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作 者:刘建湘[1] 张宇舟[1] 王鸿利[1] 黄秋花[1] 曹文俊[1] 王学锋[1] 璩斌[1] 王辉东[1] 邵慧珍[1] 王振义[1] 陈竺[1] 黄薇[1]
机构地区:[1]上海第二医科大学附属瑞金医院,上海血液学研究所200025
出 处:《中华血液学杂志》1997年第9期464-467,共4页Chinese Journal of Hematology
基 金:国家自然科学基金!39470319;卫生部青年基金!95-2-46;上海血液学研究所胡应洲奖励基金
摘 要:目的:对血友病甲进行基因诊断。方法:采用多聚酶链反应(PCR),变性梯度凝胶电泳(DGGE)和DNA测序等方法对上海地区血友病甲基因突变进行检测。50例无内含子22倒位的血友病甲患者(其中重型24例,中型9例,轻型17例,无亲缘关系患者45例)先用PCR扩增基因组DNA,扩增范围包括所有外显子[编码B区的外显子14(氨基酸783~1598)部分除外,但包含凝血酶切割位点AA740和1689]及其侧翼内含子序列,然后对扩增片段进行DGGE分析,发现异常条带则进行DNA测序。结果:11例无亲缘关系患者中检出突变11种,其中无义突变5种,均为重型;错义突变5种,均为轻、中型;小缺失1例。其中,466Lys(AAG)-Thr(ACG),719Tyr(TAC)-Stop(TAG)及312Ile(ATC)-xxC为新发现的突变。结论:除内含子22倒位外,绝大部分血友病甲基因突变为单碱基置换导致的点突变。有亲缘关系的患者都有相同的基因突变。基因突变与临床表现基本相符。Objective:To detect gene mutations in hemophilia A in Shanghai. Methods:PCR,denatur ing gradient gel electrophoresis (DGGE) atd DNA sequencing were used. Fifty Chinese cases of hemophilia A without intron 22 inversion, including 24 severe, 9 moderate and 17 mild cases, were screened. Genomic DNA was amplified using GC-clamped primers covering all the exons and flanking in tron regions,excluding the middle portion of extron 14 encoding the B domain,but including the thrombin cleavage sites at AA740 and 1689. The amplified GC-clamped PCR fragments were then electrophoresed on DGGE. The abnormal bands were sequenced. Results: Eleven different mutations were identified, in cluding 5 nonsense mutations, 5 missense mutations and one small deletion. Among them, 3 mutations,466Lys (AAG )-Thr (ACG ), 719Tyr (TAC )-Stop (TAG ) and 312Ile (ATC )-xxC have not been reported be fore. Conclusion: Apart from intron 22 inversion,most gene mutations in hemophilia A were point mu tations resulted from single base substitution. Generally the genetic defects correspond to the c1inical man ifestations.
分 类 号:R554.1[医药卫生—血液循环系统疾病]
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