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转化小鼠成纤维细胞主要分泌蛋白基因的克隆与表达。一种受转化调控的分泌型溶酶体蛋白酶。

Cloning and expression of the gene for the major excreted protein of transformed mouse fibroblasts. A secreted lysosomal protease regulated by transformation.

作者信息

Troen B R, Ascherman D, Atlas D, Gottesman M M

机构信息

Laboratory of Molecular Biology, National Cancer Institute, Bethesda, Maryland 20892.

出版信息

J Biol Chem. 1988 Jan 5;263(1):254-61.

PMID:2826441
Abstract

The major excreted protein (MEP) of mouse fibroblast cells is the 39,000 Mr precursor to a lysosomal acid protease (cathepsin L) induced by malignant transformation, growth factors, and tumor promoters. We have cloned and characterized the gene for MEP from NIH-3T3 cells. This cosmid clone (pcosMMEP), containing the unique 12,000-base pair mouse MEP gene, has been transfected into monkey kidney (CV-1) cells and human epidermoid carcinoma (A431) cells. The stable A4MEP transfectants produce mouse MEP that is an active cathepsin which is secreted, glycosylated, and processed intracellularly to lower molecular weight forms as in the wild-type NIH-3T3 cells. The CVMEP cells (nontransformed phenotype) produce quantities of mouse MEP similar to that found in NIH-3T3 cells, whereas the A4MEP cells (transformed phenotype) produce greater amounts of MEP similar to the levels seen in Kirsten virus-transformed NIH-3T3 cells. The MEP mRNAs from both mouse cells and stably transfected human cells are the same size and have the same single major site for initiation of transcription, indicating that the cloned mouse MEP promoter is active in transfected cells.

摘要

小鼠成纤维细胞的主要分泌蛋白(MEP)是一种分子量为39,000的前体蛋白,它可被恶性转化、生长因子和肿瘤启动子诱导生成溶酶体酸性蛋白酶(组织蛋白酶L)。我们已从小鼠成纤维细胞NIH-3T3中克隆并鉴定了MEP基因。这个黏粒克隆(pcosMMEP)包含独特的12,000碱基对的小鼠MEP基因,已被转染到猴肾(CV-1)细胞和人表皮样癌(A431)细胞中。稳定的A4MEP转染细胞产生小鼠MEP,它是一种有活性的组织蛋白酶,能像野生型NIH-3T3细胞那样被分泌、糖基化并在细胞内加工成较低分子量的形式。CVMEP细胞(非转化表型)产生的小鼠MEP量与NIH-3T3细胞中的相似,而A4MEP细胞(转化表型)产生的MEP量更多,与柯斯顿病毒转化的NIH-3T3细胞中的水平相似。来自小鼠细胞和稳定转染的人细胞的MEP mRNA大小相同,且具有相同的单一主要转录起始位点,这表明克隆的小鼠MEP启动子在转染细胞中具有活性。

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