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二氢蝶啶还原酶缺乏症的分子分析:日本患者中两个新突变的鉴定

Molecular analysis of dihydropteridine reductase deficiency: identification of two novel mutations in Japanese patients.

作者信息

Ikeda H, Matsubara Y, Mikami H, Kure S, Owada M, Gough T, Smooker P M, Dobbs M, Dahl H H, Cotton R G, Narisawa K

机构信息

Department of Biochemical Genetics, Tohoku University School of Medicine, Sendai, Japan.

出版信息

Hum Genet. 1997 Oct;100(5-6):637-42. doi: 10.1007/s004390050566.

Abstract

Mutations in the dihydropteridine reductase (DHPR) gene result in hyperphenylalaninaemia and deficiency of various neurotransmitters in the central nervous system, causing severe neurological symptoms. We studied two Japanese patients with DHPR deficiency and identified a missense and a splicing error mutation, respectively. A homozygous missense mutation (tryptophan36-to-arginine) was detected in patient 1. The mutation abolished DHPR activity according to in vitro expression studies. The DHPR mRNA in patient 2 was markedly decreased. Reverse transcription-polymerase chain reaction of the mRNA generated a cDNA fragment with a 152-bp insertion. The inserted sequence contained a termination codon, which was likely to affect the stability of the mRNA. Analysis of genomic DNA showed that the insertion was derived from putative intron 3 of the DHPR gene, and an intronic A-to-G substitution was present adjacent to the 3'-end of the inserted sequence. The nucleotide change generated a sequence similar to an RNA splice donor site and probably activated an upstream cryptic acceptor site, thus producing an abnormal extra exon.

摘要

二氢蝶啶还原酶(DHPR)基因突变会导致高苯丙氨酸血症以及中枢神经系统中多种神经递质缺乏,从而引发严重的神经症状。我们研究了两名患有DHPR缺乏症的日本患者,分别鉴定出一个错义突变和一个剪接错误突变。在患者1中检测到一个纯合错义突变(色氨酸36突变为精氨酸)。根据体外表达研究,该突变消除了DHPR活性。患者2的DHPR mRNA明显减少。对该mRNA进行逆转录-聚合酶链反应产生了一个插入了152 bp的cDNA片段。插入的序列包含一个终止密码子,这可能会影响mRNA的稳定性。基因组DNA分析表明,该插入片段源自DHPR基因的推定内含子3,并且在插入序列的3'端相邻处存在一个内含子A到G的替换。核苷酸变化产生了一个类似于RNA剪接供体位点的序列,并可能激活了上游的隐蔽受体位点,从而产生了一个异常的额外外显子。

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