NF-BETA-A, A FACTOR REQUIRED FOR MAXIMAL INTERLEUKIN-1-BETA GENE-EXPRESSION IS IDENTICAL TO THE ETS FAMILY MEMBER PU.1 - EVIDENCE FOR STRUCTURAL ALTERATION FOLLOWING LPS ACTIVATION

被引：37

作者：

BURAS, JA

REENSTRA, WR

FENTON, MJ

机构：

[1] DEPT MED,BOSTON,MA 02118

[2] EVANS DEPT CLIN RES,BOSTON,MA 02118

[3] BOSTON UNIV,SCH MED,DEPT DERMATOL,BOSTON,MA 02118

来源：

MOLECULAR IMMUNOLOGY | 1995年 / 32卷 / 08期

关键词：

INTERLEUKIN; 1; PU.1; SPI-1; GENE EXPRESSION; TRANSCRIPTION; DNA BINDING PROTEINS;

D O I：

10.1016/0161-5890(95)00018-A

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：

We have previously identified and characterized the macrophage-, neutrophil- and B cell-specific nuclear factor beta A (NF beta A), which is involved in transcriptional regulation of the interleukin-1 beta (IL-1 beta) gene. NF beta A binds to a highly conserved sequence element located 6 bp upstream of the TATA motif within the IL-1 beta promoter and is required for maximal expression of the IL-1 beta gene. Here we show that NF beta A is identical to the previously identified ets gene family member PU.1. The NF beta A binding element shares 100% sequence identity with a novel PU.1 binding element recently found in the immunoglobulin J-chain promoter. Methylation interference DNA footprinting data demonstrated that NF beta A and PU.1 make identical protein/DNA contacts. In vitro synthesized PU.1 possesses a mobility and binding specificity identical to NF beta A as determined by electrophoretic mobility shift analysis (EMSA). Antisera directed against amino acids 39-55 of PU.1 recognizes NF beta A in a manner indistinguishable from PU.1 in EMSA 'supershift' studies. NF beta A and PU.1 also possess similiar protein structure as determined by proteolytic clipping bandshift analysis. Furthermore, we show that PU.1 is able to transactivate an NF beta A-dependent promoter when co-transfected into HeLa cells which lack PU.1/NF beta A. EMSA studies using recombinant TATA binding protein (TBP) and PU.1 suggest that PU.1 may induce assembly of a distinct TBP-dependent complex on the IL-1 beta promoter. Finally, immunohistochemical confocal laser scanning microscopy studies suggest that LPS stimulation of RAW macrophages induces a structural change in the N-terminal transcriptional activation domain of PU.1.

引用

页码：541 / &

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