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骨骼肌LIM蛋白1(SLIM1)两种同工型的特性。SLIM1定位于粘着斑,而其同工型slimmer定位于成肌细胞的细胞核和肌管的细胞质,这表明它们在细胞骨架和核质通讯中具有不同的作用。

Characterization of two isoforms of the skeletal muscle LIM protein 1, SLIM1. Localization of SLIM1 at focal adhesions and the isoform slimmer in the nucleus of myoblasts and cytoplasm of myotubes suggests distinct roles in the cytoskeleton and in nuclear-cytoplasmic communication.

作者信息

Brown S, McGrath M J, Ooms L M, Gurung R, Maimone M M, Mitchell C A

机构信息

Department of Biochemistry and Molecular Biology, Monash University, Clayton, Victoria, Australia 3168.

出版信息

J Biol Chem. 1999 Sep 17;274(38):27083-91. doi: 10.1074/jbc.274.38.27083.

DOI:10.1074/jbc.274.38.27083
PMID:10480922
Abstract

We have cloned and characterized a novel isoform of the skeletal muscle LIM protein 1 (SLIM1), designated SLIMMER. SLIM1 contains an N-terminal single zinc finger followed by four LIM domains. SLIMMER is identical to SLIM1 over the first three LIM domains but contains a novel C-terminal 96 amino acids with three potential bipartite nuclear localization signals, a putative nuclear export sequence, and 27 amino acids identical to the RBP-J binding region of KyoT2, a murine isoform of SLIM1. SLIM1 localized to the cytosol of Sol8 myoblasts and myotubes. SLIMMER was detected in the nucleus of myoblasts and, following differentiation into myotubes, was exclusively cytosolic. Recombinant green fluorescent protein-SLIM1 localized to the cytoplasm and associated with focal adhesions and actin filaments in COS-7 cells, while green fluorescent protein-SLIMMER was predominantly nuclear. SLIMMER truncation mutants revealed that the first nuclear localization signal mediates nuclear localization. The addition of the proposed nuclear export sequence decreased the level of exclusively nuclear expression and increased cytosolic SLIMMER expression in COS-7 cells. The leucine-rich nuclear export signal was required for the export of SLIMMER from the nucleus of myoblasts to the cytoplasm of myotubes. Collectively, these results suggest distinct roles for SLIM1 and SLIMMER in focal adhesions and nuclear-cytoplasmic communication.

摘要

我们已经克隆并鉴定了一种新型的骨骼肌LIM蛋白1(SLIM1)同工型,命名为SLIMMER。SLIM1包含一个N端单锌指,其后跟着四个LIM结构域。SLIMMER在前三个LIM结构域上与SLIM1相同,但包含一个新的C端96个氨基酸序列,具有三个潜在的双分型核定位信号、一个假定的核输出序列,以及27个与KyoT2(SLIM1的一种小鼠同工型)的RBP-J结合区域相同的氨基酸。SLIM1定位于Sol8成肌细胞和肌管的细胞质中。在成肌细胞的细胞核中检测到了SLIMMER,在分化为肌管后,它只存在于细胞质中。重组绿色荧光蛋白-SLIM1定位于COS-7细胞的细胞质中,并与粘着斑和肌动蛋白丝相关,而绿色荧光蛋白-SLIMMER主要定位于细胞核中。SLIMMER截短突变体表明,第一个核定位信号介导核定位。在COS-7细胞中,添加提议的核输出序列降低了仅在细胞核中表达的水平,并增加了细胞质中SLIMMER的表达。富含亮氨酸的核输出信号是SLIMMER从成肌细胞核输出到肌管细胞质所必需的。总的来说,这些结果表明SLIM1和SLIMMER在粘着斑和核质通讯中具有不同的作用。

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