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从单个斑马鱼胚胎中建立细胞系。

Establishment of cell lines from individual zebrafish embryos.

机构信息

Institute for Biological and Chemical Systems-Biological Information Processing (IBCS-BIP), Karlsruhe Institute of Technology, Germany.

Centre for Organismal Studies Heidelberg, Ruprecht-Karls-Universität Heidelberg, Germany.

出版信息

Lab Anim. 2023 Oct;57(5):518-528. doi: 10.1177/00236772231157162. Epub 2023 Mar 9.

DOI:10.1177/00236772231157162
PMID:36896487
Abstract

With the increasing use of fish as model species for research, cell cultures derived from caudal fin explants as well as pre-hatching stage embryos have provided powerful tools that can complement or serve as an ethically more acceptable alternative to live animal experiments. The widely-used protocols to establish these lines require, as a starting point, homogeneous pools of embryos or viable adult fish which are large enough for collecting sufficient fin tissue. This excludes the use of fish lines with adverse phenotypes or lines that exhibit mortality at early developmental stages and so can only be propagated as heterozygotes. Specifically, when no visually overt mutant phenotype is detectable for identifying homozygous mutants at early embryonic stages, it is then impossible to sort pools of embryos with the same genotypes to generate cell lines from the progeny of a heterozygote in-cross. Here, we describe a simple protocol to generate cell lines on a large scale starting from individual early embryos that can subsequently be genotyped by polymerase chain reaction. This protocol should help to establish fish cell culture models as a routine approach for the functional characterization of genetic changes in fish models such as the zebrafish. Furthermore, it should contribute to a reduction of experiments which are ethically discouraged to avoid pain and distress.

摘要

随着鱼类作为研究模型的应用日益增多,源自尾鳍外植体和孵化前胚胎的细胞培养已提供了强有力的工具,可作为活体动物实验的补充或更符合伦理的替代方法。广泛使用的建立这些细胞系的方案需要作为起点的均一胚胎或有活力的成年鱼类的池,其大小足以收集足够的鳍组织。这排除了使用具有不良表型或在早期发育阶段表现出死亡率的鱼类品系的可能性,因此只能作为杂合体进行繁殖。具体来说,当在早期胚胎阶段无法检测到明显的视觉突变表型来鉴定纯合突变体时,就不可能对具有相同基因型的胚胎池进行分类,以从杂合体自交的后代中生成细胞系。在这里,我们描述了一种从单个早期胚胎开始大规模生成细胞系的简单方案,随后可以通过聚合酶链反应对其进行基因分型。该方案应有助于建立鱼类细胞培养模型作为鱼类模型(如斑马鱼)中遗传变化的功能特征的常规方法。此外,它有助于减少因避免疼痛和痛苦而受到伦理劝阻的实验。

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