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针对顺铂耐药相关ABC转运蛋白cMOAT/MRP2/ABCC2的核酶的动力学特性

Kinetic characterization of ribozymes directed against the cisplatin resistance-associated ABC transporter cMOAT/MRP2/ABCC2.

作者信息

Materna V, Holm P S, Dietel M, Lage H

机构信息

Institute of Pathology, Humboldt University Berlin, Germany.

出版信息

Cancer Gene Ther. 2001 Mar;8(3):176-84. doi: 10.1038/sj.cgt.7700293.

Abstract

The enhanced expression of the human ABC transporter, cMOAT (MRP2/ABCC2), is associated with resistance of tumor cells against platinum-containing compounds, such as cisplatin. Therefore, cMOAT represents an interesting candidate factor for modulation of antineoplastic drug resistance. Two different hammerhead ribozymes, which exhibit high catalytic cleavage activities towards specific RNA sequences encoding cMOAT, were designed. Cleavage sites of these ribozymes are the GUC sites in codons 704 and 708 of the open reading frame in the cMOAT-specific mRNA molecule. Hammerhead ribozymes were in vitro synthesized using bacteriophage T7 RNA polymerase and oligonucleotide primers whereby one primer contains a T7 RNA polymerase promoter sequence. cMOAT-encoding substrate RNA molecules were created by a reverse transcription polymerase chain reaction using RNA prepared from the cisplatin-resistant human ovarian carcinoma cell line A2780RCIS overexpressing the cMOAT-encoding transcript. In a cell-free system, both anti-cMOAT ribozymes cleaved their substrate in a highly efficient manner at a physiologic pH and temperature. The cleavage reaction was dependent on time and ribozyme:substrate ratio for determining specific kinetic parameters.

摘要

人ABC转运蛋白cMOAT(MRP2/ABCC2)的表达增强与肿瘤细胞对含铂化合物(如顺铂)的耐药性相关。因此,cMOAT是调节抗肿瘤药物耐药性的一个有趣的候选因素。设计了两种不同的锤头状核酶,它们对编码cMOAT的特定RNA序列具有高催化切割活性。这些核酶的切割位点是cMOAT特异性mRNA分子开放阅读框中第704和708密码子中的GUC位点。使用噬菌体T7 RNA聚合酶和寡核苷酸引物体外合成锤头状核酶,其中一个引物包含T7 RNA聚合酶启动子序列。通过逆转录聚合酶链反应,使用从过表达编码cMOAT转录本的顺铂耐药人卵巢癌细胞系A2780RCIS制备的RNA,产生编码cMOAT的底物RNA分子。在无细胞系统中,两种抗cMOAT核酶在生理pH和温度下以高效方式切割其底物。切割反应取决于时间和核酶与底物的比例,以确定特定的动力学参数。

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