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开发一种全面的实时 PCR 检测方法,用于肌营养不良基因分析和中国家庭的产前诊断。

Development of a comprehensive real-time PCR assay for dystrophin gene analysis and prenatal diagnosis of Chinese families.

机构信息

Department of Genetics, School of Medicine, Zhejiang University, 866 Yuhangtang Road, Hangzhou, China.

出版信息

Clin Chim Acta. 2013 Sep 23;424:33-8. doi: 10.1016/j.cca.2013.05.006. Epub 2013 May 13.

Abstract

BACKGROUND

To develop a comprehensive method to analyze deletions or duplications of the dystrophin gene in both patients and carriers of Duchenne muscular dystrophy (DMD), likewise applied to prenatal diagnosis.

METHODS

A total of thirty Chinese families were recruited, composed of 29 DMD affected males and 38 female relatives containing four pregnant women. Deletions were previously screened by multiplex PCR. A comprehensive real-time PCR assay using SYBR Green I dye was performed for the initial detection of duplications in patients with a seven-exon primer set, carrier detection for female relatives and prenatal diagnosis for the 4 of them. The results were later confirmed by multiple ligation-dependent probe amplification (MLPA) and linkage analysis.

RESULTS

Three out of 4 duplications were first discovered by real-time PCR. Carrier status was ascertained in 22 and rejected in the remaining sixteen female relatives. Furthermore, 4 fetuses were diagnosed as two normal females, one normal male and one female carrier, respectively.

CONCLUSIONS

Our real-time PCR assay is useful in duplication screen with a detection rate of >70%, as well as rapid and reliable in both carrier detection and prenatal diagnosis of DMD families with known deletions and duplications.

摘要

背景

为了开发一种全面的方法来分析杜兴氏肌营养不良症(DMD)患者和携带者的肌营养不良蛋白基因缺失或重复,同样适用于产前诊断。

方法

共招募了 30 个中国家庭,包括 29 名 DMD 受累男性和 38 名女性亲属,其中包括 4 名孕妇。缺失先前通过多重 PCR 进行筛选。使用 SYBR Green I 染料的综合实时 PCR 检测对 7 个外显子引物组的患者进行初步的重复检测,对女性亲属进行携带者检测,对其中的 4 人进行产前诊断。结果随后通过多重连接依赖性探针扩增(MLPA)和连锁分析进行确认。

结果

实时 PCR 首次发现了 4 个重复中的 3 个。22 名女性亲属被确定为携带者状态,其余 16 名被拒绝。此外,4 个胎儿分别被诊断为 2 个正常女性、1 个正常男性和 1 个女性携带者。

结论

我们的实时 PCR 检测方法在重复检测中具有>70%的检出率,并且在已知缺失和重复的 DMD 家庭的携带者检测和产前诊断中快速可靠。

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