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利用锌指核酸酶对虹鳟(Oncorhynchus mykiss)主性别决定基因进行可遗传靶向敲除。

Heritable targeted inactivation of the rainbow trout (Oncorhynchus mykiss) master sex-determining gene using zinc-finger nucleases.

机构信息

INRA, UR1037, LPGP, Fish Physiology and Genomics, 35000, Rennes, France.

出版信息

Mar Biotechnol (NY). 2014 Apr;16(2):243-50. doi: 10.1007/s10126-013-9546-8. Epub 2013 Oct 2.

DOI:10.1007/s10126-013-9546-8
PMID:24085607
Abstract

Gene targeting is a powerful tool for analyzing gene function. Recently, new technology for gene targeting using engineered zinc-finger nucleases (ZFNs) has been described in fish species. However, it has not yet been widely used for cold water and slow developing species, such as Salmonidae. Here, we present the results of successful ZFN-mediated disruption of the sex-determining gene sdY (sexually dimorphic on the Y chromosome) in rainbow trout (Oncorhynchus mykiss). Three pairs of ZFN mRNA targeted to different regions of the sdY gene were injected into fertilized rainbow trout eggs. Sperm from 1-year-old male founders (parental generation one or P1) carrying a ZFN-induced mutation in their germline were then used to produce F1 non-mosaic animals. In these F1 populations, we characterized 14 different mutations in the sdY gene, including one mutation leading to the deletion of leucine 43 (L43) and 13 mutations at other target sites that had different effects on the SdY protein, i.e., amino acid insertions, deletions, and frameshift mutations producing premature stop codons in the mRNA. The gonadal phenotype analysis of the F1-mutated animals revealed that the single L43 amino acid deletion did not lead to a male-to-female sex reversal, but all other mutations induced a clear ovarian phenotype. These results show that targeted gene disruption using ZFN is efficient in rainbow trout but depends on the ZFN design. We also characterized new sdY mutations resulting in male-to-female sex reversal, and we conclude that L43 seems dispensable for SdY function.

摘要

基因打靶是分析基因功能的强大工具。最近,使用工程化锌指核酸酶(ZFNs)进行基因打靶的新技术已在鱼类物种中得到描述。然而,它尚未广泛用于冷水和发育缓慢的物种,如鲑科鱼类。在这里,我们展示了成功使用 ZFN 介导破坏虹鳟(Oncorhynchus mykiss)性别决定基因 sdY(Y 染色体上的性别二态性)的结果。将三对靶向 sdY 基因不同区域的 ZFN mRNA 注射到受精的虹鳟鱼卵中。然后,使用携带生殖系中 ZFN 诱导突变的 1 岁雄性亲鱼(第一代或 P1)的精子来产生非嵌合 F1 动物。在这些 F1 群体中,我们鉴定了 sdY 基因中的 14 种不同突变,包括导致亮氨酸 43(L43)缺失的突变和其他 13 个靶位点的突变,这些突变对 SdY 蛋白有不同的影响,即氨基酸插入、缺失和导致 mRNA 产生提前终止密码子的移码突变。F1 突变动物的性腺表型分析表明,单个 L43 氨基酸缺失不会导致雄性到雌性的性别反转,但所有其他突变都诱导了明显的卵巢表型。这些结果表明,使用 ZFN 进行靶向基因敲除在虹鳟中是有效的,但取决于 ZFN 的设计。我们还鉴定了导致雄性到雌性性别反转的新 sdY 突变,并得出结论,L43 似乎对 SdY 功能不是必需的。

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