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一种新型人类羰基还原酶CBR3及核糖体假基因定位于人类染色体21q22.2

Mapping of a novel human carbonyl reductase, CBR3, and ribosomal pseudogenes to human chromosome 21q22.2.

作者信息

Watanabe K, Sugawara C, Ono A, Fukuzumi Y, Itakura S, Yamazaki M, Tashiro H, Osoegawa K, Soeda E, Nomura T

机构信息

Bioscience Research Laboratory, FUJIYA Co., Ltd., 228 Soya, Hadano, 257, Japan.

出版信息

Genomics. 1998 Aug 15;52(1):95-100. doi: 10.1006/geno.1998.5380.

Abstract

To find the genes contributing to Down syndrome, we constructed a 4-Mb sequence-ready map spanning chromosome 21q22.2 with megabase-sized cosmid/P1-derived artificial chromosome (PAC) contigs. The restriction map with rare cutting enzymes, followed by sequencing from the clustering sites, has defined CpG islands and revealed the genes associated with CpG islands (Accession No. D85771). Of these, two human carbonyl reductases (CBR; EC1.1.1.184) were found in a PAC 25P16 clone. CBR catalyzes the reduction of a large number of biologically and pharmacologically active carbonyl compounds to their corresponding alcohols and has been mapped in 21q22.1. To confirm these results, we sequenced the PAC clone in shotgun strategies and identified a novel carbonyl reductase, designated CBR3, 62 kb downstream from the original CBR. In addition, three ribosomal pseudogenes, L23a, S9, and L3, and some cDNAs with ESTs were mapped in the sequence. In conclusion, the sequence analysis for CpG islands predicted from the megabase-sized contigs will reveal and identify the genes involved in Down syndrome.

摘要

为了找到与唐氏综合征相关的基因,我们构建了一个覆盖21号染色体q22.2区域、大小为4兆碱基的序列就绪图谱,该图谱由兆碱基大小的黏粒/ P1衍生人工染色体(PAC)重叠群组成。用稀有切割酶构建的限制酶图谱,随后从聚类位点进行测序,确定了CpG岛,并揭示了与CpG岛相关的基因(登录号:D85771)。其中,在一个PAC 25P16克隆中发现了两种人类羰基还原酶(CBR;EC1.1.1.184)。CBR催化大量具有生物学和药理学活性的羰基化合物还原为相应的醇,并已定位在21q22.1区域。为了证实这些结果,我们采用鸟枪法对PAC克隆进行测序,并在原始CBR下游62 kb处鉴定出一个新的羰基还原酶,命名为CBR3。此外,还在该序列中定位了三个核糖体假基因L23a、S9和L3,以及一些带有EST的cDNA。总之,对从兆碱基大小的重叠群预测的CpG岛进行序列分析,将揭示和鉴定与唐氏综合征相关的基因。

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