glutamate uptake and release

谷氨酸摄取和释放
  • 文章类型: Journal Article
    HIV感染星形胶质细胞导致基因表达和复制受限,但HIV早期基因Tat的大量表达,Nef和Rev.到目前为止,大量的神经HIV研究都集中在Tat蛋白上,它对星形胶质细胞的影响,以及它在神经HIV中的作用。在目前的研究中,我们旨在确定Nef表达对星形胶质细胞及其功能的影响。使用VSVG假型HIV病毒的转染或感染,我们发现Nef的表达下调了胶质纤维酸性蛋白(GFAP)的表达。然后我们发现Nef表达也导致GFAPmRNA表达降低。使用GFAP启动子驱动的报告基因测定进一步证实转录调节。我们进行了转录因子谱分析阵列,以比较Nef完整和Nef缺陷的HIV感染细胞之间转录因子的表达,并确定了八种表达变化为1.5倍或更高的转录因子:三种由Nef上调(Stat1,Stat5和TFIID)。和五个由Nef下调(AR,气体/ISRE,HIF,Sp1和p53)。然后,我们证明了从GFAP启动子中去除Sp1结合位点导致启动子活性水平低得多,并且对GFAP启动子的Nef效应逆转,证实Sp1在GFAP启动子活性和Nef诱导的GFAP表达中的重要作用。最后,我们发现Nef的表达导致星形胶质细胞对谷氨酸的摄取增加、谷氨酸的释放减少以及星形胶质细胞的增殖增加。一起来看,这些结果表明,Nef导致星形胶质细胞GFAP表达下调和谷氨酸代谢改变,和星形胶质细胞增殖,可能是神经HIV的重要贡献者。
    HIV infection of astrocytes leads to restricted gene expression and replication but abundant expression of HIV early genes Tat, Nef and Rev. A great deal of neuroHIV research has so far been focused on Tat protein, its effects on astrocytes, and its roles in neuroHIV. In the current study, we aimed to determine effects of Nef expression on astrocytes and their function. Using transfection or infection of VSVG-pseudotyped HIV viruses, we showed that Nef expression down-modulated glial fibrillary acidic protein (GFAP) expression. We then showed that Nef expression also led to decreased GFAP mRNA expression. The transcriptional regulation was further confirmed using a GFAP promoter-driven reporter gene assay. We performed transcription factor profiling array to compare the expression of transcription factors between Nef-intact and Nef-deficient HIV-infected cells and identified eight transcription factors with expression changes of 1.5-fold or higher: three up-regulated by Nef (Stat1, Stat5, and TFIID), and five down-regulated by Nef (AR, GAS/ISRE, HIF, Sp1, and p53). We then demonstrated that removal of the Sp1 binding sites from the GFAP promoter resulted in a much lower level of the promoter activity and reversal of Nef effects on the GFAP promoter, confirming important roles of Sp1 in the GFAP promoter activity and for Nef-induced GFAP expression. Lastly, we showed that Nef expression led to increased glutamate uptake and decreased glutamate release by astrocytes and increased astrocyte proliferation. Taken together, these results indicate that Nef leads to down-modulation of GFAP expression and alteration of glutamate metabolism in astrocytes, and astrocyte proliferation and could be an important contributor to neuroHIV.
