MUTATIONAL ANALYSIS OF INTERFERON (IFN) REGULATORY FACTOR-1 AND FACTOR-2 - EFFECTS ON THE INDUCTION OF IFN-BETA GENE-EXPRESSION

被引:0
|
作者
LIN, RT
MUSTAFA, A
NGUYEN, H
GEWERT, D
HISCOTT, J
机构
[1] SIR MORTIMER B DAVIS JEWISH HOSP,LADY DAVIS INST MED RES,ABE STERN CANC RES LAB,MONTREAL H3T 1E2,PQ,CANADA
[2] MCGILL UNIV,DEPT IMMUNOL & MICROBIOL,MONTREAL H3T 1E2,PQ,CANADA
[3] WELLCOME FDN LTD,DEPT CELL BIOL,BECKENHAM BR3 3BS,KENT,ENGLAND
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中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Interferon (IFN) regulatory factor 1 (IRF-1) and IRF-2 are structurally similar but functionally distinct transcription factors that bind to the positive regulatory domains I and III (PRDI/III) within the human IFN-beta promoter. To begin structure-function analysis of IRF-1 and IRF-8, the regulatory potential of carboxyl-terminal deletion mutants was analyzed by co-transfection studies in human cells and was correlated with DNA binding capacity. Transcriptional repression by IRF-2 was contained within the first 125 amino-terminal amino acids and correlated directly with IRF-2 DNA binding; deletion to a protein of 100 amino acids resulted in loss of repression and IRF-2 DNA binding. Thus, the carboxyl terminus appears dispensible for trans-repression. Hybrid constructs which fuse the DNA binding domain of HRF-1 and IRF-2 to the trans-activation domain of NF-kappa B p65 were also generated; both IRF-1/p65 and IRF-2/p65 chimeras were strong transcriptional activators. IRF-2-mediated repression was also dominant over trans-activation by these fusion proteins. The trans-activation region of IRF-1 resides in the carboxyl terminus, primarily carboxyl-terminal to amino acid 250. Mutation of three potential casein kinase II phosphorylation sites within the IRF carboxyl terminus failed to identify an essential site that contributes to IRF-1 trans-activation potential.
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页码:17542 / 17549
页数:8
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