Copy number variation sequencing for diagnosis of cytomegalovirus infection based low-depth whole-genome sequencing technology in fetus:Three cases and literature review

Objective:To summarize the application value of copy number variant sequencing(CNV-seq)in the detection of fetal chromosome and cytomegalovirus load.Methods:The study analyzed the clinical basic data,relevant laboratory tests,treatment process,and outcomes of three patients with positive cytomegalovirus load detected by CNV-seq for fetal chromosomes and cytomegalovirus load,and literature review was done simutaneoubly.Results:In all three cases,the amniotic fluid cytomegalovirus load was less than 105 Copies/ml,and there were no significant neurological abnormalities observed during pregnancy or postpartum follow-up.There is no literature review on the application of CNV-seq technology in the detection of cytomegalovirus infection,only literature reports on genome analysis of CMV-DNA in confirmed patients were available.Conclusion:CNV-seq can be used to detect cytomegalovirus load,which may have a certain degree of predictive value for fetal outcome.CNV-seq can simultaneously detect fetal chromosomes and pathogenic microorganisms,which is of great significance for the prevention and control of birth defects.

CNV analysis of Meishan pig by nextgeneration sequencing and effects of AHR gene CNV on pig reproductive traits

Background:Reproductive performance of livestock is an economically important aspect of global food production.The Chinese Meishan pig is a prolific breed,with an average of three to five more piglets per litter than European breeds;however,the genetic basis for this difference is not well understood.Results:In this study,we investigated copy number variations(CNVs)of 32 Meishan pigs and 29 Duroc pigs by nextgeneration sequencing.A genome-wide analysis of 61 pigs revealed 12,668 copy number variable regions(CNVRs)that were further divided into three categories based on copy number(CN)of the whole population,i.e.,gain(n=7,638),and loss(n=5,030)CNVRs.We then compared Meishan and Duroc pigs and identified 17.17Mb of 6,387 CNVRs that only existing in Meishan pigs CNVRs that overlapped the reproduction-related gene encoding the aryl hydrocarbon receptor(AHR)gene.We found that normal AHR CN was more frequent than CN loss in four different pig breeds.An association analysis showed that AHR CN had a positive effect on litter size(P<0.05)and that a higher CN was associated with higher total number born(P<0.05),number born alive(P<0.05),number of weaned piglets,and birth weight.Conclusions:The present study provides comprehensive CNVRs for Meishan and Duroc pigs through large-scale population resequencing.Our results provide a supplement for the high-resolution map of copy number variation in the porcine genome and valuable information for the investigation of genomic structural variation underlying traits of interest in pig.In addition,the association results provide evidence for AHR as a candidate gene associated with reproductive traits that can be used as a genetic marker in pig breeding programs.

De novel heterozygous copy number deletion on 7q31.31-7q31.32 involving TSPAN12 gene with familial exudative vitreoretinopathy in a Chinese family

AIM:To investigate the genetic and clinical characteristics of patients with a large heterozygous copy number deletion on 7q31.31-7q31.32.METHODS:A family with familial exudative vitreoretinopathy(FEVR)phenotype was included in the study.Whole-exome sequencing(WES)was initially used to locate copy number variations(CNVs)on 7q31.31-31.32,but failed to detect the precise breakpoint.The long-read sequencing,Oxford Nanopore sequencing Technology(ONT)was used to get the accurate breakpoint which is verified by quantitative real-time polymerase chain reaction(QPCR)and Sanger Sequencing.RESULTS:The proband,along with her father and younger brother,were found to have a heterozygous 4.5 Mb CNV deletion located on 7q31.31-31.32,which included the FEVRrelated gene TSPAN12.The specific deletion was confirmed as del(7)(q31.31q31.32)chr7:g.119451239_123956818del.The proband exhibited a phase 2A FEVR phenotype,characterized by a falciform retinal fold,macular dragging,and peripheral neovascularization with leaking of fluorescence.These symptoms led to a significant decrease in visual acuity in both eyes.On the other hand,the affected father and younger brother showed a milder phenotype.CONCLUSION:The heterozygous CNV deletion located on 7q31.31-7q31.32 is associated with the FEVR phenotype.The use of long-read sequencing techniques is essential for accurate molecular diagnosis of genetic disorders.

