Regulation of mammary stem/progenitor cells by p53 and parity

Tao, Luwei

01 January 2011

Breast cancer is the most common tumor among women with inherited mutations in the p53 gene (Li-Fraumeni syndrome). The tumors represent the basal-like subtype which has been suggested to originate from mammary stem/progenitor cells. In mouse mammary epithelium, mammosphere-forming potential was increased with decreased dosage of the gene encoding the p53 tumor suppressor protein (Trp53). Limiting dilution transplantation also showed a 3.3-fold increase in the frequency of long-term regenerative mammary stem cells in Trp53-/- mice. The repression of mammospheres by p53 was apparent despite the absence of apoptotic responses to radiation indicating a dissociation of these two activities of p53. The effects of p53 on progenitor cells were also observed in TM40A cells using both mammosphere-forming assays and the DsRed-let7c-sensor. The frequency of long-term label-retaining epithelial cells (LRECs) was decreased in Trp53-/- mammary glands indicating that asymmetric segregation of DNA is diminished and contributes to the expansion of the mammary stem cells. Treatment with an inhibitor of γ-secretase (DAPT) reduced the number of Trp53-/- mammospheres to the level found in Trp53+/+ cells. These results demonstrate that basal levels of p53 restrict mammary stem/progenitor cells. Notch is a target of γ-secretase suggesting that the Notch pathway is a therapeutic target to prevent expansion of this vulnerable pool of cells. The expansion of p53-deficient mammary stem/progenitor cells can also be reversed after the expression of C-terminal p53, suggesting that the C-terminal domains of p53 may be responsible for the regulation of mammary stem/progenitor cells self-renewal. In parous mammary gland, increased p53 responsiveness sensitized mammary stem/progenitor cells to ionizing radiation without affecting the self-renewal of these cells, which may be responsible for the parity-induced protection against breast cancer.

Box C/D small nucleolar RNAs: Biogenesis, structure and utilization for in vivo ribozyme studies

Samarsky, Dmitry A

01 January 1998

Eukaryotic cells contain scores of small nucleolar RNAs (snoRNAs), which are required for maturation of pre-rRNA. Two large snoRNA families exist defined by vital box C/D and box H/ACA motifs. The goal of the present study was to gain new insights into the structure and biogenesis of the box C/D snoRNAs; the knowledge developed from this effort was then recruited for practical applications. The investigation was conducted with the phylogenetically conserved U14 and U3 box C/D snoRNAs, from the yeast Saccharomyces cerevisiae. The specific aims included: (1) identification of cis-elements sufficient for biogenesis of the U14 snoRNA; (2) development of a functional map for the U3 snoRNA, and; (3) development of a U3-based model ribozyme system for in vivo studies. Conclusions derived from the U14 biogenesis studies are: (1) production of U14 involves ordered folding of the precursor RNA, and this step is required for formation of the vital box C/D structure motif, and; (2) the active box C/D motif, which is now predicted to consist solely of the box C and D elements, is necessary and sufficient for both accumulation and targeting RNA to the nucleolus. A general model for box C/D snoRNA biogenesis is proposed. Functional mapping of U3 revealed that: (1) boxes C$\sp\prime$ and D and flanking helices are critical for U3 accumulation; (2) boxes B and C are not essential for U3 production, but are important for function, due most likely to binding of a trans-acting factor(s); (3) the 5$\sp\prime$ portion of U3 is required for function, but not stability, and; (4) the non-conserved hairpins, which account for 50% of the molecule, are not required for accumulation or function. Based on the knowledge obtained with U14 and U3, a model ribozyme system featuring chimeric U3:ribozyme RNAs, or "snorbozymes", was developed and tested in vivo. Remarkably, the cleavage efficiency by a hammerhead ribozyme, both in cis- and in trans-configurations, appears quantitative! Other advantages of the system are: (1) a final product is stable, and; (2) authentic in vivo cleavage can be easily distinguished from artifactual cleavages. Snorbozymes are predicted to be useful for targeting natural transcripts in any eukaryotes, for fundamental research or practical applications.

