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精子发生过程中粘着斑激酶(FAK)功能与调控的新见解。

New insights into FAK function and regulation during spermatogenesis.

作者信息

Gungor-Ordueri N Ece, Mruk Dolores D, Wan Hin-ting, Wong Elissa W P, Celik-Ozenci Ciler, Lie Pearl P Y, Cheng C Yan

机构信息

The Mary M. Wohlford Laboratory for Male Contraceptive Research, Center for Biomedical Research, Population Council, New York, USA.

Department of Histology and Embryology, Faculty of Medicine, Akdeniz University, Antalya, Turkey.

出版信息

Histol Histopathol. 2014 Aug;29(8):977-89. doi: 10.14670/HH-29.977. Epub 2014 Feb 27.

Abstract

Germ cell transport across the seminiferous epithelium during the epithelial cycle is crucial to spermatogenesis, although molecular mechanism(s) that regulate these events remain unknown. Studies have shown that spatiotemporal expression of crucial regulatory proteins during the epithelial cycle represents an efficient and physiologically important mechanism to regulate spermatogenesis without involving de novo synthesis of proteins and/or expression of genes. Herein, we critically review the role of focal adhesion kinase (FAK) in coordinating the transport of spermatids and preleptotene spermatocytes across the epithelium and the BTB, respectively, along the apical ectoplasmic specialization (ES) - blood-testis barrier - basement membrane (BM) functional axis during spermatogenesis. In the testis, p-FAK-Tyr³⁸⁷ and p-FAK-Tyr⁴⁰⁷ are spatiotemporally expressed during the epithelial cycle at the actin-rich anchoring junction known as ES, regulating cell adhesion at the Sertoli-spermatid (apical ES) and Sertoli cell-cell (basal ES) interface. Phosphorylated forms of FAK exert their effects by regulating the homeostasis of F-actin at the ES, mediated via their effects on actin polymerization so that microfilaments are efficiently re-organized, such as from their "bundled" to "de-bundled/branched" configuration and vice versa during the epithelial cycle to facilitate the transport of: (i) spermatids across the epithelium, and (ii) preleptotene spermatocytes across the BTB. In summary, p-FAK-Tyr⁴⁰⁷ and p-FAK-Tyr³⁸⁷ are important regulators of spermatogenesis which serve as molecular switches that turn "on" and "off" adhesion function at the apical ES and the basal ES/BTB, mediated via their spatiotemporal expression during the epithelial cycle. A hypothetical model depicting the role of these two molecular switches is also proposed.

摘要

在生精上皮周期中,生殖细胞穿过生精上皮对于精子发生至关重要,尽管调节这些过程的分子机制仍不清楚。研究表明,上皮周期中关键调节蛋白的时空表达代表了一种高效且生理上重要的机制,可在不涉及蛋白质从头合成和/或基因表达的情况下调节精子发生。在此,我们批判性地综述了粘着斑激酶(FAK)在精子发生过程中,分别沿着顶端胞质特化(ES)-血睾屏障-基底膜(BM)功能轴,协调精子细胞和前细线期精母细胞穿过上皮和血睾屏障的运输中的作用。在睾丸中,p-FAK-Tyr³⁹⁷和p-FAK-Tyr⁸⁶¹在生精上皮周期中,于富含肌动蛋白的锚定连接即ES处进行时空表达,调节支持细胞-精子细胞(顶端ES)和支持细胞-支持细胞(基底ES)界面处的细胞粘附。FAK的磷酸化形式通过调节ES处F-肌动蛋白的稳态发挥作用,这是通过它们对肌动蛋白聚合的影响介导的,以便微丝在生精上皮周期中能有效地重新组织,比如从“成束”到“解束/分支”构型,反之亦然,以促进:(i)精子细胞穿过上皮,以及(ii)前细线期精母细胞穿过血睾屏障。总之,p-FAK-Tyr⁸⁶¹和p-FAK-Tyr³⁹⁷是精子发生的重要调节因子,它们作为分子开关,通过在生精上皮周期中的时空表达,开启和关闭顶端ES以及基底ES/血睾屏障处的粘附功能。本文还提出了一个描述这两个分子开关作用的假设模型。

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