摘要
目的:建立一种对性连锁遗传病胎儿进行产前性别诊断的方法。方法:采用聚合酶链式反应(PCR)扩增男性特异的SRY基因,扩增片段大小为422bp。结果:对不同标本的扩增表明,10例男性标本中均出现该特异扩增片段,而女性无此片段;20例羊水标本的扩增结果与其新生儿实际性别完全一致;47例绒毛标本中22例阳性,阴性/阳性之比为1∶1.136,接近实际的胎儿性别之比。同时进行了全血和羊水的直接PCR,在4μl至0.5μl血时可出现扩增带,羊水在2ml至0.5ml时也出现扩增带。结论:PCR特异扩增SRY基因片段。
Objective: To establish the method for prenatal sex diagnosis of the fetus carrying sexlinked genetic disorder. Method: Human SRY gene was amplified by polymerase chain reaction. A 422 bp male specific fragment was obtained. Results: The fragment was identified in 10 men, but unidentified in 10 women. The diagnostic accordance rate of 20 amniotic fluid samples was 100%. 22 of 47 chorionic villi samples were positive. The rate of positive/negative (22/25) was nearly the sex rate of newborn babies. In the meantime, directPCR amplification of blood and amniotic fluid was completed. The fragment was shown from 4 μl to 0.5 μl of blood and from 2 ml to 0.5 ml of amniotic fluid. Conclusion: The results show that fetal sex determination by PCR will be suitable for clinical prenatal diagnosis of sexlinked genetic disorders.
出处
《中华妇产科杂志》
CAS
CSCD
北大核心
1997年第11期652-654,共3页
Chinese Journal of Obstetrics and Gynecology