Functional characterization of stress associated proteins (SAPS) from arabidopsis

Dixit, Anirudha R

01 January 2011

Abiotic stresses such as drought, salt, cold, heat and exposure to toxic metals adversely affect growth and productivity of crop plants and are serious threats to agriculture. Members of Stress Associated Protein (SAP) family in rice have been shown to provide tolerance to multiple abiotic stresses. There are 18 and 14 reported members of SAP family in rice and Arabidopsis, respectively. These SAPs contain A20, AN1, or both A20/AN1 zinc finger domains at the N- or C-terminus. Some members of SAP family proteins also contain extra Cys2-His2 RING motifs on the C-terminus. We describe here the functional characterization of two novel SAP genes, AtSAP10 and AtSAP11, from Arabidopsis thaliana ecotype Columbia. AtSAP10 gene contains an A20 and AN1 zinc-finger domain at the N- and C-terminal, respectively. Arabidopsis SAP10 showed differential regulation by various abiotic stresses such as heavy metals and metalloids (Ni, Cd, Mn, Zn, and As), high and low temperatures, cold, and ABA. Overexpression of AtSAP10 in Arabidopsis conferred strong tolerance to heavy metals such as Ni, Mn, and Zn and to high temperature stress. AtSAP10 transgenic plants under these stress conditions grew green and healthy, attained several-fold more biomass, and had longer roots as compared to wild type plants. Further, while these transgenic plants accumulated significantly greater amounts of Ni and Mn in both shoots and root tissues, there was no significant difference in the accumulation of Zn. AtSAP10 promoter-GUS fusion studies revealed a root and floral organ-specific expression of AtSAP10. Overexpression of AtSAP10-GFP fusion protein showed the localization in both nucleus and cytoplasm. A second gene from AtSAP family, AtSAP11, contains two AN1 zinc finger domains at N-terminal and two C2H2 zinc finger domains at C-terminus. Arabidopsis SAP11 showed differential regulation by various abiotic stresses such as heavy metals and metalloids (As, Cd and Zn), high and low temperatures, cold, and salt. Overexpression of AtSAP11 in Arabidopsis conferred moderate tolerance to heavy metals As and Zn and slightly enhanced tolerance to drought stress. AtSAP11 overexpression plants did not accumulate significantly higher amounts arsenic in shoots or roots. AtSAP11 promoter-GUS fusion studies revealed a floral organ-specific and fruit specific expression of AtSAP11. AtSAP11-GFP fusion showed an ER like localization of the fusion protein. Thus these results showed that AtSAP10 and AtSAP11 are potentially useful candidate genes for engineering tolerance to heavy metals and to abiotic stress in cultivated plants.

Molecular biology|Plant biology|Genetics

Bacterial ribosomes and temperature sensitivity

January 1973

acase@tulane.edu

Tulane University

Biology, Genetics

Ph.D

Genetic epidemiology of tuberculosis

Ahmadipour, Nooshin

January 2002

No description available.

Biology, Genetics.

Health Sciences, Pathology.

The role of the androgen receptor CAG repeat polymorphism in the AR-T877A prostate cancer somatic mutant /

Southwell, Jason M.

January 2006

No description available.

Health Sciences, Oncology.

Biology, Genetics.

Antisense inhibition of methylenetetrahydrofolate reductase as a cancer treatment and a pharmacogenetic study to examine the effects of a common polymorphism

Sekhon, Jaspreet.

January 2001

No description available.

Health Sciences, Oncology.

Biology, Genetics.

Three transgenic hemoglobin SAD (S-Antilles, -Punjab), partial-"knockout" murine models of human sickle cell disease : the generation and phenotypic analysis of SAD mice with (1) heterozygous-null deletion of the murine a-globin genes, (2) homozygous-null deletion of the murine a-globin genes, and (3) heterozygous null deletions of the murine a- and b-globin genes

Wright, Adrian C.

January 2000

No description available.

Biology, Genetics.

Health Sciences, Pathology.

Cytokine gene expression in human immunodeficiency virus infected myeloid cells

D'Addario, Mario G., Jr.

January 1992

No description available.

Biology, Genetics.

Health Sciences, Immunology.

Genetics of host innate immune factors in Tuberculosis susceptibility

Malik, Suneil

January 2005

No description available.

Health Sciences, Pathology.

Biology, Genetics.