Further analyses of variation of ribosome DNA copy number and polymorphism in ciliates provide insights relevant to studies of both molecular ecology and phylogeny

Sequence-based approaches, such as analyses of ribosome DNA(rDNA) clone libraries and high-throughput amplicon sequencing, have been used extensively to infer evolutionary relationships and elucidate the biodiversity in microbial communities.However, recent studies demonstrate both r DNA copy number variation and intra-individual(intra-genomic) sequence variation in many organisms, which challenges the application of the rDNA-based surveys. In ciliates, an ecologically important clade of microbial eukaryotes, rDNA copy number and sequence variation are rarely studied. In the present study, we estimate the intraindividual small subunit rDNA(SSU r DNA) copy number and sequence variation in a wide range of taxa covering nine classes and 18 orders of the phylum Ciliophora. Our studies reveal that:(i) intra-individual sequence variation of SSU rDNA is ubiquitous in all groups of ciliates detected and the polymorphic level varies among taxa;(ii) there is a most common version of SSU rDNA sequence in each cell that is highly predominant and may represent the germline micronuclear template;(iii)compared with the most common version, other variant sequences differ in only 1–3 nucleotides, likely generated during macronuclear(somatic) amplification;(iv) the intra-cell sequence variation is unlikely to impact phylogenetic analyses;(v) the rDNA copy number in ciliates is highly variable, ranging from 103 to 106, with the highest record in Stentor roeselii. Overall,these analyses indicate the need for careful consideration of SSU r DNAvariation in analyses of the role of ciliates in ecosystems.

Copy number variation profile-based genomic typing of premenstrual dysphoric disorder in Chinese

Premenstrual dysphoric disorder(PMDD) affects nearly 5% of women of reproductive age. Symptomatic heterogeneity, together with largely unknown genetics, has greatly hindered its effective treatment. In the present study, analysis of genomic sequencing-based copy number variations(CNVs) called from 100 kb white blood cell DNA sequence windows by means of semisupervized clustering led to the segregation of patient genomes into the D and V groups, which correlated with the depression and invasion clinical types,respectively, with 89.0% consistency. Application of diagnostic CNV features selected using the correlation-based machine learning method enabled the classification of the CNVs obtained into the D group, V group, total patient group, and control group with an average accuracy of 83.0%. The power of the diagnostic CNV features was 0.98 on average, suggesting that these CNV features could be used for the molecular diagnosis of the major clinical types of PMDD. This demonstrated concordance between the CNV profiles and clinical types of PMDD supported the validity of symptom-based diagnosis of PMDD for differentiating between its two major clinical types, as well as the predominantly genetic nature of PMDD with a host of overlaps between multiple susceptibility genes/pathways and the diagnostic CNV features as indicators of involvement in PMDD etiology.

884例性染色体异常胎儿产前诊断结果分析

目的 对884例无创产前筛查(NIPS)提示性染色体异常的羊水样本进行核型分析、荧光原位杂交技术(FISH)和拷贝数变异测序(CNV-seq)检测,探讨不同方法在产前诊断中的价值。方法 选取2015年1月—2022年12月天津市中心妇产科医院孕早期NIPS提示胎儿为性染色体异常的孕妇884例,于孕中期采集羊水样本,进行羊水细胞核型分析和FISH检测,对结果不一致或培养失败的样本进一步行CNV-seq检测。结果 884例孕妇中,有341例(38.6%)检出异常核型,11例(1.2%)羊水细胞培养失败。NIPS性染色体阳性预测值为39.2%(341/873)。341例核型分析异常样本中,最常见的核型异常类型是47,XXY(108例),其次为47,XXX(80例)、47,XYY(68例)、45,X(18例),共检出51例嵌合体。884例孕妇中,有862例FISH检测结果与核型分析或CNV-seq结果一致,FISH的阳性预测值为97.5%;24例与核型分析结果不一致,进一步行CNV-seq检测,有22例CNV-seq结果与核型分析结果一致,并能相互补充分析;2例不一致样本中,1例核型分析结果为46,~+mar,FISH和CNV-seq结果均为45,X;1例核型分析结果为嵌合Y染色体异染色质区缺失,FISH和CNV-seq结果均为嵌合体,结构未见异常。结论 NIPS提示性染色体异常时,建议首选FISH和核型分析联合检测,可快速、准确地诊断染色体异常。对于疑似染色体特殊结构异常,建议进行FISH、核型分析和CNV-seq联合检测,可明确遗传学病因。

