Y-chromosomal microdeletions and partial deletions of the Azoospermia Factor c(AZFc)region in normozoospermic,severe oligozoospermic and azoospermic men in Sri Lanka

Aim： To assess for the first time the occurrence of Y chromosomal microdeletions and partial deletions of the Azoospermia Factor c （AZFc） region in Sri Lankan men and to correlate them with clinical parameters. Methods： In a retrospective study, we analyzed 96 infertile men （78 with non-obstructive azoospermia） and 87 controls with normal spermatogenesis. AZFa, AZFb, AZFc and partial deletions within the AZFc region were analyzed by multiplex polymerase chain reaction （PCR） according to established protocols. Results： No AZFa, AZFb or AZFc deletions were found in the control group. Seven patients in the group of infertile men were found to have deletions as following： one AZFa, two AZFc, two AZFbc and two AZFabc. The relative distribution of these patterns was significantly different compared with that found in the German population. Extension analysis confirmed that the deletions occurred according to the current pathogenic model, gr/gr deletions were found to be equally present both in the patients （n = 4） and in the control group （n = 4）. One b2/b3 deletion was found in the patient group. Conclusion： These results suggest that the frequency and pattern of microdeletions of the Y chromosome in Sri Lankan men are similar to those found in other populations and confirm that gr/gr deletions are not sufficient to cause spermatogenetic failure. （Asian J Androl 2006 Jan; 8： 39-44）

The prevalence of azoospermia factor microdeletion on the Y chromosome of Chinese infertile men detected by multi-analyte suspension array technology

Aim： To develop a high-throughput multiplex, fast and simple assay to scan azoospermia factor （AZF） region microdeletions on the Y chromosome and establish the prevalence of Y chromosomal microdeletions in Chinese infertile males with azoospermia or oligozoospermia. Methods： In total, 178 infertile patients with azoospermia （nonobstructed）, 134 infertile patients with oligozoospermia as well as 40 fertile man controls were included in the present study. The samples were screened for AZF microdeletion using optimized multi-analyte suspension array （MASA） technology. Results： Of the 312 patients, 36 （11.5%） were found to have deletions in the AZF region. The rnicrodeletion frequency was 14% （25/178） in the azoospermia group and 8.2% （11/134） in the oligospermia group. Among 36 patients with microdeletions, 19 had deletions in the AZFc region, seven had deletions in AZFa and six had deletions in AZFb. In addition, four patients had both AZFb and AZFc deletions. No deletion in the AZF region was found in the 40 fertile controls. Conclusion： There is a high prevalence of Y chromosomal microdeletions in Chinese infertile males with azoospermia or oligozoospermia. The MASA technology, which has been established in the present study, provides a sensitive and high-throughput method for detecting the deletion of the Y chromosome. And the results suggest that genetic screening should be advised to infertile men before starting assisted reproductive treatments.

Uniform deletion junctions of complete azoospermia factor region c deletion in infertile men in Taiwan

Aim： To determine the deletion junctions of infertile men in Taiwan with azoospermia factor region c （AZFc） deletions and to evaluate the genotype/phenotype correlation. Methods： Genomic DNAs from 460 infertile men were examined. Bacterial artificial chromosome clones were used to verify the accuracy of polymerase chain reaction. Deletion junctions of the AZFc region were determined by analysis of sequence-tagged sites and gene-specific markers. Results： Complete AZFc deletions, including BPY2, CDY1 and DAZ genes, were identified in 24 men. The proximal breakpoints were clustered between sY1197 and sY1192, and the distal breakpoints were clustered between sY1054 and sYl125 in all but one of the 24 men. The testicular phenotypes of men with complete AZFc deletion varied from oligozoospermia, to hypospematogenesis, to maturation arrest. Conclusion： We identified a group of infertile men with uniform deletion junctions of AZFc in the Taiwan population. Despite this homogeneous genetic defect in the AZFc region, no clear genotypedphenotype correlation could be demonstrated. （Asian JAndrol 2006 Mar; 8： 205-211）

Molecular genetic analysis of microdeletion on AZF/DAZ gene in patients with idiopathic azoospermia and severe oligozoospermia in Fujian

