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In vitro spermatogenesis: A century-long research journey, still half way around

机译:体外精子发生:一个世纪长的研究旅程,仍然是半途

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摘要

Background: Spermatogenesis is one of the most complicated cellular differentiation processes in a body. Researchers struggled to find and develop a micro-environmental condition that can support the process in vitro. Such endeavors can be traced back to a century ago and are yet continuing.Methods: Reports on in vitro spermatogenesis and related works were selected and classified into four categories based on the method used; organ culture, tubule culture, cell culture, and 3-dimensional cell culture methods. Each report was critically reviewed from the present point of view by authors who have been working on in vitro spermatogenesis with organ culture method over a decade. Results: The organ culture method has the longest history and is the most successful method, which produced fertile mouse sperm from spermatogonial stem cells. Formulation of the medium was a key factor, most importantly serum-derived substances. However, factors in the serum that induce and support spermatogenesis in the cultured tissue remain to be identified. In addition, the success of mouse spermatogenesis is yet to be applied to other animals. On looking into the history of cell culture method, it became clear that Sertoli cells as feeder cells play an important role. Even with Sertoli cells, however, spermatogenic development has been limited to small parts of spermatogenesis, a segmented period of meiotic prophase for instance. Recent developments of organoid or 3-dimensional culture techniques are promising but they still need further refinements.Conclusion: The study of in vitro spermatogenesis progressed significantly over the last century. We need more work, however, to establish a culture system that can induce and maintain complete spermatogenesis of many if not all mammalian species.
机译:背景:精子发生是体内最复杂的细胞分化过程之一。研究人员努力发现并开发一种可在体外支持该过程的微观环境条件。这种努力可以追溯到一个世纪前,但尚未继续。方法:选择有关体外精子发生和相关工程的报告,并根据所用方法分为四类;器官培养,小管培养,细胞培养和三维细胞培养方法。每份报告都从本次审查了一直在十年内与器官培养方法致力于体外精子的作者。结果:器官培养方法具有最长的历史,是最成功的方法,从精牙科干细胞中产生肥沃的小鼠精子。培养基的制剂是一个关键因素,最重要的是血清衍生的物质。然而,诱导和支持培养组织中诱导和支持精子发生的血清中的因素仍然被鉴定。此外,小鼠精子发生的成功尚未适用于其他动物。在调查细胞培养方法的历史上,显然塞托细胞随着饲养细胞发挥重要作用。然而,即使与塞托罗里细胞一样,精子发育也限于精子发生的小部分,例如减数分裂的PERHASHASE。有机体或三维培养技术的最新发展是有前途的,但它们仍然需要进一步的改进。结论:在上个世纪的体外精子发生的研究进展显着。然而,我们需要更多的工作,建立一种培养系统,可以诱导和保持许多哺乳动物种类的完全精子发生。

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