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Mediation of suppression of c‐fos transcription in rasT24‐transformed rat cells by a cis‐acting represser element
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AbstractProlonged expression of activated ras mutants resulted in both neoplastic transformation and suppression of serum‐induced c‐fos expression in Rat1 fibroblasts. Expression of other serum‐inducible genes, including c‐jun and β‐actin, was not suppressed in ras‐transformed Rat1 cells, indicating that these effects are specific for c‐fos and that growth‐factor signal transduction pathways remain essentially intact. Run‐on transcription studies indicated that c‐fos transcription was blocked at the level of initiation in these cells. Transient transfection studies using 360 bp from the wild‐type c‐fos promoter as well as a series of mutated c‐fos promoter fragments linked to the chloramphenicol acetyltransferase gene indicated that repression of c‐fos was mediated by approximately 49 bp immediately upstream of the dyad symmetry element (DSE). Deletion of this region, referred to as the upstream represser region (URR), restored serum inducibility to the c‐fos promoter in ras‐transformed cells. In contrast, suppression of c‐fos transcription was not affected by either deletion of 240 bp between the DSE and the TATA element or by base‐substitution mutations that inactivate the ternary complex factor and fos‐AP‐1‐like binding sites. In addition, in vitro competition studies indicated that ras‐transformed cells express one or more represser factors that interact with as‐yet‐unidentified elements within the c‐fos promoter (possibly the URR) and block serum induction of c‐fos. These findings suggest that prolonged expression of activated ras results in the activation of one or more as‐yet‐unidentified proteins that suppress transcription of the c‐fos gene by interacting with the URR. © 1994 Wiley‐Liss, Inc.
Title: Mediation of suppression of c‐fos transcription in rasT24‐transformed rat cells by a cis‐acting represser element
Description:
AbstractProlonged expression of activated ras mutants resulted in both neoplastic transformation and suppression of serum‐induced c‐fos expression in Rat1 fibroblasts.
Expression of other serum‐inducible genes, including c‐jun and β‐actin, was not suppressed in ras‐transformed Rat1 cells, indicating that these effects are specific for c‐fos and that growth‐factor signal transduction pathways remain essentially intact.
Run‐on transcription studies indicated that c‐fos transcription was blocked at the level of initiation in these cells.
Transient transfection studies using 360 bp from the wild‐type c‐fos promoter as well as a series of mutated c‐fos promoter fragments linked to the chloramphenicol acetyltransferase gene indicated that repression of c‐fos was mediated by approximately 49 bp immediately upstream of the dyad symmetry element (DSE).
Deletion of this region, referred to as the upstream represser region (URR), restored serum inducibility to the c‐fos promoter in ras‐transformed cells.
In contrast, suppression of c‐fos transcription was not affected by either deletion of 240 bp between the DSE and the TATA element or by base‐substitution mutations that inactivate the ternary complex factor and fos‐AP‐1‐like binding sites.
In addition, in vitro competition studies indicated that ras‐transformed cells express one or more represser factors that interact with as‐yet‐unidentified elements within the c‐fos promoter (possibly the URR) and block serum induction of c‐fos.
These findings suggest that prolonged expression of activated ras results in the activation of one or more as‐yet‐unidentified proteins that suppress transcription of the c‐fos gene by interacting with the URR.
© 1994 Wiley‐Liss, Inc.
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