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IN VITRO PROPAGATION AND HOMING OF LIVER-DERIVED DENDRITIC CELL PROGENITORS TO LYMPHOID TISSUES OF ALLOGENEIC RECIPIENTS

机译:肝源性树突状细胞祖细胞到异源受体淋巴组织的体外繁殖和归巢

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摘要

Dendritic cell (DC) progenitors were propagated in liquid culture from nonparenchymal cells resident in normal mouse (B10.BR; H-2k, I-E+) liver in response to granulocyte-macrophage colony stimulating factor (GM-CSF). The liver-derived DC progenitors were MHC class H−/dim and did not express counter receptors for CTLA-4, a structural homologue of the T cell activation molecule CD28. Following subcutaneous or intravenous injection, these liver-derived cells migrated to T cell-dependent areas of lymph nodes and spleen of unmodified, allogeneic (B10; H-2b; I-E) recipients, where they were identified 1-5 days, and 1 and 2 months after injection by their strong surface expression of donor MHC class II (I-Ek) and their dendritic morphology. Maximal numbers of liver-derived DC in the spleen were recorded 5 days after injection. Both clusters of strongly donor MHC class II+ cells— and (more rarely) dividing cells—could also be identified, suggesting cell replication in situ. Using the same techniques employed to generate DC progenitors from normal liver, GM-CSF-stimulated cells were propagated for 10 days from the bone marrow and spleen of nonimmunosuppressed mice sacrificed 14 days after orthotopic liver transplantation (B10;H-2b → C3H;H-2k). Immunocytochemical staining for recipient and donor MHC class II phenotype revealed the growth both of host cells with DC characteristics, and of cells expressing donor alloantigens (I-Ab. These results are consistent with the growth, in response to GM-CSF, of donor-derived DC from progenitors seeded from the liver allograft to recipient lymphoid tissue. The functional activity of the progenitors of chimeric DC and the possible role of these cells in the establishment and maintenance of donor-specific tolerance following liver transplantation remain to be determined.
机译:树突状细胞(DC)祖细胞在液体培养中从正常小鼠(B10.BR; H-2 k ,IE + )肝脏中的非实质细胞中繁殖而出-巨噬细胞集落刺激因子(GM-CSF)。肝脏来源的DC祖细胞是MHC H -/ dim 类,不表达CTLA-4的反受体,CTLA-4是T细胞活化分子CD28的结构同源物。皮下或静脉内注射后,这些肝源性细胞迁移到未修饰的同种异体(B10; H-2 b ; IE -的淋巴结和脾脏的T细胞依赖性区域。 >)接受者,他们在注射后1-5天,注射后1和2个月被发现,这是由于其II类供体MHC的强表面表达(IE k )及其树突形态。注射后5天记录脾脏中肝来源的DC的最大数目。还可以鉴定出两个强供体MHC II类 + 细胞簇,以及(很少有)分裂的细胞簇,提示细胞原位复制。使用从正常肝脏生成DC祖细胞的相同技术,将GM-CSF刺激的细胞从原位肝移植后14天处死的非免疫抑制小鼠的骨髓和脾脏中繁殖出10天(B10; H-2 b →C3H; H-2 k )。对受体和供体MHC II类表型的免疫细胞化学染色显示,具有DC特征的宿主细胞和表达供体同种抗原(IA b )的细胞均生长。这些结果与GM的生长一致-CSF,来自肝脏同种异体移植到受体淋巴组织的祖细胞的供体来源的DC嵌合DC的祖细胞的功能活性以及这些细胞在肝移植后建立和维持供体特异性耐受中的可能作用仍然存在待定。

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