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培养肌细胞的核内肌动蛋白棒中ADF与丝切蛋白的共定位。

Colocalization of ADF and cofilin in intranuclear actin rods of cultured muscle cells.

作者信息

Ono S, Abe H, Nagaoka R, Obinata T

机构信息

Department of Biology, Faculty of Science, Chiba University, Japan.

出版信息

J Muscle Res Cell Motil. 1993 Apr;14(2):195-204. doi: 10.1007/BF00115454.

Abstract

Immunofluorescence microscopy revealed that two actin-binding proteins of low molecular weight with different functional activity, ADF and cofilin, are transported into nuclei of cultured myogenic cells to form rod structures there together with actin, when the cells were incubated in medium containing dimethylsulfoxide. In most cases, ADF and cofilin colocalized in the same nuclear actin rods, but ADF appeared to predominate in mononucleated cells, while cofilin was present in multinucleated myotubes. In some mononucleated cells, the nuclear actin rods were composed of ADF and actin but devoid of cofilin. An ADF homologue in mammals, destrin, was also translocated into nuclear actin rods under similar conditions. As a nuclear transport signal sequence exists in cofilin and ADF but not in actin, ADF and/or cofilin may be responsible for the nuclear import of actin in myogenic cells under certain conditions.

摘要

免疫荧光显微镜检查显示,当在含有二甲基亚砜的培养基中培养细胞时,两种具有不同功能活性的低分子量肌动蛋白结合蛋白,即ADF和丝切蛋白,会被转运到培养的成肌细胞核中,并在那里与肌动蛋白一起形成杆状结构。在大多数情况下,ADF和丝切蛋白共定位于相同的核肌动蛋白杆中,但ADF似乎在单核细胞中占主导地位,而丝切蛋白则存在于多核肌管中。在一些单核细胞中,核肌动蛋白杆由ADF和肌动蛋白组成,但不含丝切蛋白。在类似条件下,哺乳动物中的ADF同源物,即肌动蛋白解聚因子,也会转位到核肌动蛋白杆中。由于丝切蛋白和ADF中存在核转运信号序列,而肌动蛋白中不存在,因此在某些条件下,ADF和/或丝切蛋白可能负责成肌细胞核中肌动蛋白的核输入。

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