Literature DB >> 2470651

The promoter elements of the mouse myelin basic protein gene function efficiently in NG108-15 neuronal/glial cells.

M Miura1, T Tamura, A Aoyama, K Mikoshiba.   

Abstract

We measured transiently-expressed beta-galactosidase activity by introducing the mouse myelin basic protein (MBP)-lacZ chimeric gene (MBP-lacZ) into the NG108-15 neuronal/glial hybrid cell line. Deletion studies of the promoter region of the MBP gene showed that the promoter region between -1318 bp and -254 bp might contain sequences that repress MBP promoter activity. Fine deletion analysis using BAL 31 exonuclease revealed sequences between bp -208 and -140, -139 and -118, and -89 and -75 which were critical for promoter activity in NG 108-15 cells. DNaseI footprinting analysis revealed a cellular factor(s) that bind to the promoter region between bp -127 and -106 with NG108-15 whole cell extracts. The SV40 promoter was activated by insertion of the sequences around the region protected in footprinting experiments, in a manner independent of its orientation in NG108-15 cells. This protected region is thought to be one of the critical cis-acting DNA elements for efficient transcription.

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Year:  1989        PMID: 2470651     DOI: 10.1016/0378-1119(89)90380-6

Source DB:  PubMed          Journal:  Gene        ISSN: 0378-1119            Impact factor:   3.688


  15 in total

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3.  Tissue-specific in vitro transcription from the mouse myelin basic protein promoter.

Authors:  T Tamura; A Aoyama; T Inoue; M Miura; H Okano; K Mikoshiba
Journal:  Mol Cell Biol       Date:  1989-07       Impact factor: 4.272

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9.  Stimulation of myelin basic protein gene transcription by Fyn tyrosine kinase for myelination.

Authors:  H Umemori; Y Kadowaki; K Hirosawa; Y Yoshida; K Hironaka; H Okano; T Yamamoto
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Authors:  R A Saavedra; A Lipson; K S Kimbro; C Ljubetic
Journal:  J Mol Neurosci       Date:  1993       Impact factor: 3.444

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