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作 者:周海燕[1] 王新[2] 易宇凌[3] 邹永华[1] 欧阳曙明[1] 倪斌[1]
机构地区:[1]湖南省计划生育研究所湖南省现代优生技术重点实验室,长沙410008 [2]中南大学湘雅二医院妇产科,长沙410011 [3]湖南省妇幼保健院妇产科,长沙410008
出 处:《中国优生与遗传杂志》2011年第11期16-18,共3页Chinese Journal of Birth Health & Heredity
摘 要:目的为了建立一种在先天性心脏病(congenital heart disease,CHD)患者中快速、有效检测染色体22q11微缺失检测方法。方法从22q11区域内选取5个短串联重复多态位点(STRs)(D22S941、D22S944、D22S264、D22S311、D22S306),应用PCR扩增方法对20例CHD患者及其父母进行22q11微缺失筛查。结果发现4例CHD患者可能存在22q11微缺失。对筛查出可疑阳性病例再运用荧光标记PCR-STR分型方法进行诊断,结果有1例确诊为D22S941缺失。结论此项研究表明普通PCR方法只能作为22q11微缺失筛查的一种手段,荧光标记PCR-STR分型由于准确、高效,可以作为22q11微缺失确诊方法。Objective: To develop a rapid, economical and efficient approach for molecular detection of 22q11.2 microdeletion in patients with congenital heart diseases (CHD). Methods: Five repeat markers (D22S941, D22S944, D22S264, D22S311, D22S306) located in the proximal region of chromosome 22ql 1 were selected in this study. Twenty patients with congenital heart disease and their unaffected parents were analysized by using PCR method to screen 22ql 1 microdeletion. Results: Four cases may have the deletion at chromosome 22q11. The deletions were confirmed further by fluorescence labeling PCR and one patient had the 22ql 1 deletion. Conclusion: This study demonstrated that genotying of STR markers was a useful means of screening 22ql1 microdeletion for its easy experimental procedures, cost effectiveness, while fluorescence labeling PCR - STR typing method can be used in this microdeletion diagnosis, because that it was accurate and effective.
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