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造血移植的小鼠模型:转基因绿色荧光蛋白品系的局限性及一种用于分析红系嵌合现象的高效液相色谱方法

Mouse models of hematopoietic engraftment: limitations of transgenic green fluorescent protein strains and a high-performance liquid chromatography approach to analysis of erythroid chimerism.

作者信息

Spangrude Gerald J, Cho Scott, Guedelhoefer Otto, Vanwoerkom Ryan C, Fleming William H

机构信息

Department of Medicine, University of Utah, 30 N 1900 East, Salt Lake City, 84132-2408, USA.

出版信息

Stem Cells. 2006 Sep;24(9):2045-51. doi: 10.1634/stemcells.2006-0013. Epub 2006 May 11.

DOI:10.1634/stemcells.2006-0013
PMID:16690777
Abstract

Transgenic mouse strains ubiquitously expressing green fluorescent protein (GFP) have enabled investigators to develop in vivo transplant models that can detect donor contributions to many different tissues. However, most GFP transgenics lack expression of the reporter in the erythroid lineage. We evaluated expression of GFP in the bone marrow of the OsbY01 transgenic mouse (B6-GFP) in the context of CD71 and TER-119 expression and found that GFP fluorescence is lost prior to the basophilic erythroblast stage of development. However, platelets in B6-GFP mice were found to be uniformly positive for GFP. We therefore used the GFP transgenic model in combination with allelic variants of CD45 and the hemoglobin beta (Hbb) chain to develop a model system that allows all blood lineages to be followed in a mouse model of bone marrow transplantation (BMT). To detect Hbb variant molecules, we developed a new protocol based on high-performance liquid chromatography that is sensitive and precise, allowing rapid and quantitative analysis of erythroid chimerism. Platelet and leukocyte engraftment were detected by flow cytometry. BMT into sublethally irradiated (4 Gy) recipients demonstrated the failure of B6-GFP-derived cells to engraft relative to B6-CD45(a)-derived cells, suggesting that an immune barrier may prevent efficient engraftment of the transgenic cells in a setting of minimal ablation. These results establish limitations in the use of transgenic GFP expression as a donor marker in transplantation models.

摘要

广泛表达绿色荧光蛋白(GFP)的转基因小鼠品系使研究人员能够建立体内移植模型,用于检测供体对多种不同组织的贡献。然而,大多数GFP转基因小鼠在红系谱系中缺乏报告基因的表达。我们在CD71和TER-119表达的背景下评估了OsbY01转基因小鼠(B6-GFP)骨髓中GFP的表达,发现GFP荧光在嗜碱性成红细胞发育阶段之前就消失了。然而,发现B6-GFP小鼠的血小板对GFP呈均匀阳性。因此,我们将GFP转基因模型与CD45等位基因变体和血红蛋白β(Hbb)链结合使用,开发了一个模型系统,该系统可在骨髓移植(BMT)小鼠模型中追踪所有血液谱系。为了检测Hbb变体分子,我们基于高效液相色谱法开发了一种新方案,该方案灵敏且精确,能够对红系嵌合进行快速定量分析。通过流式细胞术检测血小板和白细胞的植入情况。将BMT移植到亚致死剂量照射(4 Gy)的受体中,结果表明相对于B6-CD45(a)来源的细胞,B6-GFP来源的细胞植入失败,这表明在最小程度消融的情况下,免疫屏障可能会阻止转基因细胞的有效植入。这些结果揭示了在移植模型中使用转基因GFP表达作为供体标记的局限性。

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Mouse models of hematopoietic engraftment: limitations of transgenic green fluorescent protein strains and a high-performance liquid chromatography approach to analysis of erythroid chimerism.造血移植的小鼠模型:转基因绿色荧光蛋白品系的局限性及一种用于分析红系嵌合现象的高效液相色谱方法
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