Zhang Xiaoqing, Xu Yuejuan, Liu Deyuan, Geng Juan, Chen Sun, Jiang Zhengwen, Fu Qihua, Sun Kun
Department of Laboratory Medicine, Shanghai Children's Medical Center, Shanghai Jiao Tong University School of Medicine, Shanghai, 200127, Peoples Republic of China.
Department of Pediatric Cardiology, Xinhua Hospital, Shanghai Jiao Tong University School of Medicine, Shanghai, 200092, Peoples Republic of China.
BMC Genomics. 2015 May 8;16(1):364. doi: 10.1186/s12864-015-1590-5.
Copy number variations (CNVs) of chromosomal region 22q11.2 are associated with a subset of patients with congenital heart disease (CHD). Accurate and efficient detection of CNV is important for genetic analysis of CHD. The aim of the study was to introduce a novel approach named CNVplex®, a high-throughput analysis technique designed for efficient detection of chromosomal CNVs, and to explore the prevalence of sub-chromosomal imbalances in 22q11.2 loci in patients with CHD from a single institute.
We developed a novel technique, CNVplex®, for high-throughput detection of sub-chromosomal copy number aberrations. Modified from the multiplex ligation-dependent probe amplification (MLPA) method, it introduced a lengthening ligation system and four universal primer sets, which simplified the synthesis of probes and significantly improved the flexibility of the experiment. We used 110 samples, which were extensively characterized with chromosomal microarray analysis and MLPA, to validate the performance of the newly developed method. Furthermore, CNVplex® was used to screen for sub-chromosomal imbalances in 22q11.2 loci in 818 CHD patients consecutively enrolled from Shanghai Children's Medical Center. In the methodology development phase, CNVplex® detected all copy number aberrations that were previously identified with both chromosomal microarray analysis and MLPA, demonstrating 100% sensitivity and specificity. In the validation phase, 22q11.2 deletion and 22q11.2 duplication were detected in 39 and 1 of 818 patients with CHD by CNVplex®, respectively. Our data demonstrated that the frequency of 22q11.2 deletion varied among sub-groups of CHD patients. Notably, 22q11.2 deletion was more commonly observed in cases with conotruncal defect (CTD) than in cases with non-CTD (P<0.001). With higher resolution and more probes against selected chromosomal loci, CNVplex® also identified several individuals with small CNVs and alterations in other chromosomes.
CNVplex® is sensitive and specific in its detection of CNVs, and it is an alternative to MLPA for batch screening of pathogenetic CNVs in known genomic loci.
染色体22q11.2区域的拷贝数变异(CNV)与一部分先天性心脏病(CHD)患者相关。准确且高效地检测CNV对于CHD的遗传分析很重要。本研究的目的是引入一种名为CNVplex®的新方法,这是一种为高效检测染色体CNV而设计的高通量分析技术,并探索来自单一机构的CHD患者中22q11.2位点亚染色体失衡的患病率。
我们开发了一种名为CNVplex®的新技术,用于高通量检测亚染色体拷贝数畸变。它是对多重连接依赖探针扩增(MLPA)方法的改进,引入了延长连接系统和四组通用引物,简化了探针合成并显著提高了实验的灵活性。我们使用了110个样本,这些样本通过染色体微阵列分析和MLPA进行了广泛表征,以验证新开发方法的性能。此外,CNVplex®用于筛查连续从上海儿童医学中心招募的818例CHD患者中22q11.2位点的亚染色体失衡。在方法开发阶段,CNVplex®检测到了所有先前通过染色体微阵列分析和MLPA鉴定出的拷贝数畸变,显示出100%的敏感性和特异性。在验证阶段,通过CNVplex®在818例CHD患者中分别检测到39例22q11.2缺失和1例22q11.2重复。我们的数据表明,22q11.2缺失的频率在CHD患者亚组中有所不同。值得注意的是,22q11.2缺失在圆锥动脉干缺损(CTD)病例中比在非CTD病例中更常见(P<0.001)。由于具有更高的分辨率和针对选定染色体位点的更多探针,CNVplex®还鉴定出了几个具有小CNV和其他染色体改变的个体。
CNVplex®在检测CNV方面具有敏感性和特异性,并且是用于批量筛查已知基因组位点致病CNV的MLPA替代方法。
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