Arredondo-Vega F X, Santisteban I, Kelly S, Schlossman C M, Umetsu D T, Hershfield M S
Department of Medicine, Duke University Medical Center, Durham, NC 27710.
Am J Hum Genet. 1994 May;54(5):820-30.
Adenosine deaminase (ADA) deficiency usually causes severe combined immune deficiency in infancy. Milder phenotypes, with delayed or late onset and gradual decline in immune function, also occur and are associated with less severely impaired deoxyadenosine (dAdo) catabolism. We have characterized the mutations responsible for ADA deficiency in siblings with striking disparity in clinical phenotype. Erythrocyte dAdo nucleotide pool size, which reflects total residual ADA activity, was lower in the older, more mildly affected sib (RG) than in her younger, more severely affected sister (EG). Cultured T cells, fibroblasts, and B lymphoblasts of RG had detectable residual ADA activity, while cells of EG did not. ADA mRNA was undetectable by northern analysis in these cells of both patients. Both sibs were found to be compound heterozygotes for the following novel splicing defects: (1) a G+1-->A substitution at the 5' splice site of IVS 2 and (2) a complex 17-bp rearrangement of the 3' splice site of IVS 8, which inserted a run of seven purines into the polypyrimidine tract and altered the reading frame of exon 9. PCR-amplified ADA cDNA clones with premature translation stop codons arising from aberrant pre-mRNA splicing were identified, which were consistent with these mutations. However, some cDNA clones from T cells of both patients and from fibroblasts and Epstein-Barr virus (EBV)-transformed B cells of RG, were normally spliced at both the exon 2/3 and exon 8/9 junctions. A normal coding sequence was documented for clones from both sibs. The normal cDNA clones did not appear to arise from either contamination or PCR artifact, and mosaicism seems unlikely to have been involved. These findings suggest (1) that a low level of normal pre-mRNA splicing may occur despite mutation of the invariant first nucleotide of the 5' splice donor sequence and (2) that differences in efficiency of such splicing may account for the difference in residual ADA activity, immune dysfunction, and clinical severity in these siblings.
腺苷脱氨酶(ADA)缺乏通常在婴儿期导致严重联合免疫缺陷。也会出现较轻的表型,免疫功能延迟或较晚出现并逐渐下降,这与脱氧腺苷(dAdo)分解代谢受损程度较轻有关。我们对临床表型差异显著的同胞中导致ADA缺乏的突变进行了特征分析。反映总残余ADA活性的红细胞dAdo核苷酸池大小,在年龄较大、受影响较轻的同胞(RG)中低于其年龄较小、受影响较重的妹妹(EG)。RG的培养T细胞、成纤维细胞和B淋巴母细胞具有可检测到的残余ADA活性,而EG的细胞则没有。通过Northern分析在两名患者的这些细胞中均未检测到ADA mRNA。发现两名同胞均为以下新型剪接缺陷的复合杂合子:(1)IVS 2的5'剪接位点处G+1→A替换,以及(2)IVS 8的3'剪接位点处17 bp的复杂重排,该重排将一串七个嘌呤插入多嘧啶序列并改变了外显子9的阅读框。鉴定出由异常前体mRNA剪接产生的带有过早翻译终止密码子的PCR扩增ADA cDNA克隆,这与这些突变一致。然而,来自两名患者T细胞以及RG的成纤维细胞和爱泼斯坦-巴尔病毒(EBV)转化B细胞的一些cDNA克隆,在2/3外显子和8/9外显子连接处均正常剪接。记录了来自两名同胞的克隆的正常编码序列。正常cDNA克隆似乎既不是由污染也不是由PCR假象产生的,并且似乎不太可能涉及镶嵌现象。这些发现表明:(1)尽管5'剪接供体序列的不变第一个核苷酸发生突变,但可能仍会发生低水平的正常前体mRNA剪接;(2)这种剪接效率的差异可能解释了这些同胞中残余ADA活性、免疫功能障碍和临床严重程度的差异。
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