Objective: To identify microdeletions in azoospermia factor(AZF) gene loci in patients with idiopathic azoospermia and severe oligozoospermia in Fujian. Methods: Molecular genetic detection method was used to detect microdeletion at the AZFa, AZFb, AZFc /DAZ,SRY region of Y chromosome in 47 azoospermia and 4 severe oligozoospermia patients. Genomic DNA was extracted from peripheral blood. The sequence tagged site (STS) primers tested in each cases were sY84(AZFa), sY 143(AZFb) sY254(AZFc).SRY region of Y chromosome for control. The PCR products were analyzed on a 2.0% agarose gel. Results: Microdeletions of the Y-chromosomal AZF loci were revealed in 18(35.3%,18/51) of 51 patients with idiopathic azoospermia and severe oligozoospermia. AZFa deletion was found in four (7.8%) patients, AZF b in five (9.8%) patients, AZF c in four (7.8%) patients. AZF a+b in one(1.9%)patient, AZF b+c in two (3.9%) patients, AZF a+b+c in two (3.9%)patients respectively. No deletion of SRY region was found. No deletion of AZF a, AZF b, AZF c/DAZ,SRY regions was found in five fertile male who had at least one or more children. Conclusions: Microdeletions on AZF/DAZ gene loci were major genetics defects leading to azoospermia and severe oligozoospermia in male idiopathic infertility in Fujian. It is necessary to have genetic counseling and carry out microdeletion detection on AZF/DAZ gene loci before performing intracytoplasmic sperm injection (ICSI).

Y染色体AZFc区缺失患者使用睾丸取精精子与射出精子行ICSI的结局比较

目的 比较Y染色体长臂无精子症因子(AZF)c区缺失患者使用新鲜射出精子与睾丸取精精子行卵胞浆内单精子注射(ICSI)后的受精情况和妊娠结局。方法 采用回顾性队列研究,分析2017年1月至2022年12月因AZFc区缺失于西北妇女儿童医院行自精ICSI助孕患者的临床资料。根据女方取卵日男方不同取精方式分为两组:男方行睾丸手术取精的患者纳入睾丸取精组(n=68),男方新鲜射出精子的患者纳入对照组(n=242),比较两组的一般资料和ICSI结局。结果 睾丸取精组的男方LH水平显著高于对照组(P<0.05)。两组间的卵裂数、双原核(2PN)数、可用胚胎数、优质胚胎数比较均无显著性差异(P>0.05);睾丸取精组的囊胚形成数显著低于对照组(P<0.05)。睾丸取精组、对照组的首个新鲜移植周期数分别为30个周期和125个周期,睾丸取精组的受精率、正常受精率、卵裂率、可用胚胎率、囊胚形成率均显著低于对照组(P<0.05),两组间的种植率、临床妊娠率、流产率及活产率比较均无显著性差异(P>0.05)。单因素Logistic分析结果显示,取精方式与受精率、正常受精率、可用胚胎率、优质胚胎率、囊胚形成率、种植率、临床妊娠率、流产率及活产率不具有显著关联性(P>0.05),但会显著影响卵裂率[OR=2.62,95%CI(0.87,4.36),P=0.003];多因素Logistic回归分析显示,在校正囊胚形成数及男方LH水平这两个混杂因素后,对照组的卵裂率仍显著高于睾丸取精组[OR=-3.002,95%CI(-5.182,-0.821),P=0.007]。结论 对于AZFc区缺失患者,相较于新鲜射出精子,采用睾丸取精精子行ICSI时的卵裂率明显降低,虽然二者的妊娠结局没有明显差异,但考虑到手术取精的风险及经济成本,仍建议优先选择射精精子来进行ICSI。

原发性无精、少弱精症患者Y染色体AZF微缺失检测

目的:研究男性不育与Y染色体位点缺失的相关性,建立可靠的原发性无精子症和少弱精子症患者Y染色体微缺失的基因诊断方法。方法:采用多重PCR技术,对100例染色体核型正常的、无精子症和少弱精子症患者Y染色体无精子因子(azoospermia factor,AZF)区域的6个序列标签位点进行检测。结果:100例患者中,4例(4%)Y染色体上存在不同位点等位基因片段的缺失,其中3例患者为无精子症;1例为严重少弱精子症。结论:以多重PCR为基础的AZF微缺失筛查是一种简单有效的诊断原发性无精子症和少弱精子症的方法。Y染色体微缺失是严重生精障碍的重要原因之一。

男性不育患者Y染色体AZF区微缺失分析

目的:探讨Y染色体上无精子因子(AZF)微缺失与男性不育的关系。方法:应用多重PCR技术,采用AZF区9个序列标签位点(STS),对107例男性不育患者(83例无精子症和24例严重少精子症)和20例正常生育男性外周血进行微缺失分析。结果:在107例无精症和少精子症不育患者中11例AZF区域微缺失,缺失率10.3%,其中无精症组缺失率为9.6%(8/83),少精子症组缺失率为12.5%(3/24)。11例微缺失患者中,单独AZFc区缺失患者5例(45.5%),AZFc+d区缺失患者4例(36.4%),AZFb+c区、AZFb+c+d区缺失患者各1例(9.1%);位点sY254和sY255缺失患者分别为72.7%(8/11)和100%(11/11)。20例正常生育男性未检测出Y染色体微缺失。结论:Y染色体AZF微缺失是导致男性不育患者精子发生障碍的重要原因。