101例胎儿性染色体非整倍体异常核型分布特征及妊娠结局分析

目的分析101例胎儿性染色体非整倍体(sex chromosome aneuploidy,SCA)异常核型分布特征及妊娠结局。方法回顾性收集2016年1月~2021年12月7821例于广西壮族自治区人民医院成功进行产前核型诊断孕妇的临床资料,均行细胞培养染色体核型分析与拷贝数变异测序(copy number variation sequencing,CNV-seq)检测,对检出的101例SCA异常胎儿病历进行分析。结果SCA共检出101例,检出率为1.29%。其中克氏综合征占比33.66%,超雌综合征占比17.82%,超雄综合征占比12.87%,特纳综合征占比10.89%,其他非整倍体异常(包括:48,XXXY 1例,69,XXY[80%]/68,XXY,-22[20%]1例)占比1.98%,嵌合体占比22.77%。101例SCA产前指征结果为:年龄≥35周岁占比53.47%(54/101),血清生化指标筛查高/临界风险占比4.95%(5/101),胎儿超声检测异常占比17.82%(18/101),无创产前基因检测(non-invasive prenatal testing,NIPT)异常占比51.49%(52/101),不良孕产史占比12.87%(13/101),其他原因(孕妇脑瘫1例、双方珠蛋白生成障碍性贫血4例)5例行产前诊断,占比4.95%(5/101),部分病例并发多项产前诊断指征。23例诊断为性染色体嵌合体的胎儿,其中有22例通过核型与CNV-seq双向验证,11例孕妇选择终止妊娠,其余选择继续妊娠。结论产前核型诊断联合血清学检测、孕期超声等不同产前筛查手段,有利于提高SCA检出率。而CNV-seq可对性染色体嵌合体孕妇的遗传咨询提供更多临床依据。

全外显子测序联合基因组拷贝数变异测序在儿科遗传病诊断中的应用

目的探讨全外显子测序(whole exome sequencing,WES)联合基因组拷贝数变异测序(copy number variation sequencing,CNVseq)在儿科遗传病诊断中的应用价值。方法选取2019年8月至2023年7月郑州市妇幼保健院新生儿科及儿科收治的怀疑患有遗传性疾病或临床诊断不明确的患儿为研究对象,采集患儿及其父母外周血进行WES及CNVseq检测,对检出的变异进行分类及评级,并进行一代测序或qPCR验证。结果共纳入患儿33例,其中男性18例,女性15例,年龄范围为1 d~8岁。WES的阳性检出率为36.4%(12/33),CNVseq阳性检出率为9.1%(3/33),两者联合阳性检出率为45.5%(15/33)。结论WES联合CNVseq是儿童遗传性疾病分子诊断的有力工具,可作为一线检测手段在临床大力推广。

高龄孕妇产前诊断胎儿染色体异常结果特征分析

目的分析高龄孕妇介入性产前诊断胎儿染色体异常结果的特征。方法回顾性选取2020年1月至2023年6月于唐山市妇幼保健院产前诊断遗传病诊断中心就诊的行羊膜腔穿刺术的638例高龄孕妇作为研究对象,按照孕妇预产年龄分为A组(35~<40岁,n=463)和B组(≥40岁,n=175),统计2组高龄孕妇羊水细胞染色体核型分析结果和全基因组拷贝数变异测序(copy number variation sequencing,CNV-seq)检测结果。统计学方法采用χ^(2)检验。结果638例高龄孕妇中,羊水细胞染色体异常核型检出率为8.3%(53/638),其中A组和B组的检出率分别为6.9%(32/463)和12.0%(21/175),B组高于A组(χ^(2)=15.241,P<0.05)。CNV-seq检测结果显示,羊水细胞染色体异常拷贝数变异(copy number variation,CNV)检出率为10.2%(65/638),其中A组和B组的检出率分别为8.9%(41/463)和13.7%(24/175),B组高于A组(χ^(2)=13.634,P<0.05)。结论在高龄孕妇中,胎儿染色体异常发生率随着孕妇年龄增长而上升,行产前诊断羊水细胞染色体核型分析及CNV-seq检测可提高胎儿染色体遗传病的检出率。

