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Deletion or underexpression of the Y-chromosome genes CDY2 and HSFY is associated with maturation arrest in American men with nonobstructive azoospermia 被引量:3
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作者 Peter J Stahl Anna N Mielnik +2 位作者 Christopher E Barbieri Peter N Schlegel Darius A Paduch 《Asian Journal of Andrology》 SCIE CAS CSCD 2012年第5期676-682,共7页
Maturation arrest (MA) refers to failure of germ cell development leading to clinical nonobstructive azoospermia. Although the azoospermic factor (AZF) region of the human Y chromosome is clearly implicated in som... Maturation arrest (MA) refers to failure of germ cell development leading to clinical nonobstructive azoospermia. Although the azoospermic factor (AZF) region of the human Y chromosome is clearly implicated in some cases, thus far very little is known about which individual Y-chromosome genes are important for complete male germ cell development. We sought to identify single genes on the Y chromosome that may be implicated in the pathogenesis of nonobstructive azoospermia associated with MA in the American population. Genotype-phenotype analysis of 132 men with Y-chromosome microdeletions was performed. Protein-coding genes associated with MA were identified by visual analysis of a genotype-phenotype map. Genes associated with MA were selected as those genes within a segment of the Y chromosome that, when completely or partially deleted, were always associated with MA and absence of retrievable testicular sperm. Expression of each identified gene transcript was then measured with quantitative RT-PCR in testicular tissue from separate cohorts of patients with idiopathic MA and obstructive azoospermia. Ten candidate genes for association with MA were identified within an 8.4-Mb segment of the Y chromosome overlapping the AZFb region. CDY2and HSFYwere the only identified genes for which differences in expression were observed between the MA and obstructive azoospermia cohorts. Men with obstructive azoospermia had 12-fold higher relative expression of CDY2transcript (1.33__.0.40 vs. 0.11+_0.04; P=O.O003) and 16-fold higher expression of HSFYtranscript (0.78__.0.32 vs. 0.05_0.02; P=O.O005) compared to men with MA. CDY2 and HSFYwere also underexpressed in patients with Sertoli cell only syndrome. These data indicate that CDY2and HSFYare located within a segment of the Y chromosome that is important for sperm maturation, and are underexpressed in testicular tissue derived from men with MA. These observations suggest that impairments in CDY2 or HSFYexpression could be implicated in the pathogenesis of M 展开更多
关键词 CDY1 protein CDY2 protein genetics HISTOLOGY HSFY human make infertility nonobstructive azoospermia spermato-genesis sperm maturation
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连接黏附分子C的研究进展 被引量:4
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作者 杨勇 唐文 《医学综述》 2010年第13期1953-1957,共5页
连接黏附分子C(JAM-C)是近几年来研究逐渐增多的一种免疫球蛋白。JAM-C的分子结构、分布及其与特定配体作用的特点,决定了JAM-C在精子的形成、调节细胞旁通透性、调节白细胞的游走、调节血管的发生和肿瘤的增长、转移等多种生理、病理... 连接黏附分子C(JAM-C)是近几年来研究逐渐增多的一种免疫球蛋白。JAM-C的分子结构、分布及其与特定配体作用的特点,决定了JAM-C在精子的形成、调节细胞旁通透性、调节白细胞的游走、调节血管的发生和肿瘤的增长、转移等多种生理、病理过程中起到了极其重要的作用,也对相关疾病的诊断及治疗提供了新的研究方向。现就JAM-C的分布表达、病理生理作用、与相应疾病的关系以及其可能作为未来疾病治疗的靶点予以综述。 展开更多
关键词 连接黏附分子C 血管发生 白细胞游走 精子发生 肿瘤转移
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氯氰菊酯通过调控miR-409b对青春期鼠雄性生殖系统的影响及作用机制 被引量:1
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作者 徐玮 邵颖颖 杜二球 《中国现代医生》 2021年第28期27-30,F0003,共5页
目的探讨氯氰菊酯对青春期雄性大鼠生殖系统的影响及相关机制。方法随机将40只SD健康青春期雄性大鼠分为正常组和低、中、高剂量组各10只,四组大鼠分别进行干预。采用RT-PCR法检测miR-409b、miR-30b-3p表达,检测各组大鼠生殖系统重量,... 目的探讨氯氰菊酯对青春期雄性大鼠生殖系统的影响及相关机制。方法随机将40只SD健康青春期雄性大鼠分为正常组和低、中、高剂量组各10只,四组大鼠分别进行干预。采用RT-PCR法检测miR-409b、miR-30b-3p表达,检测各组大鼠生殖系统重量,检测精子生成、存活情况,采用免疫透射比浊法检测性激素、氧化应激指标水平。结果高剂量组miR-409b、miR-30b-3p表达、精囊重量高于低、中剂量组(P<0.05),前列腺、睾丸、附睾重量及精子数量、每日精子生成量、精子成活率低于低、中剂量组(P<0.05)。高剂量组T、LH水平低于低、中剂量组(P<0.05),FSH、LPO、TAS、ROS水平高于低、中剂量组(P<0.05)。结论氯氰菊酯干预能够调控青春期雄性大鼠miR-409b、miR-30b-3p表达,影响大鼠生殖系统发育、精子生成、存活及性激素水平,其机制可能是氯氰菊酯干预能够引起睾丸氧化应激反应。 展开更多
关键词 氯氰菊酯 生殖系统 氧化应激 睾丸 性激素 精囊 精子生成
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