炎症过程中载脂蛋白E亚型在星形胶质细胞和小胶质细胞的表达和分泌

神经炎症是神经退行性疾病的常见特征,受阿尔茨海默病危险因素载脂蛋白E(APOE)的调节。apoE蛋白在大脑中由星形胶质细胞和小胶质细胞合成。在人类APOE(E2、E3和E4)靶向替代小鼠的星形胶质细胞和小胶质细胞的原代培养物中,我们发现星形胶质细胞分泌2种apoE,而细胞内apoE只包含1种。2种形式的分泌型星形胶质细胞apoE在糖蛋白分离过程中均发生结合,酶促去除聚糖使2种形式的apoE融合为单一形式。因此,星形胶质细胞分泌的2种apoE是不同的糖基化的蛋白。小胶质细胞仅释放1种apoE,而细胞内apoE则由2种形式组成;分泌的apoE和2种细胞内apoE中的其中1种是糖基化的。我们用内源性肿瘤坏死因子α(TNFα)或外源性脂多糖(LPS)促炎刺激物处理原代培养的胶质细胞。LPS对星形细胞的apoE没有影响,而APOE2和APOE3小胶质细胞释放的apoE增加;对APOE4小胶质细胞也没有影响。与APOE2和APOE3小胶质细胞相比,APOE4小胶质细胞显示出更高的TNFα基线分泌。TNFα处理仅降低了APOE4星形胶质细胞中apoE的分泌和细胞表达。星形胶质细胞和小胶质细胞产生apoE种类的模式不受炎症的影响。2种处理后的星形胶质细胞中均未显示APOE mRNA的变化。总之,我们的数据表明,星形胶质细胞和小胶质细胞差异表达和分泌糖基化形式的apoE;并且相较于APOE2和APOE3,APOE4星形胶质细胞和小胶质细胞在免疫调节方面存在缺陷。

Pharmacogenetics of asparaginase in acute lymphoblastic leukemia

Asparaginase is a key component in leukemias and lymphomas treatment protocols and is suggested as a treatment for other malignancies in which an amino acid depletion strategy is indicated.Asparaginase intolerance is subject to inter-individual variability and can manifest as hypersensitivity reactions,pancreatitis,thrombosis,as well as metabolic abnormalities,and may affect treatment outcome.Pharmacogenetics aims at enhancing treatment efficacy and safety by better understanding the genetic basis of variability and its effect on the pharmacological responses.Many groups tried to tackle the pharmacogenetics of asparaginase but the potential implementation of such findings remains debatable.In this review,we highlight the most important findings reported in studies of the pharmacogenetics of asparaginase related complications and treatment outcome in acute lymphoblastic leukemia.

Interleukin-1β-induced inflammatory signaling in C20 human microglial cells

Aim: Increased inflammatory signaling in microglia is implicated in the pathogenesis of neurodegenerative diseases, trauma, psychiatric disorders, and anxiety/depression. Understanding inflammatory signaling in microglia is critical for advancing treatment options. Studying rodent-derived microglia has yielded substantial information, yet, much remains to better understand inflammatory signaling in human microglia. Hence, there is great interest in developing immortalized human microglial cell lines. The C20 human microglial cell line was recently developed and our primary objective was to advance our knowledge of inflammatory signaling in these cells. Methods: Expression of the microglia specific marker transmembrane protein 119 (TMEM119) was assessed by western blot analysis. Lipopolysaccharide (LPS)- and interleukin-1β (IL-1β)-induced cytokine/chemokine expression was determined by ELISA. Phosphorylation of inhibitory kappa B alpha (IκBα), nuclear factor (NF)-κB p65, and p38 mitogen-activated protein kinase (p38 MAPK) was measured by western blot analysis. Results: TMEM119 was expressed in unstimulated C20 cells, and to a greater extent in IL-1β-stimulated cells. IL-1βsignificantly induced IL-6, monocyte chemoattractant protein-1/CCL2, and interferon-γ inducible protein 10/CXCL10 expression. LPS induced CCL2 expression, but not IL-6 or CXCL10 expression. IL-1β induced inflammatory signaling as indicated by increased phosphorylation of IκBα, NF-κB p65 and p38 MAPK. Conclusion: We provide the first evidence that C20 microglia express TMEM119. This is the initial report of IL-1β-induced activation of IκBα, NF-κB p65, and p38 MAPK and subsequent CXCL10, CCL2 and IL-6 secretion in C20cells. These findings advance our understanding of inflammatory signaling in C20 cells and support the value of this cell line as a research tool.