Johnson M D, Housey G M, Kirschmeier P T, Weinstein I B
Cancer Center, College of Physicians and Surgeons, Columbia University, New York, New York 10032.
Mol Cell Biol. 1987 Aug;7(8):2821-9. doi: 10.1128/mcb.7.8.2821-2829.1987.
cDNA clones representing genes whose expression is modulated by treatment with mitogens and tumor promoters were isolated and characterized. TPA-S1 corresponds to an mRNA species whose abundance was increased markedly within 1 h of exposure to the tumor promoter 12-O-tetradecanoyl phorbol-13-acetate (TPA), and TPA-R1 represents an mRNA that was decreased in TPA-treated cells. The induction of TPA-S1 was blocked by actinomycin D but was not affected by cycloheximide, and it was specific for phorbol esters with tumor-promoting activity. The role of protein kinase C in the induction of TPA-S1 is supported by the following lines of evidence. (i) Agents that activated protein kinase C (TPA, platelet-derived growth factor, and diacylglycerol) also increased TPA-S1 mRNA levels. (ii) A potent PKC inhibitor blocked the induction of TPA-S1. (iii) Down-regulation of PKC activity, by treatment of cells with TPA for 24 h, resulted in a loss of responsiveness to TPA-S1 induction by subsequent TPA treatment. DNA sequence analysis of TPA-S1 predicts a cysteine-rich, secreted protein with a molecular weight of 22.6 X 10(3) that exhibits homology with sequences representing a protein with human erythroid-potentiating activity and protease inhibitory activity.
分离并鉴定了代表其表达受促细胞分裂剂和肿瘤启动子处理调节的基因的cDNA克隆。TPA-S1对应于一种mRNA种类,其丰度在暴露于肿瘤启动子12-O-十四烷酰佛波醇-13-乙酸酯(TPA)后1小时内显著增加,而TPA-R1代表在TPA处理的细胞中减少的一种mRNA。TPA-S1的诱导被放线菌素D阻断,但不受环己酰亚胺影响,并且它对具有肿瘤促进活性的佛波酯具有特异性。蛋白激酶C在TPA-S1诱导中的作用得到以下几方面证据的支持。(i)激活蛋白激酶C的试剂(TPA、血小板衍生生长因子和二酰基甘油)也增加了TPA-S1 mRNA水平。(ii)一种有效的PKC抑制剂阻断了TPA-S1的诱导。(iii)通过用TPA处理细胞24小时来下调PKC活性,导致随后用TPA处理时对TPA-S1诱导的反应性丧失。TPA-S1的DNA序列分析预测了一种富含半胱氨酸的分泌蛋白,分子量为22.6×10³,与代表具有人红细胞增强活性和蛋白酶抑制活性的蛋白的序列具有同源性。
