人小细胞肺癌细胞系中拓扑异构酶II基因重排的特征分析。

Characterization of a topoisomerase II gene rearrangement in a human small-cell lung cancer cell line.

作者信息

Binaschi M, Giaccone G, Gazdar A F, De Isabella P, Ricotti G C, Capranico G, Zunino F

机构信息

Division of Experimental Oncology B, Istituto Nazionale per lo Studio e la Cura dei Tumori, Milan, Italy.

出版信息

J Natl Cancer Inst. 1992 Nov 18;84(22):1710-6. doi: 10.1093/jnci/84.22.1710.

DOI:10.1093/jnci/84.22.1710

PMID:1331483

Abstract

BACKGROUND

Small-cell lung cancer (SCLC) is a highly chemosensitive tumor, but the recurrent disease that is common after initial response is often unresponsive to further chemotherapy. Although the mechanisms of drug resistance in SCLC have not been established, studies suggest that alterations of the nuclear enzyme DNA topoisomerase II may reduce the sensitivity of the cell to drug action. This enzyme is recognized as a primary target for cytotoxic activity of important antitumor agents.

PURPOSE

In this study, we attempted to determine if altered forms of DNA topoisomerase II are responsible for reduced drug sensitivity.

METHODS

We characterized a rearrangement of the topoisomerase II p170 gene (also known as TOP2) in a relatively chemoresistant SCLC cell line, NCI-H69, and compared topoisomerase II expression and activity in this line with those in the chemosensitive NCI-H187 cell line. Fragments of complementary DNA from the topoisomerase II gene were generated by polymerase chain reaction. Immunodetection was accomplished by using the monoclonal antibody 7E6 against the human topoisomerase II p170 isoform. Using DNA probes corresponding to different complementary DNA regions, we showed that the rearrangement was localized at the 3' terminus of one allele of the topoisomerase II gene.

RESULTS

In addition to the normal 6.2-kilobase (kb) topoisomerase II messenger RNA (mRNA), the NCI-H69 line expressed a 7.4-kb topoisomerase II transcript, presumably encoded by the rearranged allele. Moreover, this transcript, although longer than the normal mRNA, lacked a substantial portion of the 3'-terminal p170 gene coding sequence. Topoisomerase II activity in nuclear extracts, as determined by the P4 phage DNA-unknotting assay, was more easily detected and measured at lower NaCl concentrations in NCI-H69 than in NCI-H187 cells.

CONCLUSION

These results are consistent with the hypothesis that the chemoresistant NCI-H69 cell line may express, in addition to the normal enzyme, an altered topoisomerase II enzyme possibly encoded by the 7.4-kb mRNA, which in turn may be transcribed from the rearranged gene allele.

IMPLICATION

These observations emphasize the role of topoisomerase II in determining drug sensitivity and suggest that such gene rearrangements may contribute to resistance of SCLC cells to topoisomerase II inhibitors.

摘要

背景

小细胞肺癌（SCLC）是一种对化疗高度敏感的肿瘤，但初始缓解后常见的复发疾病往往对进一步化疗无反应。尽管小细胞肺癌耐药机制尚未明确，但研究表明，核酶DNA拓扑异构酶II的改变可能会降低细胞对药物作用的敏感性。这种酶被认为是重要抗肿瘤药物细胞毒性活性的主要靶点。

目的

在本研究中，我们试图确定DNA拓扑异构酶II的改变形式是否导致药物敏感性降低。

方法

我们对相对耐药的小细胞肺癌细胞系NCI-H69中拓扑异构酶II p170基因（也称为TOP2）的重排进行了表征，并将该细胞系中拓扑异构酶II的表达和活性与敏感的NCI-H187细胞系进行了比较。通过聚合酶链反应生成拓扑异构酶II基因的互补DNA片段。使用针对人类拓扑异构酶II p170亚型的单克隆抗体7E6进行免疫检测。使用对应于不同互补DNA区域的DNA探针，我们表明重排位于拓扑异构酶II基因一个等位基因的3'末端。

结果

除了正常的6.2千碱基（kb）拓扑异构酶II信使RNA（mRNA）外，NCI-H69细胞系还表达了一个7.4 kb的拓扑异构酶II转录本，推测由重排的等位基因编码。此外，该转录本虽然比正常mRNA长，但缺少3'末端p170基因编码序列的很大一部分。通过P4噬菌体DNA解结试验测定，在较低NaCl浓度下，NCI-H69细胞核提取物中的拓扑异构酶II活性比NCI-H187细胞中更容易检测和测量。