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精子在小鼠曲细精管中的释放和运输的三维分析和体内成像。

Three-dimensional analysis and in vivo imaging for sperm release and transport in the murine seminiferous tubule.

机构信息

Department of Anatomy, Tokyo Medical University, Tokyo, Japan.

Department of Histology and Cell Biology, Graduate School of Medical Sciences, Kanazawa University, Kanazawa, Japan.

出版信息

Reproduction. 2022 May 23;164(1):9-18. doi: 10.1530/REP-21-0400.

Abstract

Spermatozoa released from Sertoli cells must be transported to the epididymis. However, the mechanism of the luminal flow in seminiferous tubules has remained unclear to date. Therefore, in this study, we investigated luminal flow and movements in the seminiferous tubules by three-dimensional analysis and in vivo imaging. Serial 5-μm-thick mouse testicular sections at 50-µm-intervals were prepared and stained by Periodic Acid-Schiff-hematoxylin. After three-dimensional reconstruction of the seminiferous tubules, the localization of the released spermatozoa and the stages observed in the sections were recorded in each reconstructed tubule. Luminal movements in the seminiferous tubules were observed by in vivo imaging using a fluorescent-reporter mouse and two-photon excitation microscopy system. Spermatozoa without contact to the seminiferous epithelium were not accumulated toward the rete testis. Additionally, such spermatozoa were found on their way not only to the most proximal rete testis but also a more distant rete testis from any stage VIII seminiferous epithelia. In vivo imaging demonstrated that the direction of the flagella of spermatozoa attached to the seminiferous epithelium was repeatedly reversed. The epithelium at the inner curve of the seminiferous tubule was shaken more actively and had fewer spermatozoa attached compared with the epithelium at the outer curve. Our results hence suggest that the luminal flow in the seminiferous tubules is repeatedly reversed and that this physical force helps spermatozoa to be released from Sertoli cells. In brief: Spermatozoa are released from Sertoli cells and flow in the seminiferous tubule to the rete testis. Our results suggest that the luminal flow in the tubules is repeatedly reversed and that this physical force helps spermatozoa release from the Sertoli cells.

摘要

从支持细胞中释放的精子必须运输到附睾。然而,迄今为止,曲细精管内管腔流动的机制仍不清楚。因此,在这项研究中,我们通过三维分析和体内成像研究了曲细精管内的管腔流动和运动。每隔 50μm 制备并染色 5μm 厚的小鼠睾丸连续切片,通过过碘酸希夫-苏木精染色。对曲细精管进行三维重建后,记录每个重建管中的精子释放位置和切片中观察到的阶段。使用荧光报告小鼠和双光子激发显微镜系统进行体内成像,观察曲细精管内的管腔运动。没有与曲细精管上皮接触的精子不会聚集到睾丸网。此外,这些精子不仅在向最靠近的睾丸网移动,而且在远离任何 8 期曲细精管上皮的更远的睾丸网移动。体内成像显示,附着在曲细精管上皮的精子的鞭毛方向反复反转。与外曲线的上皮相比,曲细精管内曲线的上皮更活跃地摇动,附着的精子更少。因此,我们的结果表明,曲细精管内的管腔流反复反转,这种物理力有助于精子从支持细胞中释放。简而言之:精子从支持细胞中释放出来并在曲细精管中流向睾丸网。我们的结果表明,管腔内的流动反复反转,这种物理力有助于精子从支持细胞中释放。

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