Haviland D L, Haviland J C, Fleischer D T, Wetsel R A
Department of Pediatrics, Washington University School of Medicine, St. Louis, Missouri 63110.
J Biol Chem. 1991 Jun 25;266(18):11818-25.
To understand fifth complement component (C5) gene regulation, splicing, and C5 protein deficiency at the molecular level, the organization of the murine C5 gene was determined. The C5 structural gene is present as a single copy in the mouse genome as demonstrated by Southern blot analysis. Accordingly, three cosmid clones were isolated from a genomic library that was prepared from mouse strain B10.D2/nSnJ. These clones overlapped and contained the structural gene encoding the complete C5 alpha-chain and 90% of the beta-chain. The 5'-flanking region of the C5 gene was obtained from a clone isolated from a genomic lambda-MOPC-41 library. Unique restriction fragments were prepared from the genomic clones and subcloned, and the exons were sequenced. All introns were sized by sequencing or Southern analysis. The C5 structural gene was found to be a highly interrupted gene of approximately 78 kilobases containing 42 exons and 41 introns. The exons ranged in length from 58 to 247 base pairs, with an average length of 131 base pairs. The introns ranged in size from 100 base pairs to 4 kilobases with an average length of 1.5 kilobases. The C5 alpha-chain was encoded by 49 kilobases containing 26 exons; the beta-chain was encoded by 29 kilobases containing 16 exons. The C5a coding sequence was split between two exons. All intron/exon junctions followed the normal consensus rule except at intron 35 in which the 5'-donor GT was substituted by GC. The 2-base-pair gene deletion and HindIII and PvuII restriction fragment length polymorphisms associated with murine C5 deficiency were localized to exon 7, exon 16, and intron 20, respectively. Comparison of the intron-exon junctions of the murine C5, human C3, and mouse C4 genes indicated that these genes are nearly identical in structural organization. However, the rat alpha 2-macroglobulin gene showed only moderate genomic organizational similarity to the murine C5 gene. A major and a minor transcriptional initiation site in the C5 gene were identified by primer extensions and confirmed by RNase protection assays. Sequence analysis of the 5'-flanking region (760 base pairs) revealed a TATA-like and CAAT box upstream of the major transcriptional initiation site at positions -274 and -303, respectively, suggesting an atypical promoter. The 5'-flanking region also contained sequences identical with several cis-acting motifs known to bind the liver-specific nuclear protein LF-A1 and the nuclear protein NF-kappa B.(ABSTRACT TRUNCATED AT 250 WORDS)
为了在分子水平上理解第五补体成分(C5)基因的调控、剪接以及C5蛋白缺陷,我们确定了小鼠C5基因的结构。Southern印迹分析表明,C5结构基因在小鼠基因组中以单拷贝形式存在。因此,我们从由B10.D2/nSnJ小鼠品系构建的基因组文库中分离出了三个黏粒克隆。这些克隆相互重叠,包含编码完整C5α链和90%β链的结构基因。C5基因的5'侧翼区域是从一个从基因组λ-MOPC-41文库中分离出的克隆获得的。从基因组克隆中制备了独特的限制性片段并进行亚克隆,然后对各外显子进行测序。所有内含子通过测序或Southern分析确定大小。发现C5结构基因是一个高度间断的基因,约78千碱基,包含42个外显子和41个内含子。外显子长度从58到247个碱基对不等,平均长度为131个碱基对。内含子大小从100个碱基对到4千碱基不等,平均长度为1.5千碱基。C5α链由49千碱基编码,包含26个外显子;β链由29千碱基编码,包含16个外显子。C5a编码序列分布在两个外显子之间。除了第35号内含子中5'供体GT被GC取代外,所有内含子/外显子连接均遵循正常的共有规则。与小鼠C5缺陷相关的2碱基对基因缺失以及HindIII和PvuII限制性片段长度多态性分别定位于第7外显子、第16外显子和第20内含子。对小鼠C5、人C3和小鼠C4基因的内含子-外显子连接进行比较表明,这些基因在结构组织上几乎相同。然而,大鼠α2-巨球蛋白基因与小鼠C5基因仅显示出中等程度的基因组组织相似性。通过引物延伸鉴定了C5基因中的一个主要转录起始位点和一个次要转录起始位点,并通过RNA酶保护试验得到证实。对5'侧翼区域(760个碱基对)的序列分析显示,在主要转录起始位点上游-274和-303位置分别有一个类似TATA盒和CAAT盒的序列,提示这是一个非典型启动子。5'侧翼区域还包含与几个已知能结合肝脏特异性核蛋白LF-A1和核蛋白NF-κB的顺式作用基序相同的序列。(摘要截短至250字)
