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生成表达 CD45.1 表位的 C57BL/6J 小鼠品系,以改善造血干细胞植入和过继细胞转移实验。

Generation of a C57BL/6J mouse strain expressing the CD45.1 epitope to improve hematopoietic stem cell engraftment and adoptive cell transfer experiments.

机构信息

CIRI, INSERM U1111, Université Claude Bernard Lyon 1, CNRS UMR 5308, École Normale Supérieure de Lyon, Université de Lyon, Lyon, France.

SFR BioSciences, Plateau de Biologie Expérimentale de la Souris (AniRA-PBES), Ecole Normale Supérieure de Lyon, Université Claude Bernard Lyon 1, CNRS UAR3444, INSERM US8, Lyon, France.

出版信息

Lab Anim (NY). 2023 Dec;52(12):324-331. doi: 10.1038/s41684-023-01275-1. Epub 2023 Nov 28.

Abstract

Adoptive cell transfer between genetically identical hosts relies on the use of a congenic marker to distinguish the donor cells from the host cells. CD45, a glycoprotein expressed by all hematopoietic cells, is one of the main congenic markers used because its two isoforms, CD45.1 and CD45.2, can be discriminated by flow cytometry. As a consequence, C57BL/6J (B6; CD45.2) and B6.SJL-Ptprc Pepc/BoyJ (B6.SJL; CD45.1) mice are widely used in adoptive cell transfer experiments, under the presumption that they differ only at the CD45 (Ptprc) locus. However, recent studies have identified genetic variations between these congenic strains and have notably highlighted a differential expression of cathepsin E (CTSE). The B6.SJL mouse presents a number of functional differences in hematopoietic stem cell engraftment potential and immune cell numbers compared with the B6 mouse. In this study, we showed that B6 and B6.SJL mice also differ in their CD8 T cell compartment and CD8 T cell responses to viral infection. We identified Ctse as the most differentially expressed gene between CD8 T cells of B6 and B6.SJL and demonstrated that the differences reported between these two mouse strains are not due to CTSE. Finally, using CRISPR-Cas9 genome editing, we generated a CD45.1-expressing B6 mouse by inserting one nucleotide mutation (A904G) leading to an amino acid change (K302E) in the Ptprc gene of the B6 mouse. We showed that this new B6-Ptprc/J mouse resolves the experimental biases reported between the B6 and B6.SJL mouse lines and should thus represent the new gold standard for adoptive cell transfer experiments in B6.

摘要

在遗传相同的宿主之间进行的适应性细胞转移依赖于使用同基因标记来区分供体细胞和宿主细胞。CD45 是一种表达在所有造血细胞上的糖蛋白,是使用的主要同基因标记之一,因为其两种同工型 CD45.1 和 CD45.2 可以通过流式细胞术来区分。因此,C57BL/6J(B6;CD45.2)和 B6.SJL-Ptprc Pepc/BoyJ(B6.SJL;CD45.1)小鼠被广泛用于适应性细胞转移实验中,前提是它们仅在 CD45(Ptprc)基因座上存在差异。然而,最近的研究已经确定了这些同基因品系之间的遗传变异,并特别强调了组织蛋白酶 E(CTSE)的差异表达。与 B6 小鼠相比,B6.SJL 小鼠在造血干细胞植入潜力和免疫细胞数量方面表现出许多功能差异。在这项研究中,我们表明 B6 和 B6.SJL 小鼠在 CD8 T 细胞区室和 CD8 T 细胞对病毒感染的反应中也存在差异。我们确定 Ctse 是 B6 和 B6.SJL 的 CD8 T 细胞之间表达差异最大的基因,并证明这两个小鼠品系之间报道的差异不是由于 CTSE 引起的。最后,我们使用 CRISPR-Cas9 基因组编辑技术,通过在 B6 小鼠的 Ptprc 基因中插入一个核苷酸突变(A904G),导致氨基酸变化(K302E),生成了一个表达 CD45.1 的 B6 小鼠。我们表明,这种新的 B6-Ptprc/J 小鼠解决了 B6 和 B6.SJL 小鼠品系之间报道的实验偏差,因此应该成为 B6 中适应性细胞转移实验的新标准。

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