结合血清卵泡刺激素、抑制素B、染色体核型和Y染色体AZF基因微缺失与睾丸穿刺取精术成功率的相关性

目的探讨无精子症患者血清卵泡刺激素(FSH)、抑制素B(INHB)、染色体核型、Y染色体AZF基因微缺失(AZF-MD-Ych)与睾丸穿刺精子抽吸(TESA)成功率的相关性。方法在162例血清FSH正常组和100例血清FSH异常组的育龄期无精子症患者中进行对比分析,分析两组患者INHB水平、INHB/FSH的比值、外周血染色体核型和AZF-MD-Ych的差异性。排除INHB异常、染色体异常和AZF-MD-Ych阳性后,再比较两组患者TESA的成功率。结果两组患者中,血清INHB水平、INHB/FSH比值和外周血染色体核型均具有显著性差异(P<0.05),而AZF-MD-Ych这两组中没有统计学上的差异(P>0.05);在未检测到染色体异常、AZF-MD-Ych阳性及INHB异常的患者中,TESA显示精子获取率在FSH正常组为61.82%(34/55),FSH异常组均未成功(0/16),二者存在统计学差异(P<0.01)。结论现有的血清FSH正常值结合INHB、染色体核型分析和AZF-MD-Ych检查,能够综合判断TESA的成功率,四项指标均出现异常者,TESA的成功率极低。

改良多重聚合酶链反应检测Y染色体AZF微缺失

目的:对多重聚合酶链反应(PCR)优化改良,检测Y染色体无精子因子(AZF)区域微缺失。方法:实验组选择160例精子发生障碍患者,对照组90例为合格捐精者。按照欧洲男科协会和欧洲分子遗传实验质控网检测指南进行多重PCR,对Y染色体序列标签点引物序列和PCR反应条件优化改良,筛查AZFa、b、c区域的微缺失。结果:采用改良多重PCR,160例生精障碍患者中发现AZF微缺失14例(8.75%),其中AZFc12例,AZFa+b+c1例,AZFb+c1例;对照组90例未发现微缺失;两组比较,差异有极显著性(P<0.001)。所有PCR产物电泳条带清晰,时间缩短至1h。结论:对欧洲男科协会和欧洲分子遗传实验质控网推荐的多重PCR技术优化改良,用于精子发生障碍患者的YqAZF区域筛查,结果可靠、快捷、重复性好。

AZF与男性不育研究进展

AZF微缺失的发生率在1%～55%之间不等。AZF基因缺失与严重的生精功能障碍密切相关,是最常见的导致严重少弱精子症和无精子症的分子遗传学因素。对AZF及其相关基因的研究,可从分子水平阐明精子发生障碍的机制,对男性不育症的诊断、治疗及预后判断具有非常重要的意义。本文综述了AZF基因结构和功能特点,及其与男性不育、隐睾、精索静脉曲张、Klinefelter综合征、精原细胞瘤、习惯性流产等之间的关系。

无精子症和严重少精子症患者AZF/DAZ基因微缺失的分子生物学检测

目的 用分子生物学方法检测无精子症和严重少精子症患者无精子基因 (AZF)AZF/DAZ基因微缺失。 方法 应用聚合酶链反应 (PCR)技术对无精子症 4 7例、严重少精子症 4例进行Y染色体AZFa、AZFb、AZFc/DAZ、SRY的微缺失检测。 结果 5 1例患者缺失率为 35 .3% (18/ 5 1) ,其中AZFa、AZFb、AZFc的微缺失分别为 4例 (7.8% )、5例 (9.8% )和 4例 (7.8% )。无精子症患者 1例 (1.9% )为AZFa、AZFb的双重缺失 ,2例 (3.9% )为AZFb、AZFc的双重缺失 ;2例 (3.9% )为AZFa、AZFb和AZFc的三重缺失 ;5 1例SRY基因PCR扩增均为阳性。 5例已有生育的正常男性均无AZFa、AZFb、AZFc、SRY的微缺失。 结论 AZF/DAZ(包括AZFa、AZFb、AZFc/DAZ)基因的微缺失是引起无精子和严重少精子导致男性不育的重要原因之一。AZF/DAZ基因微缺失的分子生物学检测对不明原因的不育男性行胞浆内单精子注射 (ICSI)时有指导意义。

