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Generation of a Stable Transgenic Swine Model Expressing a Porcine Histone 2B-eGFP Fusion Protein for Cell Tracking and Chromosome Dynamics Studies

机译:表达猪组蛋白2B-eGFP融合蛋白的稳定转基因猪模型的产生用于细胞跟踪和染色体动力学研究

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摘要

Transgenic pigs have become an attractive research model in the field of translational research, regenerative medicine, and stem cell therapy due to their anatomic, genetic and physiological similarities with humans. The development of fluorescent proteins as molecular tags has allowed investigators to track cell migration and engraftment levels after transplantation. Here we describe the development of two transgenic pig models via SCNT expressing a fusion protein composed of eGFP and porcine Histone 2B (pH2B). This fusion protein is targeted to the nucleosomes resulting a nuclear/chromatin eGFP signal. The first model (I) was generated via random insertion of pH2B-eGFP driven by the CAG promoter (chicken beta actin promoter and rabbit Globin poly A; pCAG-pH2B-eGFP) and protected by human interferon-β matrix attachment regions (MARs). Despite the consistent, high, and ubiquitous expression of the fusion protein pH2B-eGFP in all tissues analyzed, two independently generated Model I transgenic lines developed neurodegenerative symptoms including Wallerian degeneration between 3–5 months of age, requiring euthanasia. A second transgenic model (II) was developed via CRISPR-Cas9 mediated homology-directed repair (HDR) of IRES-pH2B-eGFP into the endogenous β-actin (ACTB) locus. Model II transgenic animals showed ubiquitous expression of pH2B-eGFP on all tissues analyzed. Unlike the pCAG-pH2B-eGFP/MAR line, all Model II animals were healthy and multiple pregnancies have been established with progeny showing the expected Mendelian ratio for the transmission of the pH2B-eGFP. Expression of pH2B-eGFP was used to examine the timing of the maternal to zygotic transition after IVF, and to examine chromosome segregation of SCNT embryos. To our knowledge this is the first viable transgenic pig model with chromatin-associated eGFP allowing both cell tracking and the study of chromatin dynamics in a large animal model.
机译:由于转基因猪与人体的解剖学,遗传学和生理学相似性,它们已成为转化研究,再生医学和干细胞治疗领域的一种有吸引力的研究模型。荧光蛋白作为分子标签的发展已使研究人员能够追踪移植后的细胞迁移和植入水平。在这里,我们描述了通过SCNT表达由eGFP和猪组蛋白2B(pH2B)组成的融合蛋白的两个转基因猪模型的发展。该融合蛋白靶向核小体,产生核/染色质eGFP信号。通过随机插入由CAG启动子驱动的pH2B-eGFP(鸡β肌动蛋白启动子和兔Globin poly A; pCAG-pH2B-eGFP)并受到人干扰素-β基质附着区(MARs)保护的第一个模型(I) 。尽管在所有分析过的组织中融合蛋白pH2B-eGFP始终一致,高表达无处不在,但两个独立产生的I型转基因品系在3到5个月大时出现神经退行性症状,包括Wallerian变性,需要安乐死。通过IRES-pH2B-eGFP的CRISPR-Cas9介导的同源直接修复(HDR)将第二个转基因模型(II)开发到内源性β-肌动蛋白(ACTB)基因座中。 II型转基因动物在分析的所有组织上均普遍存在pH2B-eGFP表达。与pCAG-pH2B-eGFP / MAR系不同,所有II型动物都是健康的,并且已经建立了多胎妊娠,其后代显示出预期的孟德尔比率对pH2B-eGFP的传播。 pH2B-eGFP的表达用于检查体外受精后母体向合子转变的时间,并检查SCNT胚胎的染色体分离。据我们所知,这是第一个具有染色质相关eGFP的可行转基因猪模型,可在大型动物模型中进行细胞追踪和染色质动力学研究。

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