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[46,XX性发育障碍的SRY阴性男性发病机制的探索]

[Exploration of the pathogenesis for a SRY-negative male with 46,XX disorder of sex development].

作者信息

Liu Ailing, Zhang Lanxue, Xu Hongyan, Chong Baoqiang, Liu Xiaxia, Li Lin

机构信息

Department of Genetics Testing, Linyi People's Hospital, Linyi, Shandong 276003, China.

出版信息

Zhonghua Yi Xue Yi Chuan Xue Za Zhi. 2020 Dec 10;37(12):1403-1406. doi: 10.3760/cma.j.cn511374-20191029-00548.

Abstract

OBJECTIVE

To explore the pathogenesis for a SRY-negative male with 46,XX disorder of sex development (DSD).

METHODS

Peripheral blood samples of the patient and his family members were subjected to chromosomal karyotyping, routine PCR, real-time fluorescence quantitative PCR, whole exome sequencing and whole genome sequencing. The data was analyzed with NextGENe software.

RESULTS

Both the proband and his brother presented a 46,XX karyotype with negative SRY gene, while their father presented normal phenotype and karyotype with positive SRY gene. No pathogenic variant associated with sex development was detected by whole exome sequencing, while a 243 kb duplication was detected by whole genome sequencing in the 5' upstream region of the SOX9 gene in the proband, his brother and father. The same duplication was not found in his sister and mother.

CONCLUSION

The 243 kb duplication at the 5' upstream of the SOX9 gene may predispose to the 46,XX DSD in this family. It is speculated that there exist an unknown core regulatory element in the upstream of the SOX9, and its duplication may trigger expression of SOX9 and initiate testicular differentiation in the absence of SRY gene.

摘要

目的

探讨一名46,XX性发育障碍(DSD)的SRY阴性男性的发病机制。

方法

对患者及其家庭成员的外周血样本进行染色体核型分析、常规PCR、实时荧光定量PCR、全外显子组测序和全基因组测序。数据用NextGENe软件进行分析。

结果

先证者及其兄弟呈现46,XX核型且SRY基因阴性,而他们的父亲表现为正常表型和核型且SRY基因阳性。全外显子组测序未检测到与性发育相关的致病变异,而在全基因组测序中,先证者、其兄弟和父亲的SOX9基因5'上游区域检测到一个243 kb的重复。在其姐妹和母亲中未发现相同的重复。

结论

SOX9基因5'上游的243 kb重复可能是该家族46,XX DSD的易感因素。推测在SOX9上游存在一个未知的核心调控元件,其重复可能在无SRY基因的情况下触发SOX9的表达并启动睾丸分化。

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