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重叠的互补DNA克隆确定了与含有费城染色体的慢性粒细胞白血病细胞相关的P210c-abl基因产物的完整编码区。

Overlapping cDNA clones define the complete coding region for the P210c-abl gene product associated with chronic myelogenous leukemia cells containing the Philadelphia chromosome.

作者信息

Mes-Masson A M, McLaughlin J, Daley G Q, Paskind M, Witte O N

出版信息

Proc Natl Acad Sci U S A. 1986 Dec;83(24):9768-72. doi: 10.1073/pnas.83.24.9768.

Abstract

The Philadelphia chromosome, observed in greater than 90% of patients with chronic myelogenous leukemia, results from a reciprocal translocation between chromosomes 9 and 22. The translocation breakpoint on chromosome 9 occurs near the ABL gene and correlates with the production of a chronic myelogenous leukemia-specific 8.5-kilobase ABL-related mRNA species accompanied by a structurally altered ABL protein (P210c-abl). The N-terminal sequence of the protein is derived from the BCR gene on chromosome 22. We have isolated overlapping cDNA clones from the K-562 cell line corresponding to approximately 8.5 kilobases of mRNA and have sequenced 2550 nucleotides at the 5' end. Our results indicate that the 5' end of the 8.5-kilobase mRNA consists of greater than 400 nucleotides of noncoding sequence that are greater than 80% G + C rich. Based on our sequence analysis, we propose that initiation of translation occurs at nucleotide 471, such that the initial 927 amino acids of P210c-abl are derived from BCR sequences. Our cDNA clones thus define the complete coding sequences for the P210c-abl gene product.

摘要

在超过90%的慢性粒细胞白血病患者中观察到的费城染色体,是由9号和22号染色体之间的相互易位产生的。9号染色体上的易位断点发生在ABL基因附近,并与一种慢性粒细胞白血病特异性的8.5千碱基ABL相关mRNA物种的产生相关,同时伴有结构改变的ABL蛋白(P210c-abl)。该蛋白的N端序列来自22号染色体上的BCR基因。我们从K-562细胞系中分离出了与约8.5千碱基mRNA相对应的重叠cDNA克隆,并对5'端的2550个核苷酸进行了测序。我们的结果表明,8.5千碱基mRNA的5'端由超过400个非编码序列核苷酸组成,这些核苷酸的G + C含量超过80%。基于我们的序列分析,我们提出翻译起始于核苷酸471,因此P210c-abl最初的927个氨基酸来自BCR序列。我们的cDNA克隆因此确定了P210c-abl基因产物的完整编码序列。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/60ec/387222/483f4058fe84/pnas00328-0506-a.jpg

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