MicroRNA在哺乳动物精子发生中的作用

MicroRNAs(miRNAs)是一类长20~24 nt的单链非编码调控RNA序列。miRNA作为基因转录后表达调控分子,通过碱基互补配对的方式与靶mRNA结合,从而导致靶mRNA的降解或抑制其翻译过程。从最早发现存在于秀丽隐杆线虫Caenorhabditis elegans中的miRNA lin-4和let-7至今20多年里,研究人员已陆续从不同的种属中发现了大量的miRNA。近年来随着基因克隆、表达和功能研究技术的应用和发展,通过分析不同动物物种睾丸组织中miRNA的变化表明miRNA与精子发生过程密切相关。此外,miRNA相关的Dicer、Drosha等蛋白在初级精母细胞减数分裂粗线期所发挥的调控功能通过大量啮齿动物基因敲除模型得到证实。本文从miRNA的合成、作用机制和精子发生过程中的调控作用进行综述。     

哺乳动物精子发生过程中的细胞凋亡及其影响因素

睾丸生殖细胞凋亡是维持精子发生动态平衡,限制生精上皮生殖细胞数量的一个重要生理机制,受多种因素调控。本简要叙述精子发生过程中细胞凋亡的激素调节、基因调控及其他理化等因素的影响及其作用机制。     

长链非编码RNA在哺乳动物精子发生中的功能研究进展

长链非编码RNA(lncRNA)一般是指大于200 nt的RNA,位于细胞核内或胞浆中,不参与蛋白质编码,以RNA形式在表观遗传调控、转录调控以及转录后调控等多个层面上调控基因的表达水平。哺乳动物精子发生是一个精细调控的过程,通过雄性生殖细胞分裂和分化形成成熟精子,且精子发生受到不同阶段特异性基因表达的严格调控,而特异性基因表达又受到大量lncRNAs的调控。虽然lncRNA作为一类重要的基因表达调控因子广泛参与各类生物个体发育进程和疾病的发生,但是精子发生相关lncRNAs的报道并不多,且其生物学功能的研究有待进一步深入。因此,本文对lncRNA的起源、作用机制和在精子发生过程中调控作用的研究进展进行了总结分析。     

哺乳动物精子磷酸化蛋白质组学研究进展

蛋白质的表达、修饰及相互作用的研究已成为后基因组学时代蛋白质组学中的重要内容。蛋白质磷酸化和去磷酸化作为最普遍的翻译后修饰之一,是精子细胞信号转导和酶调控、表达的主要分子机制,亦是精子、卵细胞信号识别及完成受精作用的关键环节。对精子磷酸化蛋白功能的研究有助于深入理解精子的获能、超激活运动的维持、发生顶体反应及精卵结合等受精过程的分子调控机理。对哺乳动物精子磷酸化蛋白质组学的研究进展,包括动物精子磷酸化蛋白质组学研究的技术方法、磷酸化蛋白质种类的鉴定、定量及其功能分析进行了综述,为进一步发掘与受精相关的重要生物标志物,揭示精子发育、繁殖潜能变化及受精分子机理奠定基础。     

精子发生过程中翻译后修饰的蛋白质组学研究进展

精子发生由一系列多阶段、复杂的生物学事件所组成,受到多因素的调控。精子发生过程存在翻译延迟的现象,因此转录和蛋白表达水平变化不完全一致。蛋白质的翻译后修饰作为蛋白质功能的重要调控方式,在精子发生过程中起着重要调控作用。近年来,蛋白质组学(proteomics)的发展促进了蛋白质翻译后修饰的解析和功能研究。本文综述了精子发生过程中多种翻译后修饰的蛋白质组学研究进展,并讨论了它们在精子发生、精子功能和男性生育能力中的作用以及它们在未来临床诊疗中的价值。     

