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人类δ-氨基乙酰丙酸脱水酶(ALAD)基因:红系和管家mRNA的结构及可变剪接

Human delta-aminolevulinate dehydratase (ALAD) gene: structure and alternative splicing of the erythroid and housekeeping mRNAs.

作者信息

Kaya A H, Plewinska M, Wong D M, Desnick R J, Wetmur J G

机构信息

Department of Microbiology, Mount Sinai School of Medicine, New York, New York 10029.

出版信息

Genomics. 1994 Jan 15;19(2):242-8. doi: 10.1006/geno.1994.1054.

DOI:10.1006/geno.1994.1054
PMID:8188255
Abstract

Genomic clones containing human delta-aminolevulinate dehydratase (ALAD), the second enzyme in the heme pathway, were isolated, and the entire sequence was determined in both orientations (15,913 bp; GenBank Accession No. X64467). The gene contained two alternative noncoding exons, 1A and 1B, and 11 coding exons, 2-12. Ten Alu-repetitive elements were within the gene, including an inverted repeat that may have resulted from gene conversion. The housekeeping transcript, which included exon 1A and not 1B, was identified in a human adult liver cDNA library, while an erythroid-specific transcript, which contained exon 1B and not 1A, was detected in a human K562 erythroleukemia cDNA library. The promoter region upstream of housekeeping exon 1A was GC-rich and contained three potential Sp1 elements and a CCAAT box. Further upstream, there were three potential GATA-1 binding sites and an AP1 site. The promoter region upstream of erythroid-specific exon 1B had several CACCC boxes and two potential GATA-1 binding sites. To assess the tissue-specific expression of exons 1A and 1B, HeLa and K562 cells were transduced with CAT constructs containing either exon 1A or 1B and their respective upstream promoter region. Two housekeeping CAT constructs, with 450 and 1400 bp upstream of exon 1A, were expressed at similar levels in HeLa cells, whereas the erythroid-specific construct, containing the entire 450-bp promoter region upstream of exon 1B, was not. In contrast, the housekeeping and erythroid constructs were both expressed in K562 cells.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

分离出了包含人δ-氨基-γ-酮戊酸脱水酶(ALAD,血红素途径中的第二种酶)的基因组克隆,并确定了其两个方向的完整序列(15,913 bp;GenBank登录号X64467)。该基因包含两个选择性非编码外显子1A和1B,以及11个编码外显子2 - 12。基因内有10个Alu重复元件,包括一个可能由基因转换产生的反向重复序列。在人成人肝脏cDNA文库中鉴定出包含外显子1A而非1B的管家转录本,而在人K562红白血病cDNA文库中检测到包含外显子1B而非1A的红系特异性转录本。管家外显子1A上游的启动子区域富含GC,包含三个潜在的Sp1元件和一个CCAAT盒。再往上,有三个潜在的GATA - 1结合位点和一个AP1位点。红系特异性外显子1B上游的启动子区域有几个CACCC盒和两个潜在的GATA - 1结合位点。为了评估外显子1A和1B的组织特异性表达,用含有外显子1A或1B及其各自上游启动子区域的CAT构建体转导HeLa和K562细胞。两个管家CAT构建体,在外显子1A上游分别有450和1400 bp,在HeLa细胞中表达水平相似,而包含外显子1B上游整个450 bp启动子区域的红系特异性构建体则不表达。相反,管家和红系构建体在K562细胞中均有表达。(摘要截短于250字)

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