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新发现的碳酸酐酶CA VII的人类基因特征及其在16号染色体上的定位。

Characterization of the human gene for a newly discovered carbonic anhydrase, CA VII, and its localization to chromosome 16.

作者信息

Montgomery J C, Venta P J, Eddy R L, Fukushima Y S, Shows T B, Tashian R E

机构信息

Department of Human Genetics, University of Michigan Medical School, Ann Arbor 48109-0618.

出版信息

Genomics. 1991 Dec;11(4):835-48. doi: 10.1016/0888-7543(91)90006-z.

Abstract

Six carbonic anhydrase (CA) isozymes (CA I-VI) in mammals and other amniotes have been described. We have isolated an additional CA gene from a human genomic library and designated its putative product carbonic anhydrase VII (CA VII). The gene is approximately 10 kb long and contains seven exons and six introns found at positions identical to those determined for the previously described CA I, CA II, and CA III genes. The finding of a 17-bp GT-rich segment in a position 28 bp downstream of the poly(A)+ signal and the high correspondence of the 5' and 3' splice sites of the six introns with consensus junction sequences are consistent with the gene being functional. The 5' flanking regions of the CA VII gene do not contain the TATA and CAAT promoter elements usually found within 100 bp upstream of transcription initiation, but do contain a TTTAA sequence 102 nucleotides upstream of the initiation codon. The 5' region of the gene (-243 to +551) is GC-rich and contains 80 CpG dinucleotides and four possible Sp1 (GGGCGG or CCGCCC) binding sites. Northern analysis has identified the salivary gland as a major site of expression. The derived amino acid sequence of the CA VII gene is 263 amino acids long and has 50, 56, and 49% identity with human CA I, CA II, and CA III, respectively. No differences were found at any of the 39 positions that have remained invariant in all mammalian CA isozymes sequenced to date. Based on analysis of interspecific somatic cell hybrids, the human CA VII gene, CA7, was assigned to chromosome 16, with localization to the long arm at the q21-23 region by in situ hybridization. This is in contrast to the location of the CA I, CA II, and CA III gene cluster on human chromosome 8 and that of the human CA VI gene on chromosome 1.

摘要

哺乳动物和其他羊膜动物体内的六种碳酸酐酶(CA)同工酶(CA I - VI)已被描述。我们从人类基因组文库中分离出了另一个CA基因,并将其推定产物命名为碳酸酐酶VII(CA VII)。该基因长度约为10 kb,包含七个外显子和六个内含子,其位置与先前描述的CA I、CA II和CA III基因的位置相同。在多聚腺苷酸加尾信号下游28 bp处发现一个富含GT的17 bp片段,并且六个内含子的5'和3'剪接位点与共有连接序列高度一致,这表明该基因具有功能。CA VII基因的5'侧翼区域不包含通常在转录起始上游100 bp内发现的TATA和CAAT启动子元件,但在起始密码子上游102个核苷酸处含有一个TTTAA序列。该基因的5'区域(-243至+551)富含GC,包含80个CpG二核苷酸和四个可能的Sp1(GGGCGG或CCGCCC)结合位点。Northern分析确定唾液腺是主要表达位点。CA VII基因推导的氨基酸序列长263个氨基酸,与人类CA I、CA II和CA III的同一性分别为50%、56%和49%。在迄今为止测序的所有哺乳动物CA同工酶中保持不变的39个位置上均未发现差异。基于种间体细胞杂种分析,人类CA VII基因CA7被定位到16号染色体,通过原位杂交进一步定位到长臂的q21 - 23区域。这与人类染色体8上的CA I、CA II和CA III基因簇以及1号染色体上的人类CA VI基因的位置不同。

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