Molecular Biology

E2F

embryo development

apoptosis

cell cycle

transcriptional regulation

Conception de microARNs pour attenuer l'expression de genes

Caron, Maxime

09 1900

Les microARNs appartiennent à la famille des petits ARNs non-codants et agissent comme inhibiteurs des ARN messagers et/ou de leurs produits protéiques. Les mi- croARNs sont différents des petits ARNs interférants (siARN) car ils atténuent l’ex- pression au lieu de l’éliminer. Dans les dernières années, de nombreux microARNs et leurs cibles ont été découverts chez les mammifères et les plantes. La bioinforma- tique joue un rôle important dans ce domaine, et des programmes informatiques de découvertes de cibles ont été mis à la disposition de la communauté scientifique. Les microARNs peuvent réguler chacun des centaines de gènes, et les profils d’expression de ces derniers peuvent servir comme classificateurs de certains cancers. La modélisation des microARNs artificiels est donc justifiable, où l’un pourrait cibler des oncogènes surexprimés et promouvoir une prolifération de cellules en santé. Un outil pour créer des microARNs artificiels, nommé MultiTar V1.0, a été créé et est disponible comme application web. L’outil se base sur des propriétés structurelles et biochimiques des microARNs et utilise la recherche tabou, une métaheuristique. Il est démontré que des microARNs conçus in-silico peuvent avoir des effets lorsque testés in-vitro. Les sé- quences 3’UTR des gènes E2F1, E2F2 et E2F3 ont été soumises en entrée au programme MultiTar, et les microARNs prédits ont ensuite été testés avec des essais luciférases, des western blots et des courbes de croissance cellulaire. Au moins un microARN artificiel est capable de réguler les trois gènes par essais luciférases, et chacun des microARNs a pu réguler l’expression de E2F1 et E2F2 dans les western blots. Les courbes de crois- sance démontrent que chacun des microARNs interfère avec la croissance cellulaire. Ces résultats ouvrent de nouvelles portes vers des possibilités thérapeutiques. / MicroRNAs belong to the family of small non-coding RNAs and act as down regula- tors of messenger RNAs and/or their protein products. microRNAs differ from siRNAs by downregulating instead of shutting down. In recent years, numerous microRNAs and their targets have been found in mammals and plants. Bioinformatics plays a big role in this field, as software has emerged to find new microRNA targets. Each individual microRNA can regulate hundreds of genes, and it has been shown that microRNA expression profiles can classify human cancers. The need for artificially created mi- croRNAs is then justified, as one could target overexpressed oncogenes and promote healthy cell proliferation. MultiTar V1.0, a tool for creating artificial microRNAs, has been implemented and is available as a web application. The tool relies on structural and biological properties of microRNAs and uses a Tabusearch metaheuristic. A typical biological problem is presented and it is shown that an in-silico microRNA has in-vitro effects. The 3’UTR sequences of E2F1, E2F2 and E2F3 were given as input to the tool, and predicted microRNAs were then tested using luciferase essays, western blots and growth curves. At least one microRNA is able to regulate the three genes with luciferase essays and all of the created microRNAs were able to regulate the expres- sion of E2F1 and E2F2 with western blots. Growth curves were also studied in order to investigate overall biological effects, and reduction in growth was observed for all solutions. Results obtained with the predicted microRNAs and the target genes open a new door into therapeutic possibilities.

MicroARN

E2F

Recherche tabou

Régulation de l'expression

mir20

MicroRNA

Tabusearch

Downregulation