TOLL样受体在睾丸炎症反应与精子发生中的功能

睾丸局部炎症反应以及系统性炎症疾病均可以损伤雄性生殖能力,近年来对于TOLL样受体(Toll-like recep-tor,TLR)调节睾丸功能的研究有了较大进展,为认识炎症反应与雄性生殖障碍之间的关系提供了新的线索。TLR介导的炎症信号通路在睾丸内除了抵御病原体外,还可以调节多种睾丸细胞的功能,从而影响精子发生。炎症对精子发生的影响主要由于循环系统和睾丸中炎症因子增多,它们可以破坏生精细胞的正常发育,损害睾丸体细胞对精子发生的正常调节。相关机理的深入研究可能为雄性不育的预防与治疗提供新的思路,本文将综述TLR介导的系统性炎症疾病及睾丸局部炎症反应干扰雄性生育的研究进展。     

检控蛋白Rad17在小鼠睾丸精子发生过程中的表达及其磷酸化变化

Rad17是细胞周期检控点信号转导过程中的一个关键检控蛋白,在DNA损伤检控和DNA复制检控中具有重要功能。但Rad17在细胞减数分裂中的检控作用还不是很清楚。因细胞减数分裂在睾丸组织中非常活跃,应用Western印迹检测Rad17在不同发育时期的小鼠睾丸组织中的表达及其磷酸化水平,并应用免疫组化的方法检测小鼠睾丸组织不同时期生殖细胞内Rad17的表达变化。结果显示Rad17在小鼠睾丸组织内高表达,而在肝、肾等组织中表达水平较低;Rad17在不同周龄的小鼠睾丸组织中均高水平表达,但在4周龄以后的小鼠睾丸组织中其磷酸化水平明显升高;免疫组化结果显示Rad17在精原细胞、精母细胞的细胞核中高表达,但在成熟精子细胞中消失。这些结果提示Rad17在小鼠睾丸生殖细胞减数分裂过程中也起重要检控作用。     

哺乳动物卵母细胞及早期胚胎蛋白质组学研究进展

雌性生殖细胞发育是动物繁殖的基石,哺乳动物卵母细胞和早期胚胎在其生长发育过程中有许多独特的现象和规律,涉及一系列蛋白质合成/降解和磷酸化等状态的动态改变。对卵母细胞分裂、成熟调控机理以及植入前胚胎发育规律的研究是发育生物学领域的一项重要课题。蛋白质组学是以细胞或组织内全部的蛋白质为研究对象,系统鉴定、定量蛋白质并研究这些蛋白质功能的科学。随着蛋白质分离、鉴定技术的快速发展,蛋白质组学为卵母细胞发生、分化、成熟以及质量控制等相关研究提供了新的方法和内容,如在蛋白质定量、修饰、定位和相互作用等方面提供其他组学技术不可获得的重要信息。这些信息将有助于揭示哺乳动物卵母细胞成熟和早期胚胎发育的分子机制,对于进一步完善卵母细胞的体外成熟培养体系,提高胚胎体外生产、体细胞克隆和转基因动物生产效率具有重要意义。     

SPAG4L在人类睾丸中的表达研究

目的:观察人类睾丸新基因SPAG4L在人类不同发育阶段睾丸及隐睾中的表达,为了解该基因在精子发生中的功能奠定基础;方法:收集流产胎儿、成年人、老年人及隐睾患者的睾丸组织,应用RT-PCR和组织原位杂交技术检测SPAG4L mRNA的表达;结果:RT-PCR和组织原位杂交技术检测结果发现,SPAG4L在胎儿睾丸中几乎检测不到,在成年及老年男性睾丸中均有高表达,主要在精母细胞和圆形精子细胞中表达;在隐睾患者的睾丸中,精母细胞大量凋亡,SPAG4L表达明显下调;结论:SPAG4L主要在精子发生减数分裂阶段表达,受生长发育调控,提示该基因可能在精子发生减数分裂阶段发挥着重要的生理功能.     

大鼠睾丸生精小管上皮精子发生周期的PAS法判定

精子发生是一个包含生殖细胞成熟分裂的连续、复杂的动态过程,不同的生精小管,或同一生精小管不同区段的生精细胞的组合、分布均不相同。本文应用PAS染色法观察了大鼠睾丸生精小管上皮中各级生精细胞在精子发生过程的形态学变化特点。参照Clermont及Russell等制定的生精上皮时相的判定标准,根据生精上皮在精子发生过程中的各级生精细胞组合分布特点,把生精上皮分为ⅩⅣ个期。通过观察精子发生过程中生精上皮细胞组合的周期性形态变化特点,对精子发生过程进行精确划分,把精子发生这一连续、复杂的动态过程静止化,具体化,可以更加准确地描述和比较不同影响因素对生精小管上皮中各级生精细胞的组织学、病理学、毒理学变化。     

中国兽类标本馆藏数量

我国兽类资源丰富,兽类物种共计12目59科254属686种。近40年来我国的兽类标本采集和馆藏数量快速增加。根据最新发表的兽类名录对19家博物馆（标本馆）兽类标本馆藏的调查结果表明,我国至少保藏兽类标本166 178号,馆藏数量排名前五位的单位分别是中国科学院昆明动物研究所、中国科学院动物研究所、四川省林业科学研究院、中国科学院西北高原生物研究所和西华师范大学,馆藏数量占比84.9%。在馆藏标本中,小型兽类占91.5%,而大中型兽类标本特别是鲸豚类很少,有待加大力度对这些类群标本进行收集与保藏。     

Regulation of GDF9 and CDKN1B expression in Tibetan sheep testes during different stages of maturity

Normal spermatogenesis is heavily dependent on the balance of germ cell proliferation, differentiation and apoptosis. Growth differentiation factor 9 (GDF9) and cyclin-dependent kinase inhibitor 1 B (CDKN1B) are strongly associated with cell cycle transition from G0/G1 to S and G2/M phase and hence regulating the growth and development of testicular germ cells and somatic cells. The current study was aimed at seeking out scientific evidence to determine if GDF9 and CDKN1B gene expression functions in the development of Tibetan sheep testes. To this end, developmental testes were derived from three-month-old (pre-puberty), one-year-old (sexual maturity), and three-year-old (adult) Tibetan sheep and then the expression and localization patterns of GDF9 and CDKN1B in these testes were evaluated using quantitative real-time PCR (qRT-PCR), Western blot and immunofluorescence. qRT-PCR and Western blot results showed that GDF9 and CDKN1B were detected in the testes throughout the different developmental stages. The abundance of GDF9 mRNA and protein in the testes of one- and three-year-old Tibetan sheep were higher than that in the testes of three-month-old Tibetan sheep; the mRNA and protein abundance of the CDKN1B gene in three-month-old Tibetan sheep testes were higher than that in the testes of the one-and three-year-old sheep. Moreover, immunofluorescence results suggested that the GDF9 protein was expressed in spermatogonia and Leydig cells, and that the CDKN1B protein was localized mainly in Leydig cells with some in the seminiferous epithelium throughout developmental stages. This indicated a novel role of the GDF9 and CDKN1B genes in Leydig cell development over and above their known roles in germ cell development. These findings have significant implications for our understanding of the molecular mechanisms of GDF9 and CDKN1B genes in Tibetan sheep spermatogenesis.     

Heat shock protein 27 expression in the human testis showing normal and abnormal spermatogenesis

Heat shock proteins (HSPs) are molecular chaperones involved in protein folding, assembly and transport, and which play critical roles in the regulation of cell growth, survival and differentiation. We set out to test the hypothesis that HSP27 protein is expressed in the human testes and its expression varies with the state of spermatogenesis. HSP27 expression was examined in 30 human testicular biopsy specimens (normal spermatogenesis, maturation arrest and Sertoli cell only syndrome, 10 cases each) using immunofluorescent methods. The biopsies were obtained from patients undergoing investigations for infertility. The seminiferous epithelium of the human testes showing normal spermatogenesis had a cell type-specific expression of HSP27. HSP27 expression was strong in the cytoplasm of the Sertoli cells, spermatogonia, and Leydig cells. Alternatively, the expression was moderate in the spermatocytes, weak in the spermatids and absent in the spermatozoa. In testes showing maturation arrest, HSP27 expression was strong in the Sertoli cells, weak in the spermatogonia, and spermatocytes. It was absent in the spermatids and Leydig cells. In Sertoli cell only syndrome, HSP27 expression was strong in the Sertoli cells and absent in the Leydig cells. We report for the first time the expression patterns of HSP27 in the human testes and show differential expression during normal spermatogenesis, indicating a possible role in this process. The altered expression of this protein in testes showing abnormal spermatogenesis may be related to the pathogenesis of male infertility.     

Poly (A) binding protein is bound to both stored and polysomal mRNAs in the mammalian testis

RNA-binding proteins that bind to the 3′ untranslated region of mRNAs play important roles in regulating gene expression. Here we examine the association between the 70 kDa poly (A) binding protein (PABP) and stored (RNP) and polysomal mRNAs during mammalian male germ cell development. PABP mRNA levels increase as germ cells enter meiosis, reaching a maximum in the early postmeiotic stages, and decreasing to a nearly nondetectable level towards the end of spermatogenesis. Most of the PABP mRNA is found in the nonpolysomal fractions of postmitochondrial extracts, suggesting that PABP mRNA is either inefficiently translated or stored as RNPs during spermatogenesis. Virtually all of the testicular PABP is bound to either polysomal or nonpolysomal mRNAs, with little, if any, free PABP detectable. Analysis of several specific mRNAs reveals PABP is bound to both stored (RNP) and translated forms of the mRNAs. Western blot analysis and immunocytochemistry indicate PABP is widespread in the mammalian testis, with maximal amounts detected in postmeiotic round spermatids. The presence of PABP in elongating spermatids, a cell type in which PABP mRNA is nearly absent, suggests that PABP is a stable protein in the later stages of male germ cell development. The high level of testicular PABP in round spermatids and in mRNPs suggests a role for PABP in the storage as well as in the subsequent translation of developmentally regulated mRNAs in the mammalian testis. © 1995 Wiley-Liss, Inc.     

Peroxisomes are present in murine spermatogonia and disappear during the course of spermatogenesis

Peroxisomes are organelles that are almost ubiquitous in eukaryotic cells. They have, however, never been described in germ cells within the testis. Since some peroxisomal diseases like Adrenoleukodystrophy are associated with reduced fertility, we have re-investigated the peroxisomal compartment of the germinal epithelium of mice using in situ hybridization, immunohistochemistry, Western blotting and immunoelectron microscopy. Within the seminiferous tubules, peroxisomes are present in Sertoli cells and in germ cells. We could show that small-sized peroxisomes of typical ultrastructure are concentrated in spermatogonia and disappear during the course of spermatogenesis. Peroxisomes of spermatogonia differ in their relative protein composition from previously described peroxisomes of interstitial cells of Leydig. Since germ cells differentiate in mouse testis in a synchronized fashion, the disappearence of peroxisomes could be a suitable model system to investigate the degradation of an organelle as part of a physiological differentiation process in higher eukaryotes.     

Stages and duration of the cycle of the seminiferous epithelium in oncilla (Leopardus tigrinus, Schreber, 1775)

Six adult Leopardus tigrinus (oncilla) were studied to characterize stages of the seminiferous epithelium cycle and its relative frequency and duration, as well as morphometric parameters of the testes. Testicular fragments were obtained (incisional biopsy), embedded (glycol methacrylate), and histologic sections examined with light microscopy. The cycle of the seminiferous epithelium was categorized into eight stages (based on the tubular morphology method). The duration of one seminiferous epithelium cycle was 9.19 d, and approximately 41.37 d were required for development of sperm from spermatogonia. On average, diameter of the seminiferous tubules was 228.29 μm, epithelium height was 78.86 μm, and there were 16.99 m of testicular tubules per gram of testis. Body weight averaged 2.589 kg, of which 0.06 and 0.04% were attributed to the testis and seminiferous tubules, respectively. In conclusion, there were eight distinct stages in the seminiferous epithelium, the length of the seminiferous epithelium cycle was close to that in domestic cats and cougars, and testicular and somatic indexes were similar to those of other carnivores of similar size.     

叶绿体蛋白质组学研究进展

蛋白质组分析是鉴定蛋白质种类和功能的有力工具之一。叶绿体作为光合作用的重要细胞器,叶绿体蛋白质组学成为了研究的热点,涉及的领域包括叶绿体的总蛋白质组学、亚细胞蛋白质组学、差异蛋白质组学和蛋白质的功能等。现主要介绍蛋白质组学的常用技术以及叶绿体蛋白质组学的最新研究进展。