Abstract

Mechanisms controlling gene expression in eukaryotic cells are complex, encompassing transcriptional and post-transcriptional components. Due to inherent difficulties in their study, post-transcriptional mechanims have received relatively less attention; in particular, RNA transport has been studied as the appearance of rapidly-labeled RNA in the supernate after incubation of nuclei in vitro. Such assays would be more firmly accepted if the transported RNA was better characterized. It is the intent of this proposal to test the fidelity of carefully selected in vitro system by examining the behavior of specific sequences. Using perturbations which result in great differences in mRNA formation and abundance in vivo, metabolism of an acute phase reactant sequence (alpha1-acid glycoprotein), a hormonally-responsible globulin sequence (alpha2Mu-globulin), and marker sequences for mature (albumin) and primitive (Alpha-fetoprotein) liver cells will be examined with an in vitro transport system. An additional model will employ an analbuminemic rat strain, which transcribes albumin sequences into nuclear RNA but restricts them to the nucleus. Transported and nucleus-restricted RNA will be isolated and in vitro translation products will be examined. RNA will be separated by size electrophoretically, """"""""Northern blotted"""""""" and hybridized with specific P32-cDNA probes, and autoradiographs will be developed. Mixing experiments will document and quantitate cytoplasmic contamination of nuclear and transported preparation. These experiments will determine whether in vitro transport assays can support processing/transport of correctly-sized functional mRNA, with modulation paralleling in vivo circumstances. Providing specificity can be established (as preliminary results indicate), use of in vitro transport assays should contribute valuably to understanding controls of gene expression, especially the altered post-transcriptional RNA transport associated with carcinogenesis. If specificity cannot be established, the considerable effort and funding devoted to their use in studies of """"""""in vivo specificity"""""""" should be curtailed.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
1R01CA040145-01
Application #
3179691
Study Section
Chemical Pathology Study Section (CPA)
Project Start
1985-07-01
Project End
1988-06-30
Budget Start
1985-07-01
Budget End
1986-06-30
Support Year
1
Fiscal Year
1985
Total Cost
Indirect Cost

  Institution

Name
University of California San Francisco
Department
Type
Schools of Medicine
DUNS #
073133571
City
San Francisco
State
CA
Country
United States
Zip Code
94143

  Publications

Wang, Ning; Eckert, Kristin A; Zomorrodi, Ali R et al. (2012) Down-regulation of HtrA1 activates the epithelial-mesenchymal transition and ATM DNA damage response pathways. PLoS One 7:e39446
Broutian, Tatevik R; Brendle, Sarah A; Christensen, Neil D (2010) Differential binding patterns to host cells associated with particles of several human alphapapillomavirus types. J Gen Virol 91:531-40
Gestl, Shelley A; Leonard, Travis L; Biddle, Jessica L et al. (2007) Dormant Wnt-initiated mammary cancer can participate in reconstituting functional mammary glands. Mol Cell Biol 27:195-207
Culp, Timothy D; Cladel, Nancy M; Balogh, Karla K et al. (2006) Papillomavirus particles assembled in 293TT cells are infectious in vivo. J Virol 80:11381-4
Culp, Timothy D; Budgeon, Lynn R; Marinkovich, M Peter et al. (2006) Keratinocyte-secreted laminin 5 can function as a transient receptor for human papillomaviruses by binding virions and transferring them to adjacent cells. J Virol 80:8940-50
Culp, Timothy D; Budgeon, Lynn R; Christensen, Neil D (2006) Human papillomaviruses bind a basal extracellular matrix component secreted by keratinocytes which is distinct from a membrane-associated receptor. Virology 347:147-59
Crisman, Jacqueline M; Zhang, Binzhi; Norman, Lourdes P et al. (2004) Deletion of the mouse meprin beta metalloprotease gene diminishes the ability of leukocytes to disseminate through extracellular matrix. J Immunol 172:4510-9
Drubin, David A; Clawson, Gary A (2004) Spontaneous transformation of an immortalized hepatocyte cell line: potential role of a nuclear protease. Cancer Lett 213:39-48
MacNeill, Colin; Umstead, Todd M; Phelps, David S et al. (2004) Surfactant protein A, an innate immune factor, is expressed in the vaginal mucosa and is present in vaginal lavage fluid. Immunology 111:91-9
Pan, Wei-Hua; Xin, Ping; Bui, Vuong et al. (2003) Rapid identification of efficient target cleavage sites using a hammerhead ribozyme library in an iterative manner. Mol Ther 7:129-39

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