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从人类DNA克隆文库中分离和鉴定连锁的δ-和β-珠蛋白基因。

The isolation and characterization of linked delta- and beta-globin genes from a cloned library of human DNA.

作者信息

Lawn R M, Fritsch E F, Parker R C, Blake G, Maniatis T

出版信息

Cell. 1978 Dec;15(4):1157-74. doi: 10.1016/0092-8674(78)90043-0.

DOI:10.1016/0092-8674(78)90043-0
PMID:728996
Abstract

A cloned library of large, random embryonic human DNA fragments was constructed and screened for beta-globin sequences using the cloned human beta-globin cDNA plasmid pJW102 (Wilson et al., 1978) as a hybridization probe. Two independent clones were obtained and then characterized by restriction endonuclease cleavage analysis, hybridization experiments and partial DNA sequencing. Each of the clones carries both the adult delta- and beta-globin genes. The two genes are separated by approximately 5.4 kilobases (kb) of DNA and their orientation with respect to the direction of transcription is 5'-delta--beta-3'. Both the delta- and beta-globin genes contain a large noncoding intervening sequence (950 and 900 bp, respectively) located between the codons for amino acids 104 (arginine) and 105 (leucine). Although the location of the large intervening sequence within the coding regions of the two genes is identical, the two noncoding sequences bear little sequence homology. A second, smaller intervening sequence similar to that found in other mammalian beta-globin genes was detected near the 5' end of the human beta-globin gene. The two independently isolated beta-globin clones differ from each other by the presence of a Pst I restriction enzyme cleavage site within the large intervening sequence of the delta-globin gene of one of the clones. This suggests that the human DNA carried in the two clones was derived from two homologous chromosomes which were heterozygous for the Pst I restriction enzyme recognition sequence.

摘要

构建了一个包含大型随机人胚胎DNA片段的克隆文库,并用克隆的人β - 珠蛋白cDNA质粒pJW102(Wilson等人,1978年)作为杂交探针筛选β - 珠蛋白序列。获得了两个独立的克隆,然后通过限制性内切酶切割分析、杂交实验和部分DNA测序进行表征。每个克隆都携带成人δ - 和β - 珠蛋白基因。这两个基因被大约5.4千碱基(kb)的DNA隔开,它们相对于转录方向的方向是5'-δ--β-3'。δ - 和β - 珠蛋白基因都包含一个大的非编码间隔序列(分别为950和900 bp),位于氨基酸104(精氨酸)和105(亮氨酸)的密码子之间。尽管两个基因编码区内大间隔序列的位置相同,但这两个非编码序列几乎没有序列同源性。在人β - 珠蛋白基因的5'端附近检测到第二个较小的间隔序列,类似于在其他哺乳动物β - 珠蛋白基因中发现的序列。两个独立分离的β - 珠蛋白克隆彼此不同,原因是其中一个克隆的δ - 珠蛋白基因的大间隔序列内存在一个Pst I限制性内切酶切割位点。这表明两个克隆中携带的人DNA来自两条同源染色体,它们对于Pst I限制性内切酶识别序列是杂合的。

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