CNV-seq结合STR技术在稽留流产遗传学病因分析中的应用

目的 本研究旨在评估将低深度全基因组拷贝数变异测序(copy number variation sequencing, CNV-seq)技术与短串联重复序列(short tandem repeat, STR)技术联合应用于稽留流产患者流产组织遗传学病因分析的效果。方法 收集2019年1月至2022年11月期间因“胚胎停育”而终止妊娠的49例稽留流产患者进行CNV-seq技术和STR分型技术的联合检测。结果 研究发现孕妇流产次数≥2次组的胚胎染色体异常率明显高于流产次数<2次组,差异有统计学意义(62.1%vs 30.0%,P<0.05),而高龄孕妇组与非高龄孕妇组的胚胎染色体的异常率差异无统计学意义(70%vs 66.7%,P>0.05)。在49例流产物中,CNV-seq结合STR技术共检出34例染色体异常,检出率为69.4%(34/49)。其中染色体数目异常的有20例,包括13例非整倍体,5例多倍体(STR技术)和2例嵌合体;染色体结构异常共有14例,其中5例检出为致病性CNV。此外,还检测到了10例临床意义不明(variants of uncertain significance,VUS)的CNV。结论 将低深度CNV-seq技术与STR技术相结合,可以有效地弥补稽留流产的染色体核型分辨率低和培养难度大等缺点,并提高检测稽留流产胚胎异常染色体的能力,明确稽留流产的遗传学病因,为再次妊娠提供更准确的指导。

人恶性胸膜间皮瘤DNA从头测序及基因突变分析

通过DNA从头测序分析人胸膜间皮瘤发生的高关联度突变基因。提取恶性胸膜间皮瘤(MPM)组织和正常胸膜组织DNA,构建基因文库,用Illumina HiSeqX Ten PE 150平台测序,将测序结果与人类基因组数据库的参考序列进行比对、注释,并对测序结果进行过滤、错误率分布检查、GC含量分布检查分析。MPM组织DNA平均过滤37829946 bp,错误率小于0.12%,GC含量占41.17%,而正常胸膜组织DNA平均过滤39089681 bp,错误率小于0.1%,GC含量占41.7%,两者测序质量均在Q 30(≥80%)以上,MPM为87.43%,正常胸膜为88.36%。以上高质量测序数据通过BWA比对到参考基因组(GRCh 37/hg 19),得到最初比对序列,利用重复标记后的比对序列进行覆盖度、深度等统计,覆盖深度达到10 X以上该突变位点可信。结果显示,实验病例XL14覆盖深度达到10 X的占98.59%,覆盖率达到99.83%;对照病例Z5占98.50%,覆盖率达到99.79%。对该序列进行基因注释分析,发现一系列单核苷酸多态性、基因插入缺失、基因结构变异、基因拷贝数变异,筛选出总变异位点数29277个,可能致病的变异位点数22个,致病性的变异位点数5个,不确定变异有害性的位点数为3353个,其余变异位点均为良性。进一步对突变基因进行富集、关联性分析,预测出突变基因TXNDC2与人胸膜间皮瘤的发生高度相关,相关系数达到0.8以上;突变基因PIEN、ABCC1、UGT1A7、UGT1A3、UGT1A4、UGT1A9、ALDH3B1、UGT1A5等与人胸膜间皮瘤有一定关联性,关联度在0~0.2之间。基因TXNDC2、PIEN、ABCC1、UGT1A7、UGT1A3、UGT1A4、UGT1A9、ALDH3B1、UGT1A5的变异可能与人胸膜间皮瘤的发生发展有关。本实验为人胸膜间皮瘤分子诊断提供了参考。

