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S100相关钙结合蛋白pEL98(或mts1)在细胞运动性和肿瘤细胞侵袭中的作用。

Involvement of S100-related calcium-binding protein pEL98 (or mts1) in cell motility and tumor cell invasion.

作者信息

Takenaga K, Nakamura Y, Endo H, Sakiyama S

机构信息

Division of Chemotherapy, Chiba Cancer Center Research Institute.

出版信息

Jpn J Cancer Res. 1994 Aug;85(8):831-9. doi: 10.1111/j.1349-7006.1994.tb02955.x.

Abstract

We examined the relationship between cell motility and the expressions of pEL98 (mts1) mRNA and protein in various murine normal and transformed cells. The expression of pEL98 (mts1) in v-Ha-ras-transformed NIH3T3 cells and in normal rat kidney cells transformed by either v-Ha-ras or v-src was increased over that in the corresponding parental cells at both mRNA and protein levels. The expression in normal rat fibroblasts (3Y1) transformed by v-Ha-ras was also increased compared with that in 3Y1 cells. However, the expression of pEL98 (mts1) in 3Y1 cells transformed by v-src was increased in one clone (src 3Y1-K), but decreased in another clone (src 3Y1-H). The expression level of pEL98 (mts1) correlated well with cell motility, which was examined by measuring cell tracks by phagokinesis. In order to test direct involvement of the pEL98 (mts1) protein in cell motility, src 3Y1-H cells that showed low cell motility were transfected with pEL98 cDNA. The transfectants expressing large amounts of the pEL98 protein showed significantly higher cell motility than src 3Y1-H cells. The expression of pEL98 (mts1) was also found to be correlated with motile and invasive abilities in various clones derived from Lewis lung carcinoma. These results suggest that the pEL98 (mts1) protein plays a role in regulating cell motility and tumor cell invasiveness.

摘要

我们研究了多种小鼠正常细胞和转化细胞中细胞运动性与pEL98(mts1)mRNA及蛋白表达之间的关系。在v-Ha-ras转化的NIH3T3细胞以及由v-Ha-ras或v-src转化的正常大鼠肾细胞中,pEL98(mts1)在mRNA和蛋白水平上的表达均高于相应的亲本细胞。与3Y1细胞相比,v-Ha-ras转化的正常大鼠成纤维细胞(3Y1)中pEL98(mts1)的表达也有所增加。然而,v-src转化的3Y1细胞中,pEL98(mts1)在一个克隆(src 3Y1-K)中表达增加,而在另一个克隆(src 3Y1-H)中表达降低。pEL98(mts1)的表达水平与细胞运动性密切相关,细胞运动性通过吞噬运动测量细胞轨迹来检测。为了测试pEL98(mts1)蛋白是否直接参与细胞运动,将细胞运动性较低的src 3Y1-H细胞用pEL98 cDNA进行转染。表达大量pEL98蛋白的转染子显示出比src 3Y1-H细胞显著更高的细胞运动性。在源自Lewis肺癌的各种克隆中,还发现pEL98(mts1)的表达与运动和侵袭能力相关。这些结果表明,pEL98(mts1)蛋白在调节细胞运动性和肿瘤细胞侵袭性中发挥作用。

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