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免疫特惠的胚胎瑞士小鼠STO及STO细胞衍生的祖细胞:主要组织相容性复合体和细胞分化抗原表达模式类似于人类胚胎干细胞系。

Immune-privileged embryonic Swiss mouse STO and STO cell-derived progenitor cells: major histocompatibility complex and cell differentiation antigen expression patterns resemble those of human embryonic stem cell lines.

作者信息

Koch Katherine S, Son Kyung-Hwa, Maehr Rene, Pellicciotta Illenia, Ploegh Hidde L, Zanetti Maurizio, Sell Stewart, Leffert Hyam L

机构信息

Department of Pharmacology, School of Medicine, University of California at San Diego, La Jolla, CA 92093-0636, USA.

出版信息

Immunology. 2006 Sep;119(1):98-115. doi: 10.1111/j.1365-2567.2006.02412.x. Epub 2006 Jul 10.

Abstract

Embryonic mouse STO (S, SIM; T, 6-thioguanine resistant; O, ouabain resistant) and 3(8)21-enhanced green fluorescent protein (EGFP) cell lines exhibit long-term survival and hepatic progenitor cell behaviour after xenogeneic engraftment in non-immunosuppressed inbred rats, and were previously designated major histocompatibility complex (MHC) class I- and class II-negative lines. To determine the molecular basis for undetectable MHC determinants, the expression and haplotype of H-2K, H-2D, H-2L and I-A proteins were reassessed by reverse transcriptase-polymerase chain reaction (RT-PCR), cDNA sequencing, RNA hybridization, immunoblotting, quantitative RT-PCR (QPCR), immunocytochemistry and flow cytometry. To detect cell differentiation (CD) surface antigens characteristic of stem cells, apoptotic regulation or adaptive immunity that might facilitate progenitor cell status or immune privilege, flow cytometry was also used to screen untreated and cytokine [interferon (IFN)-gamma]-treated cultures. Despite prior PCR genotyping analyses suggestive of H-2q haplotypes in STO, 3(8)21-EGFP and parental 3(8)21 cells, all three lines expressed H-2K cDNA sequences identical to those of d-haplotype BALB/c mice, as well as constitutive and cytokine-inducible H-2K(d) determinants. In contrast, apart from H-2L(d[LOW]) display in 3(8)21 cells, H-2Dd, H-2Ld and I-Ad determinants were undetectable. All three lines expressed constitutive and cytokine-inducible CD34; however, except for inducible CD117([LOW]) expression in 3(8)21 cells, no expression of CD45, CD117, CD62L, CD80, CD86, CD90.1 or CD95L/CD178 was observed. Constitutive and cytokine-inducible CD95([LOW]) expression was detected in STO and 3(8)21 cells, but not in 3(8)21-EGFP cells. MHC (class I(+[LOW])/class II-) and CD (CD34+/CD80-/CD86-/CD95L-) expression patterns in STO and STO cell-derived progenitor cells resemble patterns reported for human embryonic stem cell lines. Whether these patterns reflect associations with mechanisms that are regulatory of immune privilege or functional tissue-specific plasticity is unknown.

摘要

胚胎小鼠STO(S,SIM;T,对6-硫代鸟嘌呤耐药;O,对哇巴因耐药)和3(8)21-增强型绿色荧光蛋白(EGFP)细胞系在非免疫抑制的近交系大鼠体内异种移植后表现出长期存活及肝祖细胞行为,之前被指定为主要组织相容性复合体(MHC)I类和II类阴性细胞系。为了确定无法检测到MHC决定簇的分子基础,通过逆转录聚合酶链反应(RT-PCR)、cDNA测序、RNA杂交、免疫印迹、定量RT-PCR(QPCR)、免疫细胞化学和流式细胞术对H-2K、H-2D、H-2L和I-A蛋白的表达及单倍型进行了重新评估。为了检测可能有助于祖细胞状态或免疫豁免的干细胞特征性细胞分化(CD)表面抗原、凋亡调节或适应性免疫,还使用流式细胞术对未处理的和经细胞因子[干扰素(IFN)-γ]处理的培养物进行了筛选。尽管之前的PCR基因分型分析提示STO、3(8)21-EGFP和亲本3(8)21细胞具有H-2q单倍型,但所有这三个细胞系均表达与d单倍型BALB/c小鼠相同的H-2K cDNA序列,以及组成型和细胞因子诱导型H-2K(d)决定簇。相比之下,除了3(8)21细胞中显示的H-2L(d[LOW])外,未检测到H-2Dd、H-2Ld和I-Ad决定簇。所有这三个细胞系均表达组成型和细胞因子诱导型CD34;然而,除了3(8)21细胞中可诱导的CD117([LOW])表达外,未观察到CD45、CD117、CD62L、CD80、CD86、CD90.1或CD95L/CD178的表达。在STO和3(8)21细胞中检测到组成型和细胞因子诱导型CD95([LOW])表达,但在3(8)21-EGFP细胞中未检测到。STO及源自STO细胞的祖细胞中的MHC(I类(+[LOW])/II类-)和CD(CD34+/CD80-/CD86-/CD95L-)表达模式与报道的人类胚胎干细胞系的模式相似。这些模式是否反映了与免疫豁免调节机制或功能性组织特异性可塑性的关联尚不清楚。

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