低深度全基因组测序技术在复发性流产遗传学病因诊断中的应用

目的应用低深度全基因组拷贝数变异分析(CNV-seq)技术研究胚胎染色体异常在复发性流产(RSA)及偶发流产(SA)中的差异。方法采集158例RSA患者(RSA组)和244例SA患者(SA组)的流产组织进行CNV-seq检测,对可疑染色体异常的夫妇进行高分辨外周血染色体核型检测。结果402例样本中有2例检测失败,检测成功率99.5%(400/402)。共检测出染色体异常238例(59.5%),包括染色体数目异常212例(89.1%),致病性拷贝数变异25例(10.5%),单亲二倍体1例(0.4%)。RSA组和SA组总体染色体异常、非整倍体、三倍体发生率差异均无统计学意义。RSA组致病性拷贝数变异在染色体异常中的构成比显著高于SA组(P<0.05)。高分辨外周血核型分析检测共发现4例平衡易位携带者。35~39岁年龄段中SA组胚胎染色体异常率高于RSA组(P<0.05)。2组早期流产中胚胎染色体异常率均明显高于中期流产;早期流产中,SA组的流产组织(POC)染色体异常率高于RSA组(P<0.05)。结论CNV-seq可以对胚胎染色体数目异常和染色体片段重复/缺失进行精准诊断,在RSA和SA的遗传学病因诊断中同样重要,可为再生育指导提供依据。

应用脑脊液mNGS-CNV分析辅助诊断合并脑积水的脑膜癌病1例报告

本文报道1例脑膜癌病患者的诊疗过程,患者老年男性,慢性病程,进行性加重,主要临床表现为进行性加重的头痛、恶心、呕吐30 d,加重9 d。头部影像学提示脑积水、脑室扩张,对脑脊液进行病原宏基因组二代测序(mNGS)结合人源序列的染色体拷贝数变异(CNV)分析,结果提示病原检测阴性,而人源序列中存在异常非整倍体,高度提示恶性肿瘤;后给予患者脑室留置Ommaya囊,反复送检脑脊液细胞学检测数次提示异型细胞;根据临床表现、脑脊液细胞学以及拷贝数变异分析结果,确诊脑膜癌病。提示mNGS-CNV分析对于诊断脑膜癌病具有重要意义。希望本例患者诊疗过程的梳理,可为脑膜癌病的诊断和治疗等提供参考。

CNV-seq结合染色体核型分析技术在产前诊断胎儿染色体异常中的价值观察

目的探讨基因组拷贝数变异测序(CNV-seq)结合染色体核型分析技术在产前诊断胎儿染色体异常中的价值。方法回顾性选取2019年6月至2022年6月于绵阳市人民医院产前诊断科行羊膜腔穿刺术且拷贝数变异(CNV)提示异常的107例孕妇为研究对象,分别行CNV-seq检测和染色体核型分析。结果在107例孕妇的羊水样本中,染色体核型分析检出58例(54.21%)胎儿核型异常,包括染色体数目异常36例(62.07%),染色体结构异常11例(18.97%),嵌合体11例(18.97%)。CNV-seq检测对染色体核型分析中的58例核型异常者均成功确诊,变异类型包括54例(93.10%)致病性,4例(6.90%)临床意义不明;CNV-seq检出13例嵌合体病例,其中2例(低于10%)染色体核型分析未检出。在49例核型未见异常羊水样本中,CNV-seq检出致病性变异类型20例(40.82%)、临床意义不明23例(46.94%)、可能良性2例(4.08%)、可能致病性1例(2.04%)、良性变异3例(6.12%)。染色体核型分析产前诊断胎儿染色体异常的阳性率均明显低于CNV-seq检测及二者联合检测的阳性率(χ^(2)=115.654,P<0.05);三种检测方法产前诊断胎儿染色体数目异常、染色体结构异常和嵌合体的检出率比较差异均无统计学意义(P>0.05)。结论在胎儿染色体异常的产前诊断中,CNV-seq可高效、特异地检出染色体核型分析技术无法检出的致病性基因组CNVs,可为产前遗传咨询提供更详细的参考信息。

