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首页> 外文期刊>Blood: The Journal of the American Society of Hematology >C1galt1-deficient mice exhibit thrombocytopenia due to abnormal terminal differentiation of megakaryocytes.
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C1galt1-deficient mice exhibit thrombocytopenia due to abnormal terminal differentiation of megakaryocytes.

机译:缺乏C1galt1的小鼠由于巨核细胞的异常终末分化而出现血小板减少症。

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C1galt1 is essential for synthesis of the core 1 structure of mucin-type O-glycans. To clarify the physiological role of O-glycans in adult hematopoiesis, we exploited the interferon-inducible Mx1-Cre transgene to conditionally ablate the C1galt(flox) allele (Mx1-C1). Mx1-C1 mice exhibit severe thrombocytopenia, giant platelets, and prolonged bleeding times. Both the number and DNA ploidy of megakaryocytes in Mx1-C1 bone marrow were similar to those in wild-type (WT) mice. However, there were few proplatelets in Mx1-C1 primary megakaryocytes. Conversely, bone marrow transplanted from Mx1-C1 to WT and splenectomized Mx1-C1 mice gave rise to observations similar to those described above. The expression of GPIbα messenger RNA was unchanged in Mx1-C1 bone marrow, whereas flow cytometric and western blot analyses using megakaryocytes and platelets revealed that the expression of GPIbα protein was significantly reduced in Mx1-C1 mice. Moreover, circulating Mx1-C1 platelets exhibited an increase in the number of microtubule coils, despite normal levels of α- and β-tubulin. Our observations suggest that O-glycan is required for terminal megakaryocyte differentiation and platelet production and that the decrease in GPIbα in cells lacking O-glycan might be caused by increased proteolysis.
机译:C1galt1对粘蛋白型O聚糖的核心1结构的合成至关重要。为了阐明O-聚糖在成人造血中的生理作用,我们利用干扰素诱导的Mx1-Cre转基因有条件地消融了C1galt(flox)等位基因(Mx1-C1)。 Mx1-C1小鼠表现出严重的血小板减少症,巨大的血小板和延长的出血时间。 Mx1-C1骨髓中巨核细胞的数量和DNA倍性均与野生型(WT)小鼠相似。但是,Mx1-C1原代巨核细胞中的原血小板很少。相反,从Mx1-C1移植到WT和脾切除的Mx1-C1小鼠的骨髓引起了与上述相似的观察结果。在Mx1-C1骨髓中,GPIbα信使RNA的表达没有变化,而使用巨核细胞和血小板的流式细胞仪和Western blot分析表明,在Mx1-C1小鼠中,GPIbα蛋白的表达显着降低。此外,尽管α-和β-微管蛋白水平正常,但是循环的Mx1-C1血小板表现出微管线圈数增加。我们的观察表明,O-聚糖对于巨核细胞的终末分化和血小板生成是必需的,而缺乏O-聚糖的细胞中GPIbα的下降可能是由于蛋白水解的增加所致。

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