The N-terminal half of the Drosophila Rel/NF-κB factor Relish, REL-68, constitutively activates transcription of specific Relish target genes

被引:36
|
作者
Wiklund, Magda-Lena [2 ]
Steinert, Stefanie [1 ]
Junell, Anna [3 ]
Hultmark, Dan [2 ]
Stoven, Svenja [1 ]
机构
[1] Umea Univ, Dept Clin Microbiol, S-90185 Umea, Sweden
[2] Umea Univ, Umea Ctr Mol Pathogenesis, S-90187 Umea, Sweden
[3] Stockholm Univ, Dept Mol Biol & Funct Genom, S-10961 Stockholm, Sweden
基金
瑞典研究理事会;
关键词
Innate immune response; Rel homology domain; I kappa B-like; Phosphorylation; Caspase cleavage; Scaffolding; Compound Rel protein; Antimicrobial peptide gene; INNATE IMMUNE-RESPONSE; CELLULAR-IMMUNITY; INSECT IMMUNITY; DOWN-REGULATION; NUCLEAR IMPORT; PROTEIN; DORSAL; PHOSPHORYLATION; EXPRESSION; DEFENSE;
D O I
10.1016/j.dci.2008.12.002
中图分类号
S9 [水产、渔业];
学科分类号
0908 ;
摘要
The Rel/NF-kappa B transcription factor Relish is a major regulator of the antimicrobial response in Drosophila. Upon immune challenge, Relish is cleaved to generate two fragments, the DNA-binding transcription factor REL-68 and the I kappa B-like REL-49. Using transgenic fly strains we show here that overexpression of REL-68 separately from REL-49 is sufficient to activate strong constitutive transcription of the Diptericin gene, but little constitutive or inducible transcription of Attacin and Cecropin, two other Relish target genes. Their transcription may therefore require additional modifications of Relish. However, phosphorylation of the conserved serine residue S431 is not involved in such modifications. This is unlike p65 and Dorsal, which are modulated by phosphorylation at their homologous site. In contrast to other I kappa B proteins, overexpression of REL-49 had no inhibitory effect on Relish-dependent transcription. Instead, we propose that the C-terminal I kappa B-like domain executes a scaffolding and recruiting function for full activation of Relish. (c) 2008 Elsevier Ltd. All rights reserved.
引用
收藏
页码:690 / 696
页数:7
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