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  • 文章类型: Journal Article
    外部磁场对大脑神经末梢的操纵有望在纳米神经技术上取得突破。通过共沉淀Fe(II)和Fe(III)盐,然后用次氯酸钠氧化并添加D-甘露糖,合成了D-甘露糖包覆的超顺磁性纳米颗粒。分析了D-甘露糖包覆的超顺磁性磁赤铁矿(γ-Fe2O3)纳米颗粒对谷氨酸能神经传递关键特征的影响。使用放射性标记的L-[(14)C]谷氨酸,研究表明,D-甘露糖包覆的γ-Fe2O3纳米颗粒不影响高亲和力Na(+)依赖性摄取,离体大鼠脑神经末梢(突触体)的补品释放和L-[(14)C]谷氨酸的细胞外水平。此外,由于应用D-甘露糖包被的γ-Fe2O3纳米颗粒,突触体的膜电位和突触小泡的酸化没有改变。用电势敏感的荧光染料罗丹明6G和pH敏感的染料吖啶橙证明了这一点。该研究还专注于分析这些纳米颗粒在通过外部磁场操纵神经末梢方面的潜在用途。结果表明,与D-甘露糖包被的γ-Fe2O3纳米颗粒(250µg/mL)孵育5分钟的超过84.3±5.0%的L-[(14)C]谷氨酸负载的突触体(1mg蛋白质/mL)移动到一个区域,其中磁铁(250mT,与用未涂覆的纳米颗粒处理的对照样品的33.5±3.0%和48.6±3.0%相比,使用了梯度5.5_/m)。因此,使用D-甘露糖包覆的γ-Fe2O3纳米颗粒,可以通过外部磁场轻松操纵孤立的脑神经末梢,而谷氨酸能神经传递的关键特征不受影响。换句话说,获得了用D-甘露糖包被的γ-Fe2O3纳米颗粒标记的功能活性突触体。
    The manipulation of brain nerve terminals by an external magnetic field promises breakthroughs in nano-neurotechnology. D-Mannose-coated superparamagnetic nanoparticles were synthesized by coprecipitation of Fe(II) and Fe(III) salts followed by oxidation with sodium hypochlorite and addition of D-mannose. Effects of D-mannose-coated superparamagnetic maghemite (γ-Fe2O3) nanoparticles on key characteristics of the glutamatergic neurotransmission were analysed. Using radiolabeled L-[(14)C]glutamate, it was shown that D-mannose-coated γ-Fe2O3 nanoparticles did not affect high-affinity Na(+)-dependent uptake, tonic release and the extracellular level of L-[(14)C]glutamate in isolated rat brain nerve terminals (synaptosomes). Also, the membrane potential of synaptosomes and acidification of synaptic vesicles was not changed as a result of the application of D-mannose-coated γ-Fe2O3 nanoparticles. This was demonstrated with the potential-sensitive fluorescent dye rhodamine 6G and the pH-sensitive dye acridine orange. The study also focused on the analysis of the potential use of these nanoparticles for manipulation of nerve terminals by an external magnetic field. It was shown that more than 84.3 ± 5.0% of L-[(14)C]glutamate-loaded synaptosomes (1 mg of protein/mL) incubated for 5 min with D-mannose-coated γ-Fe2O3 nanoparticles (250 µg/mL) moved to an area, in which the magnet (250 mT, gradient 5.5 Т/m) was applied compared to 33.5 ± 3.0% of the control and 48.6 ± 3.0% of samples that were treated with uncoated nanoparticles. Therefore, isolated brain nerve terminals can be easily manipulated by an external magnetic field using D-mannose-coated γ-Fe2O3 nanoparticles, while the key characteristics of glutamatergic neurotransmission are not affected. In other words, functionally active synaptosomes labeled with D-mannose-coated γ-Fe2O3 nanoparticles were obtained.
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  • 文章类型: Journal Article
    最近对星形胶质细胞的生理作用的研究引起了人们对这些神经胶质细胞在中枢神经系统中的功能意义的新兴趣。许多新发现的星形细胞功能最初在细胞培养系统中得到了证明和表征。我们讨论了在星形细胞Ca(2)兴奋性和双向神经元-星形胶质细胞信号传导研究中使用微培养技术和细胞粘附基质的微图案化。这种培养方法旨在通过限制相互作用的配偶体和通过控制细胞的定位来降低系统的复杂性水平。它提供了对实验条件的严格控制,从而可以详细表征细胞功能和细胞间通讯。尽管这种还原论方法在培养和原位星形细胞特性之间的观察中产生了一些差异,细胞培养系统中发现的一般现象,然而,也被发现在体内。
    Recent studies of the physiological roles of astrocytes have ignited renewed interest in the functional significance of these glial cells in the central nervous system. Many of the newly discovered astrocytic functions were initially demonstrated and characterized in cell culture systems. We discuss the use of microculture techniques and micropatterning of cell-adhesive substrates in studies of astrocytic Ca(2+) excitability and bidirectional neuron-astrocyte signaling. This culturing approach aims to reduce the level of complexity of the system by limiting the interacting partners and by controlling the localization of cells. It provides tight control over experimental conditions allowing detailed characterization of cellular functions and intercellular communication. Although such a reductionist approach yields some difference in observations between astrocytic properties in culture and in situ, general phenomena discovered in cell culture systems, however, have also been found in vivo.
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