Gonzalez-Redondo J M, Stoming T A, Lanclos K D, Gu Y C, Kutlar A, Kutlar F, Nakatsuji T, Deng B, Han I S, McKie V C
Department of Cell and Molecular Biology, Medical College of Georgia, Augusta 30912-2100.
Blood. 1988 Sep;72(3):1007-14.
The presence of various substitutions and deletions resulting in beta-thalassemia was studied in 19 black patients with homozygous beta-thalassemia and in numerous relatives; all patients were from Georgia, South Carolina, and Alabama. Methodology included gene mapping, amplification of genomic DNA with Taq polymerase, identification of known nucleotide substitutions or a single nucleotide deletion through hybridization with synthetic oligonucleotides, cloning and sequencing of a beta-globin gene, and sequencing of amplified genomic DNA. Of the 38 chromosomes tested, 21 (55%) had the A----G substitution at nt -29, eight (21%) had the C----T substitution at nt -88, three (8%) had the substitution at codon 24, while one each of the following abnormalities were also detected: frameshift at codon 6, a C----A mutation at nt 848 of the beta IVS-II (new), an A----T mutation at codon 61 (new), a deletion of 1.35 kilobases including the 5' end of beta, a Ggamma(Agamma delta beta)(0)-thalassemia, and one thalassemia determinant that remained unidentified. The C----A mutation at nt 848 of IVS-II occurred at a position 3 nucleotides 5' to the third exon, adjacent to the invariant AG dinucleotide of the acceptor sequence. The A----T mutation in codon 61 (AAG----TAG) resulted in the creation of a stop codon and thus in beta(0)-thalassemia. The various mutations occurred on chromosomes with different haplotypes; however, chromosomes with a specific mutation but with different haplotypes belonged to one specific framework, which suggested that crossovers were responsible for these different types. Hemoglobin (Hb) F levels were generally high (55% to 75% with 98.5% in one patient with beta(0)/beta(0)); a few patients with specific haplotypes and an alpha-thalassemia-2 heterozygosity had a lower Hb F level. The Ggamma in the Hb F was consistently high when the C----T mutation occurred at nt -158 to the Cap site of the Ggamma-globin gene; seven patients with +/+ at this site had an average Ggamma of 73.8%, eight patients with +/- had 64.8%, and one patient with -/- had 34.2%. Variations in hematologic values and in Hb F, Ggamma, and Hb A2 levels of relatives with a beta-thalassemia heterozygosity depended to some extent on the types of mutations or deletions and on the haplotypes of the chromosomes with the beta-thalassemia determinant.
对19例纯合β地中海贫血黑人患者及其众多亲属中导致β地中海贫血的各种替换和缺失情况进行了研究;所有患者均来自佐治亚州、南卡罗来纳州和阿拉巴马州。方法包括基因定位、用Taq聚合酶扩增基因组DNA、通过与合成寡核苷酸杂交鉴定已知的核苷酸替换或单个核苷酸缺失、β珠蛋白基因的克隆和测序以及扩增的基因组DNA测序。在检测的38条染色体中,21条(55%)在核苷酸-29处有A→G替换,8条(21%)在核苷酸-88处有C→T替换,3条(8%)在密码子24处有替换,同时还检测到以下异常各1例:密码子6处的移码、βIVS-II的核苷酸848处的C→A突变(新发现)、密码子61处的A→T突变(新发现)、包括β的5'端在内的1.35千碱基的缺失、Gγ(Agγδβ)(0) -地中海贫血以及一个未鉴定的地中海贫血决定因素。IVS-II的核苷酸848处的C→A突变发生在距第三个外显子5'端3个核苷酸的位置,与受体序列的不变AG二核苷酸相邻。密码子61处的A→T突变(AAG→TAG)导致产生一个终止密码子,从而导致β(0) -地中海贫血。各种突变发生在具有不同单倍型的染色体上;然而,具有特定突变但单倍型不同的染色体属于一个特定的框架,这表明交叉互换是这些不同类型的原因。血红蛋白(Hb)F水平通常较高(55%至75%,一名β(0)/β(0)患者中为98.5%);少数具有特定单倍型和α地中海贫血-2杂合性的患者Hb F水平较低。当Gγ珠蛋白基因的Cap位点核苷酸-158处发生C→T突变时,Hb F中的Gγ始终较高;该位点为+/+的7名患者的平均Gγ为73.8%,+/-的8名患者为64.8%,-/-的1名患者为34.2%。具有β地中海贫血杂合性的亲属的血液学值以及Hb F、Gγ和Hb A2水平的变化在一定程度上取决于突变或缺失的类型以及带有β地中海贫血决定因素的染色体的单倍型。
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