排除AZF微缺失为反复自然流产的原因

目的:探讨Y染色体上AZF微缺失和反复自然流产之间的关系。方法:收集26份男性流产胚胎的绒毛样本,51份配偶反复流产的男性血液,分别提取基因组DNA,选取位于Yq11.2上AZFa、AZFb和AZFc的12个STS位点,对流产胚胎绒毛样本和血液样本进行AZF的多重PCR检测。结果:流产胚胎的26份样本中没有发现AZF的微缺失,51份血液样本中也没有发现AZF的微缺失。结论:排除AZF微缺失为反复自然流产的原因。

特发性不育患者Y染色体AZF微缺失筛查及表型分析

目的:探讨特发性不育患者Y染色体无精子症因子(AZF)微缺失的发生率及缺失类型与表型的关系。方法:应用多重PCR方法对本院1700例特发性不育患者进行Y染色体AZF微缺失分析。结果:AZF微缺失发生率为6.59%(112/1700),其中AZFc缺失占67.86%(76/112),35例表现为无精子症,31例表现为少精子症;AZFb+c+sY145缺失占17.86%(20/112),AZFa缺失占4.46%(5/112),AZFa+b+c联合缺失占4.46%(5/112),AZFb+c联合缺失占2.68%(3/112),AZFb+c和sY84(AZFa区)缺失占1.79%(2/112),AZFc和sY143(AZFb区)缺失占0.89%(1/112),均表现为无精子症。结论:Y染色体AZFc缺失患者表型多样,AZFa和AZFb缺失均表现为无精症。对特发性不育患者进行Y染色体AZF微缺失筛查很有必要,尤其对于拟行辅助生殖技术助孕的不育患者。

150例男性不育患者Y染色体AZF基因微缺失分析

目的:探讨Y染色体无精子因子(AZF)微缺失检测在男科诊断中的应用价值。方法:采用多重聚合酶链反应技术及琼脂糖凝胶电泳方法,对150例男性不育患者AZF基因的3个STS位点进行分析。结果:150例中22例(14.67%)AZF基因位点发生微缺失,其中AZFc位点缺失最多,其次为AZFb,AZFa最低。结论:AZF基因微缺失与精子缺陷发生密切相关,对男性不育患者进行Y染色体AZF区域微缺失检测是必要的。

中国汉族人群AZFc微缺失区域序列标签位点的探讨

目的:探讨中国人群无精子因子c(azoosperm ia factor c,AZFc)微缺失的类型及AZF多重PCR筛查时序列标签位点(sequence taged sites,STSs)的选择。方法:采用多重PCR反应测定9个STS位点(sY84、sY86、sY127、sY134、sY152、sY145、sY255、sY254、sY157)筛查164例严重少精子症或非梗阻性无精子症汉族男性Y染色体微缺失,并以精子浓度正常的男性105例作为对照;同时对来自多中心的180例已确诊为sY254、sY255缺失的男性进行sY145、sY152和sY157位点分析。结果:164例严重少精子症或无精子症男性中AZFc缺失者14例(8.5%);共194例sY254、sY255缺失男性的sY145、sY152均未缺失,而sY157未缺失者仅2例。发现1例单sY157缺失的严重少精子症男性为sY1206缺失和DAZ基因中DAZ3/DAZ4基因拷贝缺失。结论:sY254、sY255和sY157缺失是中国人群AZFc缺失的最常见类型;sY145和sY152微缺失在入选的研究对象中未曾出现,因此不建议作为AZFc常规筛查的位点。"sY157的单一缺失"可能是中国人群AZFc部分缺失的一种新类型,其临床意义值得进一步探讨。

严重少精、无精患者无精子因子(AZF)的检测及意义

目的:探讨无精子因子(azoospermiafactor,AZF)与不育男性精子生成的关系。方法:检测79例无精、严重少精不育男性及10例正常生育男性的AZF基因缺失状况,并根据是否合并有其他男性学检查异常,将受检患者进一步划分为原发性和非原发性男性不育两组,比较各组间AZF基因缺失的检出率。结果:79例受检的无精或严重少精患者有8例(10.1%)AZF基因缺失,10例精液正常生育男性均未见有基因缺失。61例无精子和18例严重少精患者,分别检出6例(9.8%)和2例(11.1%)AZF基因缺失,两组AZF缺失检出率无统计学差异(P>0.05)。34例原发性和45例非原发性男性不育患者,分别有6例(17.6%)和2例(4.4%)AZF缺失,两组缺失检出率有统计学差异(P<0.05)。结论:AZF与精子生成障碍密切相关,它是原发性无精或严重少精的重要病因之一。

