Two regions responsible for the actin binding of p57, a mammalian coronin family actin-binding protein

被引:0
作者
Oku, T
Itoh, S
Okano, M
Suzuki, A
Suzuki, K
Nakajin, S
Tsuji, T
Nauseef, WM
Toyoshima, S
机构
[1] Hoshi Univ, Sch Pharm & Pharmaceut Sci, Shinagawa Ku, Tokyo 1428501, Japan
[2] Japan Tobacco Inc, Pharmaceut Frontier Res Labs, Kanazawa Ku, Yokohama, Kanagawa 2360004, Japan
[3] Univ Iowa, Inflammat Program, Iowa City, IA 52242 USA
[4] Univ Iowa, Dept Med, Iowa City, IA 52242 USA
[5] Vet Affairs Med Ctr, Iowa City, IA 52242 USA
[6] Natl Inst Hlth Sci, Pharmaceut & Med Devices Evaluat Ctr, Minato Ku, Tokyo 1058409, Japan
关键词
actin-binding protein; coronin; cytoskeleton; WD repeats; leucine zipper;
D O I
暂无
中图分类号
R9 [药学];
学科分类号
1007 ;
摘要
The actin-binding protein p57, a member of the coronin protein family, is expressed in a variety of immune cells. It has five WD repeats and a coiled-coil motif containing A leucine zipper, both of which are known to mediate protein-protein interactions. In order to identify the precise actin-binding regions in p57, and to assess the contribution of these structural motifs, we prepared various truncated p57 as fusion proteins with glutathione S-transferase (GST) and examined their actin-binding activity. A co-sedimentation assay demonstrated that p57(1-371) (C-terminal truncated p57) had the ability to bind F-actin, but p57(372-461) (a fragment containing the coiled-coil motif) did not. A segment consisting of the N-terminal 34 amino acids of p57 (p57(1-34)) was found to bind to F-actin in the co-sedimentation assay. Furthermore, fluorescence microscopic observation showed that p57(1-34) was co-localized with F-actin in COS-1 cells after the transfection with the p57(1-34) construct. Deletion of (KFRHVF15)-K-10, a sequence conserved among coronin-related proteins, from p57(1-34) abolished its actin-binding activity, suggesting that this sequence with basic and hydrophobic amino acids is crucial for p57 to bind to F-actin. However, the N-terminal deletion mutant p57(63-461) retained the binding ability to F-actin. This result suggests the presence of a second actin-binding region. Further deletion analysis revealed that p57(111-204), which includes the second and third WD repeats, also exhibited weak actin-binding activity in the co-sedimentation assay. Taken together, these data strongly suggest that at least two regions within Met-1 to Asp-34 and IIe-III to Glu-204 of p57 are responsible for its binding to the actin cytoskeleton.
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页码:409 / 416
页数:8
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