1q21.1远端微缺失/微重复综合征合并先天性心脏病4例临床及遗传学分析

目的:探讨染色体拷贝数变异测序(copy number variation sequencing,CNV-seq)诊断1q21.1远端微缺失/微重复综合征合并先天性心脏病(congenital heart disease,CHD)的临床应用价值,并对此类患者进行临床及遗传学分析。方法:回顾性分析4例就诊于甘肃省妇幼保健院,经CNV-seq诊断为1q21.1微缺失/微重复综合征合并CHD患儿的临床及遗传学特征。结果:4例1q21.1微缺失/微重复综合征合并CHD患儿染色体CNV重叠区域为chr1:g.146520000-147840000,包含心脏相关的基因有CAJ5、CAJ8、PPKAB2、CHD1L和BCL9等。1例1q21.1微重复患儿还表现为小下颌、舌后坠、上颌腭裂的多发畸形和泌尿系统的发育异常,3例1q21.1微缺失患儿中有2例表现出严重的生长发育迟缓(其中1例伴有严重的智力障碍、肌张力减低和小阴茎,1例特殊面容),1例患儿已行CHD手术,预后良好。结论:CHD合并发育迟缓和(或)特殊面容是1q21.1微缺失/微重复综合征低龄患儿的重要表型,此类表型患儿有必要做染色体CNV-seq检测,为进一步临床诊治提供理论依据。

低深度全基因组测序和染色体微阵列分析检测在颈部透明层增厚胎儿产前诊断中的价值

目的对比分析低深度全基因组测序(CNV-seq)和染色体微阵列分析(CMA)检测在颈部透明层(NT)增厚胎儿产前诊断中的价值。方法回顾性分析2019年1月至2020年12月九江市妇幼保健院接受早孕期产前检查的120例胎儿NT厚度≥2.5mm孕妇的临床资料,以随访确诊结果为金标准,比较CNV-seq和CMA检测结合染色体核型分析对出生缺陷的检测效能。结果随访确诊结果显示,120例胎儿NT厚度≥2.5mm孕妇中,致病性染色体异常22例,非致病性98例。CNV-seq检测结合染色体核型分析检出致病性染色体异常21例,非致病性99例;CMA检测结合染色体核型分析检出致病性染色体异常14例,非致病性106例。CNV-seq检测结合染色体核型分析的灵敏度、准确率均高于CMA检测,差异有统计学意义(P<0.05);两种方法特异度比较差异无统计学意义。CNV-seq检测、CMA检测的ROC曲线下面积分别为0.858、0.792,CNV-seq检测的诊断效能较高。结论CNV-seq检测结合染色体核型分析较CMA检测结合染色体核型分析在NT增厚胎儿产前诊断中的灵敏度和准确率更高,价格相对低廉,应用价值更高。

染色体核型分析联合CNV-Seq检测在高龄孕妇产前诊断中的应用

目的探讨染色体核型分析与全基因组拷贝数变异测序(CNV-Seq)技术在高龄孕妇产前诊断中联合应用的意义。方法对2020年1月至2022年12月该院收治的723例高龄孕妇的羊水细胞染色体核型分析、CNV-Seq检测结果进行回顾性分析。结果723例高龄孕妇中检出染色体异常共29例,异常检出率为4.0%。723例高龄孕妇中检出核型异常21例,异常检出率为2.9%,其中染色体非整倍体13例,包括21-三体7例,18-三体1例,性染色体非整倍体5例;染色体嵌合3例,包括性染色体嵌合2例,常染色体嵌合1例;染色体结构异常5例,包括染色体倒位3例,染色体易位2例;检出CNV-Seq异常24例,异常检出率为3.3%,其中染色体非整倍体13例,包括21-三体7例,18-三体1例,性染色体非整倍体5例;染色体嵌合3例,包括性染色体嵌合2例,常染色体嵌合1例;致病性染色体拷贝数变异8例,包括染色体微重复1例,染色体微缺失7例。其中染色体非整倍体异常中染色体核型分析和CNV-Seq检测结果一致。结论染色体核型分析联合CNV-Seq检测可提高染色体异常检出率,两种方法各自有独特的优势,可以相互验证,互补不足,染色体核型分析可比较直观地检测出染色体结构变异,而CNV-Seq可检测出染色体微缺失、微重复。

