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A scoring system for the follow up study of nuclear receptor coactivator complexes

We have systematically isolated a variety of coactivator complexes from HeLa S3 cells using proteomic approaches. In the present report, we have evaluated twelve coactivator complexes involved in nuclear receptor-dependent gene transcription that have been purified by using an immunoprecipitation me...

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Autores principales: Han, Sang Jun, Jung, Sung Yun, Malovannaya, Anna, Kim, Taeil, Lanz, Rainer B., Qin, Jun, O’Malley, Bert W.
Formato: Texto
Lenguaje:English
Publicado: The Nuclear Receptor Signaling Atlas 2006
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC1513068/
https://www.ncbi.nlm.nih.gov/pubmed/16862220
http://dx.doi.org/10.1621/nrs.04014
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author Han, Sang Jun
Jung, Sung Yun
Malovannaya, Anna
Kim, Taeil
Lanz, Rainer B.
Qin, Jun
O’Malley, Bert W.
author_facet Han, Sang Jun
Jung, Sung Yun
Malovannaya, Anna
Kim, Taeil
Lanz, Rainer B.
Qin, Jun
O’Malley, Bert W.
author_sort Han, Sang Jun
collection PubMed
description We have systematically isolated a variety of coactivator complexes from HeLa S3 cells using proteomic approaches. In the present report, we have evaluated twelve coactivator complexes involved in nuclear receptor-dependent gene transcription that have been purified by using an immunoprecipitation method. The twelve purified coactivator complexes are SRC-1, SRC-2, SRC-3, CBP, p300, CAPER, E6-AP, ASC-1, CoREST, CRSP3, CRSP2, and CDK7 containing complexes. We have identified 153 protein components associated with these coactivator complexes using mass spectrometry. In order to systematically characterize the functional roles for these components in nuclear receptor-dependent gene transcription and their investigative potential, we have developed a scoring system. This scoring system is comprised of biological and experimental parameters. The biological evaluation considers aspects such as intrinsic enzymatic activity of a protein component, cellular signaling processes in which protein components may be involved, associations with human disease, specific protein motifs, and the known biological roles of other interacting partners of the identified protein. In the experimental evaluation, we include parameters, such as the availability of research materials for the functional study of the identified protein component; such as full-length cDNA clones, antibodies, and commercially available knock-out embryonic stem (ES) cells. Each scoring parameter has been assigned an arbitrary number of points according to perceived relative importance. On the basis of this scoring system, we prioritized each of the protein components in terms of the likelihood of their importance for coactivator complex networking in nuclear receptor-dependent gene transcription.
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spelling pubmed-15130682006-07-20 A scoring system for the follow up study of nuclear receptor coactivator complexes Han, Sang Jun Jung, Sung Yun Malovannaya, Anna Kim, Taeil Lanz, Rainer B. Qin, Jun O’Malley, Bert W. Nucl Recept Signal Methods We have systematically isolated a variety of coactivator complexes from HeLa S3 cells using proteomic approaches. In the present report, we have evaluated twelve coactivator complexes involved in nuclear receptor-dependent gene transcription that have been purified by using an immunoprecipitation method. The twelve purified coactivator complexes are SRC-1, SRC-2, SRC-3, CBP, p300, CAPER, E6-AP, ASC-1, CoREST, CRSP3, CRSP2, and CDK7 containing complexes. We have identified 153 protein components associated with these coactivator complexes using mass spectrometry. In order to systematically characterize the functional roles for these components in nuclear receptor-dependent gene transcription and their investigative potential, we have developed a scoring system. This scoring system is comprised of biological and experimental parameters. The biological evaluation considers aspects such as intrinsic enzymatic activity of a protein component, cellular signaling processes in which protein components may be involved, associations with human disease, specific protein motifs, and the known biological roles of other interacting partners of the identified protein. In the experimental evaluation, we include parameters, such as the availability of research materials for the functional study of the identified protein component; such as full-length cDNA clones, antibodies, and commercially available knock-out embryonic stem (ES) cells. Each scoring parameter has been assigned an arbitrary number of points according to perceived relative importance. On the basis of this scoring system, we prioritized each of the protein components in terms of the likelihood of their importance for coactivator complex networking in nuclear receptor-dependent gene transcription. The Nuclear Receptor Signaling Atlas 2006-07-07 /pmc/articles/PMC1513068/ /pubmed/16862220 http://dx.doi.org/10.1621/nrs.04014 Text en Copyright © 2006, Han et al. This is an open-access article distributed under the terms of the Creative Commons Non-Commercial Attribution License, which permits unrestricted non-commercial use distribution and reproduction in any medium, provided the original work is properly cited.
spellingShingle Methods
Han, Sang Jun
Jung, Sung Yun
Malovannaya, Anna
Kim, Taeil
Lanz, Rainer B.
Qin, Jun
O’Malley, Bert W.
A scoring system for the follow up study of nuclear receptor coactivator complexes
title A scoring system for the follow up study of nuclear receptor coactivator complexes
title_full A scoring system for the follow up study of nuclear receptor coactivator complexes
title_fullStr A scoring system for the follow up study of nuclear receptor coactivator complexes
title_full_unstemmed A scoring system for the follow up study of nuclear receptor coactivator complexes
title_short A scoring system for the follow up study of nuclear receptor coactivator complexes
title_sort scoring system for the follow up study of nuclear receptor coactivator complexes
topic Methods
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC1513068/
https://www.ncbi.nlm.nih.gov/pubmed/16862220
http://dx.doi.org/10.1621/nrs.04014
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