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用人胞苷脱氨酶cDNA转染鼠成纤维细胞可赋予其对阿糖胞苷的抗性。

Transfection of murine fibroblast cells with human cytidine deaminase cDNA confers resistance to cytosine arabinoside.

作者信息

Momparler R L, Laliberté J, Eliopoulos N, Beauséjour C, Cournoyer D

机构信息

Département de pharmacologie, Université de Montréal, Cote Ste-Catherine, Quebec, Canada.

出版信息

Anticancer Drugs. 1996 May;7(3):266-74. doi: 10.1097/00001813-199605000-00005.

Abstract

One of the major limitations in the use of cytosine arabinoside (Ara-C) in cancer chemotherapy is the hematopoietic toxicity produced by this nucleoside analog. One approach to overcome this problem would be to insert a gene for drug resistance to Ara-C in normal hematopoietic cells to protect them from drug toxicity. An interesting candidate gene for this aim is cytidine deaminase which catalyzes the deamination of Arac-C, resulting in a significant loss of its antineoplastic activity. We have ligated the human cDNA for cytidine deaminase into the plasmid vector pMFG. Transfection of NIH 3T3-derived GP + E86 murine fibroblasts cells with this vector resulted in a marked increase (> 50-fold) in the expression of cytidine deaminase. In addition, the transfected cells showed resistance to the cytotoxic action and to the inhibition of DNA synthesis produced by Ara-C. Northern and Western blot analysis of the transfected cells showed increased expression of mRNA for cytidine deaminase and increased immunologically detectable enzyme. The ability to confer drug resistance to Ara-C through gene transfer of cytidine deaminase may have the potential as a selectable marker and for the protection of the bone marrow from the toxicity produced by this analog so as to increase its effectiveness in cancer chemotherapy.

摘要

在癌症化疗中使用阿糖胞苷(Ara-C)的主要限制之一是这种核苷类似物产生的造血毒性。克服这一问题的一种方法是在正常造血细胞中插入对Ara-C耐药的基因,以保护它们免受药物毒性。用于此目的的一个有趣的候选基因是胞苷脱氨酶,它催化阿糖胞苷的脱氨反应,导致其抗肿瘤活性显著丧失。我们已将人胞苷脱氨酶cDNA连接到质粒载体pMFG中。用该载体转染源自NIH 3T3的GP + E86小鼠成纤维细胞,导致胞苷脱氨酶的表达显著增加(> 50倍)。此外,转染的细胞对Ara-C产生的细胞毒性作用和DNA合成抑制具有抗性。对转染细胞的Northern和Western印迹分析显示,胞苷脱氨酶的mRNA表达增加,免疫可检测的酶增加。通过胞苷脱氨酶基因转移赋予对Ara-C耐药的能力可能具有作为选择标记以及保护骨髓免受该类似物产生的毒性从而提高其在癌症化疗中的有效性的潜力。

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