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十四烷酰佛波醇酯诱导的“初级反应”序列的克隆及其在密度抑制的瑞士3T3细胞和一种佛波酯不增殖变异体中的表达。

Cloning of tetradecanoyl phorbol ester-induced 'primary response' sequences and their expression in density-arrested Swiss 3T3 cells and a TPA non-proliferative variant.

作者信息

Lim R W, Varnum B C, Herschman H R

机构信息

Department of Biological Chemistry, UCLA Center for the Health Sciences 90024.

出版信息

Oncogene. 1987;1(3):263-70.

PMID:3330774
Abstract

The tumor promoter tetradecanoyl phorbol acetate (TPA) is also a potent mitogen for murine 3T3 cells. We have previously described the isolation of variant Swiss 3T3 cell lines unable to proliferative in response to TPA. In this report we sought to identify genes that are stimulated by TPA as 'primary responses', i.e., without intervening protein synthesis. We constructed a cDNA library in lambda gt10, using RNA from quiescent 3T3 cells treated with TPA in the presence of cycloheximide (CHX). Of 50,000 recombinant phages, we identified 50 isolates that demonstrated preferential hybridization to cDNA probes generated from TPA-stimulated cells. One of the clones contains a fragment of the proto-oncogene c-fos. Twenty-nine of the remaining 49 clones fall into six cross-hybridization families. All the characterized clones detected mRNAs that are also inducible by epidermal growth factor, fibroblast growth factor or elevated serum. TPA induction of all the characterized messages is rapid and transient. All these mRNAs are superinduced by a combination of mitogens and CHX. Induction of these messages following TPA addition also occurs in subconfluent 3T3 cultures; expression of these genes is, therefore, not restricted to the G0/G1 transition. Expression of all six clones was also induced by TPA and other mitogens in 3T3-TNR9 cells, a TPA non-proliferative variant.

摘要

肿瘤促进剂十四酰佛波醇乙酸酯(TPA)也是鼠3T3细胞的一种强效促有丝分裂剂。我们之前描述过分离出的瑞士3T3细胞系变体,它们对TPA无增殖反应。在本报告中,我们试图鉴定作为“初级反应”被TPA刺激的基因,即无需中间蛋白质合成的基因。我们用在放线菌酮(CHX)存在下经TPA处理的静止3T3细胞的RNA构建了λgt10 cDNA文库。在50,000个重组噬菌体中,我们鉴定出50个分离株,它们与从TPA刺激的细胞产生的cDNA探针表现出优先杂交。其中一个克隆包含原癌基因c-fos的一个片段。其余49个克隆中的29个属于六个交叉杂交家族。所有已鉴定的克隆检测到的mRNA也可被表皮生长因子、成纤维细胞生长因子或升高的血清诱导。所有已鉴定信息的TPA诱导都是快速且短暂的。所有这些mRNA在有丝分裂原和CHX共同作用下被超诱导。在亚汇合的3T3培养物中加入TPA后也会诱导这些信息的表达;因此这些基因的表达不限于G0/G1期转换阶段。在TPA无增殖反应变体3T3-TNR9细胞中,TPA和其他有丝分裂原也诱导了所有六个克隆的表达。

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