[采用靶向基因序列捕获及新一代测序技术诊断4例阿拉吉耶综合征患儿]

[Target gene sequence capture and next generation sequencing technology to diagnose four children with Alagille syndrome].

作者信息

Gao M L, Zhong X M, Ma X, Ning H J, Zhu D, Zou J Z

机构信息

Department of Gastroenterology, the Affiliated Hospital, Capital Institute of Pediatrics, Beijing 100020, China.

出版信息

Zhonghua Er Ke Za Zhi. 2016 Jun 2;54(6):441-5. doi: 10.3760/cma.j.issn.0578-1310.2016.06.011.

DOI:10.3760/cma.j.issn.0578-1310.2016.06.011

PMID:27256232

Abstract

OBJECTIVE

To make genetic diagnosis of Alagille syndrome (ALGS) patients using target gene sequence capture and next generation sequencing technology.

METHOD

Target gene sequence capture and next generation sequencing were used to detect ALGS gene of 4 patients. They were hospitalized at the Affiliated Hospital, Capital Institute of Pediatrics between January 2014 and December 2015, referred to clinical diagnosis of ALGS typical and atypical respectively in 2 cases. Blood samples were collected from patients and their parents and genomic DNA was extracted from lymphocytes. Target gene sequence capture and next generation sequencing was detected. Sanger sequencing was used to confirm the results of the patients and their parents.

RESULT

Cholestasis, heart defects, inverted triangular face and butterfly vertebrae were presented as main clinical features in 4 male patients. The first hospital visiting ages ranged from 3 months and 14 days to 3 years and 1 month. The age of onset ranged from 3 days to 42 days (median 23 days). According to the clinical diagnostic criteria of ALGS, patient 1 and patient 2 were considered as typical ALGS. The other 2 patients were considered as atypical ALGS. Four Jagged 1(JAG1) pathogenic mutations were detected. Three different missense mutations were detected in patient 1 to patient 3 with ALGS(c.839C>T(p.W280X), c. 703G>A(p.R235X), c. 1720C>T(p.V574M)). The JAG1 mutation of patient 3 was first reported. Patient 4 had one novel insertion mutation (c.1779_1780insA(p.Ile594AsnfsTer23)). Parental analysis verified that the JAG1 missense mutation of 3 patients were de novo. The results of sanger sequencing was consistent with the results of the next generation sequencing.

CONCLUSION

Target gene sequence capture combined with next generation sequencing can detect two pathogenic genes in ALGS and test genes of other related diseases in infantile cholestatic diseases simultaneously and presents a high throughput, high efficiency and low cost. It may provide molecular diagnosis and treatment for clinicians with good clinical application prospects.

摘要

目的

采用靶向基因序列捕获及二代测序技术对阿拉吉耶综合征（ALGS）患者进行基因诊断。

方法

采用靶向基因序列捕获及二代测序技术检测4例患者的ALGS基因。这4例患者于2014年1月至2015年12月在首都儿科研究所附属儿童医院住院，其中2例分别被临床诊断为典型和非典型ALGS。采集患者及其父母的血样，从淋巴细胞中提取基因组DNA。进行靶向基因序列捕获及二代测序检测。采用桑格测序法对患者及其父母的检测结果进行验证。

结果

4例男性患者的主要临床特征为胆汁淤积、心脏缺陷、倒三角形脸及蝴蝶椎。首次就诊年龄为3个月14天至3岁1个月。发病年龄为3天至42天（中位数23天）。根据ALGS的临床诊断标准，患者1和患者2被认为是典型ALGS。另外2例患者被认为是非典型ALGS。检测到4个锯齿状蛋白1（JAG1）致病突变。在1至3例ALGS患者中检测到3种不同的错义突变（c.839C>T(p.W280X)、c.703G>A(p.R235X)、c.1720C>T(p.V574M)）。患者3的JAG1突变首次报道。患者4有1个新的插入突变（c.1779_1780insA(p.Ile594AsnfsTer23)）。亲代分析证实3例患者的JAG1错义突变为新发突变。桑格测序结果与二代测序结果一致。