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Cloning and complete nucleotide sequence of a full-length cDNA encoding a catalytically functional tumor-associated aldehyde dehydrogenase.

机译：编码催化功能性肿瘤相关醛脱氢酶的全长cDNA的克隆和完整核苷酸序列。

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摘要

To study the mechanism(s) controlling expression of the tumor-associated aldehyde dehydrogenase (tumor ALDH), which appears during rat hepatocarcinogenesis, cDNAs encoding this isozyme were cloned and identified with an antibody probe. Poly(A)-containing RNA from HTC rat hepatoma cells, which have been shown to possess high levels of tumor ALDH, was used as template to synthesize double-stranded cDNA. The cDNA was methylated to protect internal sites. Two different synthetic DNA linkers were added sequentially to the cDNA to insure correct orientation for expression from the lac promoter of pUC8. A library of 100,000 independent members carrying inserts greater than 1 kilobase was obtained. From this library, two apparently identical tumor ALDH clones, differing only in size, were identified with an indirect immunological probe. The larger of the cDNA clones identified, pTALDH, was chosen for further study. Interestingly, since tumor ALDH is a dimeric enzyme, pTALDH directs synthesis of a functional tumor ALDH in the bacterial cell. The cDNA sequence has been confirmed by comparison to the amino acid sequence of tumor ALDH purified from HTC cells.

机译：为了研究控制在大鼠肝癌发生过程中出现的肿瘤相关醛脱氢酶（肿瘤ALDH）表达的机制，克隆了编码该同工酶的cDNA，并用抗体探针进行了鉴定。来自HTC大鼠肝癌细胞的含Poly（A）的RNA已被证明具有高水平的肿瘤ALDH，被用作模板来合成双链cDNA。 cDNA被甲基化以保护内部位点。依次将两个不同的合成DNA接头添加到cDNA中，以确保从pUC8的lac启动子表达的正确方向。获得了一个100,000个独立成员的库，这些成员携带的插入物大于1公里。从该文库中，用间接免疫探针鉴定了两个大小明显不同的明显相同的肿瘤ALDH克隆。选择了更大的已鉴定cDNA克隆pTALDH进行进一步研究。有趣的是，由于肿瘤ALDH是二聚酶，因此pTALDH指导细菌细胞中功能性肿瘤ALDH的合成。通过与从HTC细胞纯化的肿瘤ALDH的氨基酸序列比较，已经确认了该cDNA序列。

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Jones, D E; Brennan, M D; Hempel, J; Lindahl, R;
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年度 1988
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Cloning and complete nucleotide sequence of a full-length cDNA encoding a catalytically functional tumor-associated aldehyde dehydrogenase.

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