中国南方地区不育男性Y染色体AZF区域微缺失分析

目的检测并分析中国南方地区不育男性Y染色体上无精症因子(Azoospermia factor,AZF)区域的微缺失情况。方法运用多重PCR技术选用18个STS位点分为四组,设置空白对照,并采用正常男性DNA标本为阳性对照,筛查在海南医学院附属医院生殖医学中心就诊的1 152例诊断为无精、少精及弱精男性的AZFa、AZFb、AZFc和AZFd 4个区域的微缺失情况。结果 1 152例男性患者中共检出67例AZF微缺失,缺失率为5.8%;其中,无精症13例,弱精症1例,少精症7例,严重少精症46例。上述患者中60例被检出AZFc合并AZFd区或AZFb合并AZFd区的双重缺失,1例被检出AZFc、AZFb合并AZFd区的三重缺失;就各区缺失率而言,AZFa为1.49%(1/67),AZFb为4.48%(3/67),AZFc为92.54%(62/67),AZFd为95.52%(64/67)。结论采用多重PCR技术进行AZF微缺失检测十分简单可行,该项检测对了解男性不育发生原因、帮助临床制定辅助生殖技术方案十分必要。

Y染色体AZFc微缺失规律的研究

目的:探讨中国汉族人群Y染色体AZFc微缺失的规律。方法:采用9个STS位点(sY84、sY86、sY127、sY134、sY152、sY145、sY255、sY254、sY157)的多重PCR,排除sY84、sY86、sY127、sY134缺失的患者,共有194例严重少弱精子症或非梗阻性无精子症汉族男性发生AZFc微缺失;对其中192例sY254、sY255、sY157缺失的患者,再通过sY1191、sY1197、sY1054、sY1125及sY1206 STS位点检测,分析其缺失规律。结果:192例sY254、sY255、sY157缺失患者存在5种缺失模式,其中常见的为sY1197(+)、sY1191(-)、sY1206(-)、sY1054(-)、sY1125(+),占54.17%(104/192);sY1197(+)、sY1191(+)、sY1206(-)、sY1054(-)、sY1125(+),占28.12%(54/192);sY1197(+)、sY1191(-)、sY1206(-)、sY1054(+)、sY1125(+),占14.58%(28/192)。70.83%的AZFc微缺失患者,近端缺失区域发生在sY1197和sY1191之间(属于b2区域);82.29%的AZFc微缺失患者,远端缺失区域发生在sY1054和sY1125之间(属于b4区域)。结论:中国汉族人群AZFc微缺失有5种缺失模式,AZFc微缺失近、远端缺失位点基本集中于复制子b2和b4。

男性不育215例AZF基因检测结果分析

目的:研究Y染色体长臂的无精子因子AZF(azoospermia factor)基因的检测对诊治男性不育的重要意义。方法:对268例男性不育者进行体格检测、生殖激素六项检测、精液常规检测和染色体核型分析,选取其中染色体核型正常者215例,根据各项分析结果将其分为四组:无精症组、严重少精症组、少精症组及其他组(包括其妻反复自然流产,隐睾或严重精索静脉曲张患者)。另选健康男性20例为对照组,采用多重PCR技术对其进行AZF基因检测。结果:215例中有15例存在不同位点的AZF基因微缺失,其中无精症组6例,缺失率为14.6%,严重少精症组9例,缺失率为13.8%。无精症组和严重少精症组的缺失率与其他各组比较差异有统计学意义(P<0.05)。结论:Y染色体AZF基因缺失是严重生精障碍的重要原因之一。AZF基因筛查是一种简单有效的诊断原发性无精子症和严重少精子症的方法。

应用人类特异性引物扩增无毛小鼠SRY及AZF基因

目的 :了解人类SRY和AZF基因与雄性无毛小鼠生精基因的相关性。方法 :应用人类特异性引物扩增近交系无毛小鼠、昆明小鼠、DBA小鼠、HLC近交系小鼠的SRY和AZFa、AZFb、AZFc基因。结果 :4种小鼠均能扩增出SRY和AZFa、AZFb、AZFc基因 ,但小鼠的SRY和AZFb基因的PCR产物片段大小与人类的不一致。结论 :①无毛小鼠的SRY和AZFa、AZFb、AZFc基因与其他 3个品系小鼠的扩增产物片段大小无品系间差异。②雄性无毛小鼠繁殖率低的原因可能与生精相关基因无关。