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Cryopreservation of chicken primordial germ cells by vitrification and slow freezing: A comparative study

机译:通过玻璃化和缓慢冻结鸡原毒细胞的冷冻保存:比较研究

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摘要

In the present study, we compare a classical slow freezing (SLF) method and an aseptic vitrification (Vitrif) technique to cryopreserve a stable primordial germ cell (PGCs) line issued from the Ardennaise chicken breed. Viability immediately after warming was close to 80% and did not differ between the two cryopreservation methods. Proliferation tended to be slower for both cryopreservation methods compared with controls, but the difference was significant only for Vitrif. No difference was found between the two methods after flow cytometry analysis of stage-specific embryonic antigen-1 expression and reverse transcription-polymerase chain reaction on several factors related to PGC phenotype. After 1 week in culture, all cryopreserved cells reached controls' main morphologic and expanding (viability/proliferation) features. However, SLF generated more unwanted cells clusters than Vitrif. After injection of the PGCs into recipient embryos, vitrified PGCs reported a clear, yet not significant, tendency to colonize the gonad at a higher rate than slow frozen PGCs. SLF in cryovials remains simple, inexpensive, and less technically demanding than Vitrif. Nevertheless, the intrinsic advantages of our aseptic Vitrif method and the present study suggest that this should be considered as safer than classical SLF for cryopreserving chicken PGCs. (C) 2016 Elsevier Inc. All rights reserved.
机译:在本研究中,我们比较古典慢冻结(SLF)方法和无菌玻璃化(VITRIF)技术,以冷冻从Ardennaise鸡品种发出的稳定原始生殖细胞(PGCS)线。升温后立即的活力接近80%,两种冷冻保存方法之间没有区别。与对照相比,冷冻保存方法的增殖趋于较慢,但差异仅为vitrif而显着。在阶段特异性胚胎抗原-1表达和逆转录聚合酶链反应的几种与PGC表型相关的因素的两种方法之间没有发现差异。在培养1周后,所有冷冻保存细胞达到对照对照的主要形态和扩张(活力/增殖)特征。然而,SLF产生比VITRIF更多的不需要的细胞簇。在将PGC注入受体胚胎后,vitrized PGCS报告了澄清但不显着,以比缓慢冷冻的PGC的速率更高的速率殖民。低级SLF仍然简单,廉价且较少的技术上要求苛刻。然而,我们无菌vitrif方法的内在优点和本研究表明,对于冷冻保存鸡PGC,这应该被认为是比古典SLF更安全。 (c)2016年Elsevier Inc.保留所有权利。

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