Redzic Zoran B, Isakovic Aleksandra J, Misirlic Dencic Sonja T, Popadic Dusan, Segal Malcolm B
School of Biomedical Sciences, King's College London, London, UK.
Cerebrospinal Fluid Res. 2006 Mar 29;3:4. doi: 10.1186/1743-8454-3-4.
Efflux transport of adenosine across the choroid plexus (CP) epithelium might contribute to the homeostasis of this neuromodulator in the extracellular fluids of the brain. The aim of this study was to explore adenosine transport across sheep CP epithelial cell monolayers in primary culture.
To explore transport of adenosine across the CP epithelium, we have developed a method for primary culture of the sheep choroid plexus epithelial cells (CPEC) on plastic permeable supports and analysed [14C] adenosine transport across this cellular layer, [14C] adenosine metabolism inside the cells, and cellular uptake of [14C] adenosine from either of the chambers. The primary cell culture consisted of an enriched epithelial cell fraction from the sheep fourth ventricle CP and was grown on laminin-precoated filter inserts.
CPEC grew as monolayers forming typical polygonal islands, reaching optical confluence on the third day after the seeding. Transepithelial electrical resistance increased over the time after seeding up to 85 +/- 9 Omega cm2 at day 8, while permeability towards [14C] sucrose, a marker of paracellular diffusion, simultaneously decreased. These cells expressed some features typical of the CPEC in situ, including three nucleoside transporters at the transcript level that normally mediate adenosine transport across cellular membranes. The estimated permeability of these monolayers towards [14C] adenosine was low and the same order of magnitude as for the markers of paracellular diffusion.However, inhibition of the intracellular enzymes, adenosine kinase and adenosine deaminase, led to a significant increase in transcellular permeability, indicating that intracellular phosphorylation into nucleotides might be a reason for the low transcellular permeability. HPLC analysis with simultaneous detection of radioactivity revealed that [14C] radioactivity which appeared in the acceptor chamber after the incubation of CPEC monolayers with [14C] adenosine in the donor chamber was mostly present as [14C] hypoxanthine, a product of adenosine metabolic degradation. Therefore, it appears that CPEC in primary cultures act as an enzymatic barrier towards adenosine. Cellular uptake studies revealed that concentrative uptake of [14C] adenosine was confined only to the side of these cells facing the upper or apical chamber, indicating uneven distribution of nucleoside transporters.
腺苷经脉络丛(CP)上皮的外排转运可能有助于维持这种神经调质在脑细胞外液中的稳态。本研究的目的是探讨腺苷在原代培养的绵羊CP上皮细胞单层中的转运情况。
为了探究腺苷在CP上皮中的转运,我们开发了一种在塑料可渗透支持物上原代培养绵羊脉络丛上皮细胞(CPEC)的方法,并分析了[14C]腺苷跨该细胞层的转运、细胞内[14C]腺苷的代谢以及从任一腔室对[14C]腺苷的细胞摄取。原代细胞培养物由来自绵羊第四脑室CP的富集上皮细胞部分组成,并在层粘连蛋白预包被的滤膜小室上生长。
CPEC以单层形式生长,形成典型的多边形岛状结构,接种后第三天达到光学汇合。接种后跨上皮电阻随时间增加,在第8天达到85±9Ω·cm2,而作为细胞旁扩散标志物的[14C]蔗糖的通透性同时降低。这些细胞表现出一些原位CPEC的典型特征,包括在转录水平上有三种核苷转运体,它们通常介导腺苷跨细胞膜的转运。这些单层对[14C]腺苷的估计通透性较低,与细胞旁扩散标志物的通透性处于同一数量级。然而,抑制细胞内酶腺苷激酶和腺苷脱氨酶会导致跨细胞通透性显著增加,这表明细胞内磷酸化形成核苷酸可能是跨细胞通透性低的原因。同时检测放射性的HPLC分析表明,在供体腔室中用[14C]腺苷孵育CPEC单层后,在受体腔室中出现的[14C]放射性主要以[14C]次黄嘌呤的形式存在,这是腺苷代谢降解的产物。因此,原代培养的CPEC似乎对腺苷起到了酶屏障的作用。细胞摄取研究表明,[14C]腺苷的浓缩摄取仅局限于这些细胞面向上部或顶端腔室的一侧,表明核苷转运体分布不均。
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