Matsushita T, Tanimoto M, Yamamoto K, Sugiura I, Hamaguchi M, Takamatsu J, Kamiya T, Saito H
Department of Internal Medicine, Nagoya University School of Medicine, Japan.
J Lab Clin Med. 1990 Oct;116(4):492-7.
Three hemophilia B patients with anti-factor IX antibodies who had no detectable gross deletion of the factor IX gene by Southern blotting analysis were investigated at the molecular level. All eight exons, accompanied by their splicing junction sites and presumptive promoter regions of the factor IX gene in these patients (total 5.5 kb in length) were amplified with the use of the polymerase chain reaction, followed by complete nucleotide sequence analysis. Three different types of novel single base substitutions and a 2 base-pair nucleotide deletion were identified. Patient HB-5 had two point mutations in his factor IX gene. One was located at the promoter region at nucleotide -793 and the other (C-to-T transition) was found in exon VI of the gene changing Gln-191 to a stop codon. Patient HB-6 had a point mutation (G-to-A) in the splice acceptor site, which interrupted the normal splicing of the last intron G. A small two-nucleotide deletion in exon III was detected in patient HB-7 and yielded frameshifted amino acids and terminated by a stop codon. These resuslts suggest that not only the gross gene deletion of factor IX gene but also the point mutations or small nucleotide deletion that may cause the interruption of coding informations for mature protein synthesis is predisposed to development of anti-factor IX inhibitors in patients with hemophilia B.
对3例B型血友病患者进行了分子水平的研究,这些患者存在抗凝血因子IX抗体,Southern印迹分析未检测到凝血因子IX基因的明显大片段缺失。利用聚合酶链反应扩增了这些患者凝血因子IX基因的所有8个外显子及其剪接连接位点和假定的启动子区域(总长度为5.5 kb),随后进行了完整的核苷酸序列分析。鉴定出3种不同类型的新型单碱基替换和1个2碱基对的核苷酸缺失。患者HB - 5的凝血因子IX基因有两个点突变。一个位于启动子区域的核苷酸-793处,另一个(C到T的转换)在该基因的外显子VI中被发现,导致Gln - 191变为终止密码子。患者HB - 6在剪接受体位点有一个点突变(G到A),这中断了最后一个内含子G的正常剪接。在患者HB - 7的外显子III中检测到一个小的两核苷酸缺失,产生了移码氨基酸并由终止密码子终止。这些结果表明,不仅凝血因子IX基因的大片段缺失,而且可能导致成熟蛋白合成编码信息中断的点突变或小核苷酸缺失,都易使B型血友病患者产生抗凝血因子IX抑制剂。
