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活性己糖跨培养的人Caco-2细胞的转运:培养条件的表征及影响

Active hexose transport across cultured human Caco-2 cells: characterisation and influence of culture conditions.

作者信息

Riley S A, Warhurst G, Crowe P T, Turnberg L A

机构信息

Department of Medicine, University of Manchester, Hope Hospital, Salford, U.K.

出版信息

Biochim Biophys Acta. 1991 Jul 22;1066(2):175-82. doi: 10.1016/0005-2736(91)90184-a.

Abstract

Human Caco-2 cells (passage 80 to 100) were seeded onto collagen-coated Millipore filter assemblies and these were maintained in culture either (a) floated on the surface of the medium or (b) submerged within the body of the medium. Structural and functional assessments were made over a 30-day period. After seeding, all cells assumed a flattened, squamous configuration and rapidly became confluent. Cells submerged within the medium formed polarised monolayers with well developed junctional complexes, abundant apical microvilli and increasing levels of alkaline phosphatase activity. Cells grown floated on the surface of the medium formed complex multilayers in which polarisation was confined to the surface layer. Junctional complexes and apical microvilli were similar to those seen in submerged monolayers but alkaline phosphatase activities were higher. Transepithelial electrical resistance increased rapidly from day 1, as the layers became confluent. Electrical resistance was higher and short-circuit current and potential differences were lower across monolayers than across multilayers. After 10 days in culture, the addition of D-glucose to the apical bathing solution, of all cell layers, caused a rapid rise in short-circuit current and potential difference. These changes were sodium-dependent and phlorizin-sensitive. Galactose and 3-O-methylglucose induced similar changes and the affinity constants for these hexoses ranked in the order reported for rat jejunum (Km glucose 2.44 +/- 0.52 mM; Km galactose 8.05 +/- 1.33 mM; Km 3-O-methylglucose 22.0 +/- 5.2 mM). Culture conditions had a marked effect on hexose maximum transport rates (glucose Vmax: submerged 2.94 +/- 0.20 microA/cm2; floated 9.94 +/- 0.82 microA/cm2, P less than 0.05) but affinity constants were unchanged. Apical to basolateral mannitol fluxes, used as an index of paracellular permeability, decreased from day 1 to day 5 and then remained steady. Fluxes across monolayers and multilayers were not significantly different. We conclude that sodium-dependent hexose transport occurs in cultured Caco-2 cell layers grown on permeable supports. