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精子发生过程中透明带结合蛋白IAM38的起源与组装

The origin and assembly of a zona pellucida binding protein, IAM38, during spermiogenesis.

作者信息

Yu Yang, Vanhorne Judy, Oko Richard

机构信息

Department of Anatomy and Cell Biology, Queen's University, Kingston, Ontario, Canada.

出版信息

Microsc Res Tech. 2009 Aug;72(8):558-65. doi: 10.1002/jemt.20696.

DOI:10.1002/jemt.20696
PMID:19204925
Abstract

IAM38 is the most prominent protein of the inner acrosomal membrane extracellular coat (IAMC) of spermatozoa. It is retained by the inner acrosomal membrane after the acrosome reaction and is implicated in secondary sperm-zona binding (Yu et al., Dev Biol2006;290:32-43). Its gene knockout, Zpbp1(-/-), prevents acrosome compaction and leads to acrosome fragmentation and sterility in male mice (Lin et al., Mol Cell Biol2007;27:6794-6805). Because of this protein's important role in acrosomal formation and fertilization, the authors were interested in tracing its origin and expression during spermiogenesis. The authors reasoned that a detailed immunocytochemical investigation, utilizing anti-IAM38 antibodies as probes at the ultrastructural level, could reveal the processes involved in assembly of the IAMC and the compaction of the acrosome. High level of the IAM38 transcript was already detectable at postnatal day 20, corresponding to the time in mouse testis development when round spermatids first appear and acrosomal formation is initiated. IAM38 protein was first seen during this time (Golgi phase of spermiogenesis) within the dense core of the proacrosomal granules (PG) of round spermatids. After PG fusion to form the acrosomic vesicle (AV) the immunoreactivity was concentrated in the centrally located acrosomic granule (AG) of the AV, until acrosomal-nuclear docking occurred. Subsequently, in the cap phase, IAM38 migrated from the AG to the extracellular side of the acrosomal membrane, eventually disappearing altogether from the AG. During the elongation phase IAM38 labeling disappeared from the outer acrosomal membrane (OAM) in the apical and principal segments of the acrosome but remained lining the OAM in the equatorial segment (ES) as well as the entire IAM of the acrosome. Compaction of the ES in the maturation phase of spermiogenesis coincided with the IAM38-labeled extracellular coat of the inner and outer acrosomal membranes coming together in close proximity of each other to form a "zipper-like" structure found in the ES of mature spermatozoa. In summary, the results set a precedent, showing for the first time that glycoproteins, which originate in the acrosomic granule can be transferred to the acrosomal membrane during acrosome formation. Furthermore, the localization of IAM38 on the extracellular side of both the inner and outer acrosomal membrane during the cap phase of acrosomal development supports the role of this prominent protein in acrosomal compaction.

摘要

IAM38是精子顶体内膜细胞外被(IAMC)中最主要的蛋白质。顶体反应后,它保留在顶体内膜上,并参与精子与透明带的二次结合(Yu等人,《发育生物学》2006年;290:32 - 43)。其基因敲除小鼠Zpbp1(-/-),会阻止顶体压实,导致雄性小鼠顶体破碎和不育(Lin等人,《分子细胞生物学》2007年;27:6794 - 6805)。由于这种蛋白质在顶体形成和受精过程中具有重要作用,作者们对追踪其在精子发生过程中的起源和表达感兴趣。作者们推断,利用抗IAM38抗体作为探针,在超微结构水平上进行详细的免疫细胞化学研究,可能揭示IAMC组装和顶体压实所涉及的过程。在出生后第20天就已经可以检测到高水平的IAM38转录本,这与小鼠睾丸发育过程中圆形精子细胞首次出现并开始顶体形成的时间相对应。在这个时期(精子发生的高尔基体期),首次在圆形精子细胞的前顶体颗粒(PG)的致密核心中看到IAM38蛋白。PG融合形成顶体小泡(AV)后,免疫反应性集中在AV中央的顶体颗粒(AG)中,直到顶体与细胞核对接发生。随后,在帽期,IAM38从AG迁移到顶体膜的细胞外侧,最终从AG中完全消失。在伸长阶段,IAM38标记从顶体顶端和主体段的顶体外膜(OAM)消失,但在赤道段(ES)以及顶体的整个内膜(IAM)中仍衬于OAM。精子发生成熟阶段ES的压实与顶体内外膜上IAM38标记的细胞外被彼此紧密靠近并形成成熟精子ES中发现的“拉链样”结构同时发生。总之,这些结果开创了先例,首次表明起源于顶体颗粒的糖蛋白在顶体形成过程中可以转移到顶体膜上。此外,在顶体发育帽期,IAM38在顶体内外膜细胞外侧的定位支持了这种重要蛋白质在顶体压实中的作用。

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