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Surface charge distribution on the endothelial cell of liver sinusoids

机译:肝窦表面内皮细胞的表面电荷分布

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摘要

The topography of the charged residues on the endothelial cell surface of liver sinusoid capillaries was investigated by using electron microscopic tracers of different size and charge. The tracers used were native ferritin (pl 4.2-4.7) and its cationized (pl 8.4) and anionized (pl 3.7) derivatives, BSA coupled to colloidal gold (pl of the complex 5.1), hemeundecapeptide (pl 4.85), and alcian blue (pl greater than 10). The tracers were either injected in vivo or perfused in situ through the portal vein of the mouse liver. In some experiments, two tracers of opposite charge were sequentially perfused with extensive washing in between. The liver was processed for electron microscopy and the binding pattern of the injected markers was recorded. The electrostatic nature of the tracer binding was assessed by perfusion with high ionic strength solutions, by aldehyde quenching of the plasma membrane basic residues, and by substituting the cell surface acidic moieties with positively charged groups. Results indicate that the endothelial cells of the liver sinusoids expose on their surface both cationic and anionic residues. The density distribution of these charged groups on the cell surface is different. While the negative charge is randomly and patchily scattered all over the membrane, the cationic residues seem to be accumulated in coated pits. The charged groups co-exist in the same coated pit and bind the opposite charged macromolecule. It appears that the fixed positive and negative charges of the coated pit glycocalyx are mainly segregated in space. The layer of basic residues is located at 20-30-nm distance of the membrane, while most of the negative charges lie close to the external leaflet of the plasmalemma.
机译:使用不同大小和电荷的电子显微镜示踪剂研究了肝窦毛细血管内皮细胞表面带电残基的形貌。使用的示踪剂是天然铁蛋白(pl 4.2-4.7)及其阳离子化(pl 8.4)和阴离子化(pl 3.7)衍生物,与胶体金偶联的BSA(络合物5.1的pl),血红蛋白肽(pl 4.85)和阿尔辛蓝( pl大于10)。示踪剂可以体内注射或通过小鼠肝门静脉原位灌注。在某些实验中,依次注入两个带相反电荷的示踪剂,并在两者之间进行大量洗涤。对肝脏进行电子显微镜检查,并记录注射标记的结合模式。示踪剂结合的静电性质是通过用高离子强度溶液灌注,通过质膜碱性残基的醛猝灭,以及用带正电荷的基团代替细胞表面酸性部分来评估的。结果表明,肝窦的内皮细胞在其表面上同时暴露出阳离子和阴离子残基。这些带电基团在细胞表面的密度分布是不同的。尽管负电荷在整个膜上随机分散分布,但阳离子残留物似乎聚集在涂层的凹坑中。带电基团共存于相同的涂层凹坑中,并结合相反的带电大分子。看来,带涂层的凹腔糖萼的固定正电荷和负电荷主要在空间中隔离。碱性残留物层位于膜的20-30 nm距离处,而大多数负电荷则位于质膜的外部小叶附近。

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