两种方法检测先天性心脏发育异常胎儿的染色体结果分析

目的:探讨拷贝数变异测序(CNV-seq)技术和染色体核型分析技术检测先天性心脏发育异常(CHD)胎儿染色体的应用价值。方法:以2019年2月至2022年8月天津市中心妇产科医院经超声科诊断胎儿CHD的60例孕妇为研究对象,并根据是否伴发心外异常分为独立性CHD组和伴心外结构/软指标异常CHD组,所有孕妇行羊水穿刺进行核型分析及CNV-seq检测,统计分析两种方法对异常染色体的检出率。结果:两种方法检测共发现染色体异常患者20例,异常染色体检出率为33.3%,其中核型分析检出染色体异常例数为13例,CNV-seq检测异常CNVs例数为18例,两种方法结果均异常者11例,核型独立检出平衡易位2例,CNV-seq独立检出微缺失/微重复7例。伴心外结构/软指标异常CHD组染色体异常检出率略高于独立性CHD组,两组间比较差异无统计学意义[37.8%(14/37)vs.26.1%(6/23),χ^(2)=1.76,P>0.05]。结论:联合应用核型分析和CNV-seq检测技术,可以进一步明确诊断由染色体异常引发的胎儿CHD。

全外测序联合拷贝数变异检测在遗传性耳聋的应用

目的探讨全外显子测序(WES)联合拷贝数变异(CNV)检测在遗传性耳聋中的临床应用价值,并加深对CNV的认识。方法选取广州市红十字会医院耳鼻咽喉头颈外科就诊的双耳中度感音神经性聋患儿,无家族遗传史、用药史,完善内镜、影像学、主观和客观听力学等检查,采集外周血样本,行WES寻找致聋原因并验证。结果患儿无家族遗传史、耳毒性药物用药史等,听性脑干反应阈值、ASSR及纯音听阈测听提示双侧中度感音神经性聋。在该患儿全外显子组发现12个纯合变异,分别定位于1(CR1基因,剪接变异)、5(ZSWIM6基因、SMN1基因,同义突变)、6(ATXN1基因,框内缺失突变;TENT5A基因,框内插入突变)、7(CFTR基因,内含子)、8(TG,启动子)、9(PRDM12基因,框内缺失突变)、10(TUBGCP2基因,剪接变异)、11(TENM4基因,剪接变异)、15(STRC基因,缺失)、16(ABCC11基因,错义变异)号染色体。根据美国医学遗传学与基因组学学会指南、综合病史分析,只有STRC基因NM_153700.2:EX1-EX29E Del变异为致病变异,其余变异为良性或可能良性。多重链接探针扩增技术对靶序列进行验证,结果证实。结论本例患儿为DFNB16(OMIM:603720)的STRC基因变异导致双耳中度感音神经性聋。临床诊疗中,可根据病史,选择不同深度、广度的检测技术;加强耳科医师对CNV引起遗传性耳聋的认识。

拷贝数变异测序在检测胎儿鼻骨发育不良结果中的应用研究

目的探讨拷贝数变异测序(CNV-seq)应用在胎儿鼻骨发育结果检测的临床价值。方法选取2018年8月至2019年12月在广州市妇女儿童医疗中心柳州医院进行产前超声筛查发现胎儿鼻骨发育异常的孕妇160例为研究对象,比较染色体核型分析和CNV-seq技术检测结果差异。结果染色体核型分析检测出39例染色体异常,其中常染色体数目异常32例,性染色体异常5例,染色体结构异常2例;CNV-seq检测出16例染色体异常,其中多态性9例,明确致病性7例;年龄≥35岁孕妇羊水染色体核型异常检出率高于年龄<35岁孕妇,且在年龄≥35岁孕妇中,羊水染色体核型异常检出率高于CNV-seq检测(χ^(2)值分别为15.856、20.928,P<0.05);胎龄<24周羊水染色体核型异常检出率高于胎龄≥24周,且在胎龄<24周中,羊水染色体核型异常检出率高于CNV-seq检测(χ^(2)值分别为16.979、16.311,P<0.05);产前诊断指征2项及以上者羊水染色体核型异常检出率高于2项以下者,而CNV-seq异常检出率明显低于2项以下者(χ^(2)值分别为9.246、10.338,P<0.05);在产前诊断指征2项及以上者中,羊水染色体核型异常检出率高于CNV-seq检测(χ^(2)=27.655,P<0.05)。结论在产前超声筛查出胎儿鼻骨发育异常的孕妇中,CNV-seq有较好的应用价值,可弥补染色体核型分析的不足,有助于染色体结构异常的检出。