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抗氧化维生素和溶血磷脂对于在器官培养条件下诱导小鼠精子发生至关重要。

Antioxidant vitamins and lysophospholipids are critical for inducing mouse spermatogenesis under organ culture conditions.

机构信息

Department of Urology, Yokohama City University Graduate School of Medicine, Yokohama, Japan.

Laboratory of Biopharmaceutical and Regenerative Sciences, Institute of Molecular Medicine and Life Science, Yokohama City University Association of Medical Science, Yokohama, Japan.

出版信息

FASEB J. 2020 Jul;34(7):9480-9497. doi: 10.1096/fj.202000245R. Epub 2020 May 31.

Abstract

In vitro mouse spermatogenesis using a classical organ culture method became possible by supplementing basal culture medium with only the product of bovine serum albumin purified by chromatography (AlbuMAX), which indicated that AlbuMAX contained every chemical factor necessary for mouse spermatogenesis. However, since the identity of these factors was unclear, improvements in culture media and our understanding of the nutritional and signal substances required for spermatogenesis were hindered. In the present study, chemically defined media (CDM) without AlbuMAX was used to evaluate each supplementary factor and their combinations for the induction of spermatogenesis. Similar to in vivo conditions, retinoic acid, triiodothyronine (T ), and testosterone (T) were needed. Based on differences in spermatogenic competence between AlbuMAX, fetal bovine serum, and adult bovine serum, we identified α-tocopherol, which strongly promoted spermatogenesis when combined with ascorbic acid and glutathione. Differences were also observed in the abilities of lipids extracted from AlbuMAX using two different methods to induce spermatogenesis. This led to the identification of lysophospholipids, particularly lysophosphatidylcholine, lysophosphatidic acid, and lysophosphatidylserine, as important molecules for spermatogenesis. New CDM formulated based on these results induced and promoted spermatogenesis as efficiently as AlbuMAX-containing medium. In vitro spermatogenesis with CDM may provide a unique experimental system for research on spermatogenesis that cannot be performed in in vivo experiments.

摘要

利用经典的器官培养方法,在基础培养基中仅添加经色谱法纯化的牛血清白蛋白产物(AlbuMAX),即可实现体外小鼠精子发生,这表明 AlbuMAX 含有精子发生所需的每一种化学因素。然而,由于这些因素的身份尚不清楚,培养基的改进以及我们对精子发生所需营养和信号物质的理解受到了阻碍。在本研究中,使用不含 AlbuMAX 的化学定义培养基(CDM)来评估诱导精子发生的每种补充因子及其组合。与体内条件相似,需要视黄酸、三碘甲状腺原氨酸(T)和睾酮(T)。基于 AlbuMAX、胎牛血清和成年牛血清在精子发生能力上的差异,我们确定了α-生育酚,当与抗坏血酸和谷胱甘肽结合使用时,可强烈促进精子发生。用两种不同方法从 AlbuMAX 中提取的脂质诱导精子发生的能力也存在差异。这导致鉴定出溶血磷脂,特别是溶血磷脂酰胆碱、溶血磷脂酸和溶血磷脂酰丝氨酸,作为精子发生的重要分子。基于这些结果制定的新 CDM 有效地诱导和促进了精子发生,与含有 AlbuMAX 的培养基一样高效。基于 CDM 的体外精子发生可能为无法在体内实验中进行的精子发生研究提供独特的实验系统。

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