Regulation of mda-7 gene expression during human melanoma differentiation

被引:0
|
作者
Malavi T Madireddi
Paul Dent
Paul B Fisher
机构
[1] Herbert Irving Comprehensive Cancer Center,Department of Urology
[2] Columbia University,Department of Radiation Oncology
[3] College of Physicians and Surgeons,Department of Neurosurgery
[4] Medical College of Virginia,Department of Pathology
[5] Virginia Commonwealth University,undefined
[6] Herbert Irving Comprehensive Cancer Center,undefined
[7] Columbia University,undefined
[8] College of Physicians and Surgeons,undefined
[9] Herbert Irving Comprehensive Cancer Center,undefined
[10] Columbia University,undefined
[11] College of Physicians and Surgeons,undefined
来源
Oncogene | 2000年 / 19卷
关键词
human melanoma; posttranscriptional gene regulation; 3′-UTR; AUUUA;
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学科分类号
摘要
Induction of irreversible growth arrest and terminal differentiation in human melanoma cells following treatment with recombinant human fibroblast interferon (IFN-β) and mezerein (MEZ) results in elevated expression of a specific melanoma differentiation associated gene, mda-7. Experiments were conducted to define the mechanism involved in the regulation of mda-7 expression in differentiating human melanoma cells. The mda-7 gene is actively transcribed in uninduced HO-1 human melanoma cells and the rate of transcription of mda-7 is not significantly enhanced by treatment with IFN-β, MEZ or IFN-β+MEZ. The high basal activity of the mda-7 promoter in uninduced melanoma cells and the absence of enhancing effect upon treatment with differentiation inducers is corroborated by transfection studies using the promoter region of mda-7 linked to a luciferase reporter gene containing the SV40 polyadenylation signal sequence. RT–PCR analysis detects the presence of low levels of mda-7 transcripts in uninduced and concomitant increases in differentiation inducer treated HO-1 cells. However, steady-state mda-7 mRNA is detected only in IFN-β+MEZ and to a lesser degree in MEZ treated cells. We show that induction of terminal differentiation of HO-1 cells with IFN-β+MEZ dramatically increases the half-life of mda-7 mRNA while treatment with cycloheximide results in detectable mda-7 mRNA in control and inducer treated cells. These observations confirm constitutive activity of the mda-7 promoter in HO-1 cells irrespective of differentiation status suggesting posttranscriptional processes as important determinants of mda-7 expression during terminal differentiation. The 3′ UTR region of mda-7 contains AU-rich elements (ARE) that contribute to rapid mda-7 mRNA turnover during proliferation and reversible differentiation, a process controlled by a labile protein factor(s). Substitution of the SV40 polyadenylation signal sequence in the luciferase reporter plasmid with the mda-7-ARE-3′-UTR renders the Luciferase message unstable when expressed in proliferating and reversibly differentiated melanoma cells. In contrast, the luciferase message is stabilized when the mda-7-ARE-3′-UTR construct is expressed in terminally differentiated HO-1 cells. These results provide compelling evidence that mda-7 expression during terminal differentiation in human melanoma cells is regulated predominantly at a posttranscriptional level.
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页码:1362 / 1368
页数:6
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