棘牙鲆远洋受精卵中原始生殖细胞的可视化。

R. Goto, Taiju Saito, Y. Kawakami, Tomoe Kitauchi, Misae Takagi, T. Todo, K. Arai, E. Yamaha
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引用次数: 16

摘要

原始生殖细胞(PGCs)在胚胎发生早期出现,并通过卵发生或精子发生分化为配子。通过注射附着在斑马鱼nanos3 (zf-nos3) 3'非翻译区(3' utr)上的荧光蛋白基因融合产物转录的RNA,可以观察硬骨鱼PGCs。尽管该方法已广泛应用于硬骨鱼PGCs,但由于显微注射技术的困难,在具有硬绒毛膜的卵的远洋物种中可视化PGCs更加困难。在这项研究中,我们开发了一种可靠的显微注射受精卵的方法,在一个远洋物种,barfin比目鱼。使用带有收缩“制动器”的微针,我们能够将gfp-nos3 3'UTR mRNA引入胚胎,并确定PGCs的起源和迁移途径。我们还分离了barfin flder nos3 (bf-nos3)基因,并与斑马鱼的3'UTR序列进行了比较。bf-nos3序列的3′utr比zf-nos3长。然而,注射gfp-bf-nos3 3'UTR mRNA后,斑马鱼和斑马鱼的PGCs也可见。这些结果表明nos3的功能在这些物种之间是保守的,而不考虑序列差异。用gfp-nos3 mRNA标记PGCs的方法将为研究多种海洋鱼类胚胎中PGC的发育提供一种手段。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Visualization of primordial germ cells in the fertilized pelagic eggs of the barfin flounder Verasper moseri.
Primordial germ cells (PGCs) appear during early embryogenesis and differentiate into gametes through oogenesis or spermatogenesis. Teleost PGCs can be visualized by injecting RNA transcribed from the fusion product of a fluorescent protein gene attached to the 3' untranslated region (3'UTR) of zebrafish nanos3 (zf-nos3). Although this method has been widely applied to teleost PGCs, the visualization of PGCs in pelagic species that have eggs with a hard chorion is more problematic due to the technical difficulty of microinjection into their eggs. In this study, we developed a reliable method for microinjection of fertilized eggs in a pelagic species, the barfin flounder. Using a microneedle with a constriction "brake", we were able to introduce gfp-nos3 3'UTR mRNA into embryos and to determine the origin and migration route of PGCs. We also isolated the barfin flounder nos3 (bf-nos3) gene to compare its 3'UTR sequence with that of zebrafish. The 3'UTR of the bf-nos3 sequence was longer than that of zf-nos3. However, PGCs were also visualized after injection of gfp-bf-nos3 3'UTR mRNA both in zebrafish and barfin flounder. These results suggest that the function of nos3 is conserved between these species regardless of the sequence differences. The method developed here for labeling PGCs with gfp-nos3 mRNA will provide a means to study PGC development in the embryos of a wide range of marine fish species.
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