荧光定量PCR在中国汉族人群21三体综合征中的实际应用

Practical application of fluorescent quantitative PCR on Trisomy 21 in Chinese Han population.

作者信息

Sun Xiaobo, Yan Ming, Zhang Yuanzhen, Zhou Xin, Wang Chunhong, Zheng Fang, Xiong Chenling

机构信息

Center for Gene Diagnosis, Zhongnan Hospital of Wuhan University, Wuhan 430071, China.

出版信息

Mol Biol Rep. 2006 Sep;33(3):167-73. doi: 10.1007/s11033-006-0013-8.

DOI:10.1007/s11033-006-0013-8

PMID:16850185

Abstract

OBJECTIVE

To apply the fluorescent quantitative PCR method on the detection of Trisomy 21 by D21S11 locus and make a foundation for rapid prenatal diagnosis of Trisomy 21.

METHODS

About 409 controls (39 amniotic fluid samples and 370 peripheral blood samples) and 35 patients (4 amniotic fluid samples and 31 peripheral blood samples) with Trisomy 21 were tested using fluorescent quantitative PCR by amplification of DNA fragment on D21S11 STR locus. The results were compared with conventional cytogenetic analysis to confirm the utility of this method. And the allele frequency distributions of D21S11 STR locus were analyzed.

RESULTS

The 95% reference interval of fluorescent intensity ratios of peak heights of PCR products amplified from two alleles on D21S11 locus ranged from 0.84 to 1.42 (1.13 +/- 0.29) in heterozygous controls. About 19 out of 35 patients showed a "diallelic" pattern and their height ratio of fluorescent peaks of PCR products amplified from two alleles in patients with "diallelic" patterns were all outside of the 95% reference range of controls. The PCR products of DNA from 12 patients presented the third allele. No sample with the "monoallelic" pattern was found. Four chimeras diagnosed by cytogenetic method could not be diagnosed by this method. There were 17 and 11 alleles found in controls and patients, respectively. About 343 out of 409 controls were heterozygous and the heterozygosity was 83.86%. We did not find any significant differences in the frequency distributions of alleles on D21S11 locus between controls and patients. But there were significant differences in the frequency distributions of alleles on D21S11 locus between controls and patients. But there were significant differences in the frequency distributions of alleles on D21S11 locus among different populations.

CONCLUSIONS

The fluorescent quantitative polymerase chain reaction method was rapid, accurate, and only small amount of starting material was needed, it could be applied in rapid prenatal diagnosis of Trisomy 21. D21S11 was a good marker with high heterozygosity for the screening of Trisomy 21. And the frequency distributions of alleles on D21S11 locus were significantly related to ethnic background.

摘要

目的

应用荧光定量聚合酶链反应方法，通过检测D21S11基因座来诊断21三体综合征，为21三体综合征的快速产前诊断奠定基础。

方法

采用荧光定量聚合酶链反应，扩增D21S11 STR基因座上的DNA片段，检测约409例对照（39例羊水样本和370例外周血样本）以及35例21三体综合征患者（4例羊水样本和31例外周血样本）。将结果与传统细胞遗传学分析进行比较，以确定该方法的实用性。并分析D21S11 STR基因座的等位基因频率分布。

结果

在杂合子对照中，D21S11基因座上两个等位基因扩增的PCR产物峰高荧光强度比值的95%参考区间为0.84至1.42（1.13±0.29）。35例患者中约19例呈现“双等位基因”模式，“双等位基因”模式患者中两个等位基因扩增的PCR产物荧光峰高比值均超出对照的95%参考范围。12例患者的DNA的PCR产物出现第三个等位基因。未发现“单等位基因”模式的样本。4例经细胞遗传学方法诊断的嵌合体无法用该方法诊断。对照和患者中分别发现17个和11个等位基因。409例对照中约343例为杂合子，杂合度为83.86%。未发现对照和患者在D21S11基因座上等位基因频率分布有任何显著差异。但对照和患者在D21S11基因座上等位基因频率分布存在显著差异。不同人群在D21S11基因座上等位基因频率分布存在显著差异。