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配子生成素结合蛋白1(GGNBP1)在小鼠精子发生过程中线粒体形态发生中的一种新的潜在作用。

A novel potential role for gametogenetin-binding protein 1 (GGNBP1) in mitochondrial morphogenesis during spermatogenesis in mice.

作者信息

Aihara Takeshi, Nakamura Nobuhiro, Honda Shinji, Hirose Shigehisa

机构信息

Department of Biological Sciences, Tokyo Institute of Technology, Yokohama, Japan.

出版信息

Biol Reprod. 2009 Apr;80(4):762-70. doi: 10.1095/biolreprod.108.074013. Epub 2009 Feb 4.

DOI:10.1095/biolreprod.108.074013
PMID:19208545
Abstract

Mitochondria are dynamic organelles that undergo fusion, fission, and translocation. The dynamic property is essential for establishing energy-consuming biological processes including cellular differentiation. Early ultrastructural studies have shown that mitochondria of mammalian spermatogenic cells dramatically change their number, size, distribution, and internal structure. However, its regulatory mechanism is largely unknown. In course of searching for molecules involved in the mitochondrial morphogenesis in spermatogenesis, we identified mouse gametogenetin-binding protein 1 (GGNBP1), a DUF1055 domain-containing protein of unknown function, as a mitochondrial protein. When GGNBP1 was expressed in COS7 cells, it was localized in the intermembrane space and induced an extensive fragmentation of mitochondria in the manner dependent on the activity of the mitochondrial fission factor DNM1L. Deletion mutant analyses demonstrated that the N-terminal region is required for its mitochondrial targeting and that the C-terminal region including the DUF1055 domain is responsible for the mitochondrial fragmentation activity. Immunohistochemistry of mouse testis revealed that GGNBP1 is highly expressed in the late pachytene spermatocytes and early round spermatids. However, a subcellular fractionation study showed that it is localized to not only mitochondria but also other membranous compartments in vivo. These results suggest that GGNBP1 is involved in spermatogenesis by modifying mitochondrial dynamics and morphology.

摘要

线粒体是动态细胞器,会经历融合、裂变和易位过程。这种动态特性对于建立包括细胞分化在内的耗能生物过程至关重要。早期的超微结构研究表明,哺乳动物生精细胞的线粒体在数量、大小、分布和内部结构上会发生显著变化。然而,其调控机制在很大程度上尚不清楚。在寻找参与精子发生过程中线粒体形态发生的分子时,我们鉴定出小鼠配子生成素结合蛋白1(GGNBP1),一种功能未知的含DUF1055结构域的蛋白质,它是一种线粒体蛋白。当GGNBP1在COS7细胞中表达时,它定位于线粒体内膜间隙,并以依赖线粒体裂变因子DNM1L活性的方式诱导线粒体广泛碎片化。缺失突变分析表明,其N端区域是其线粒体靶向所必需的,而包括DUF1055结构域的C端区域负责线粒体碎片化活性。小鼠睾丸的免疫组织化学显示,GGNBP1在粗线期晚期精母细胞和早期圆形精子细胞中高表达。然而,亚细胞分级分离研究表明,它在体内不仅定位于线粒体,还定位于其他膜性区室。这些结果表明,GGNBP1通过改变线粒体动力学和形态参与精子发生。

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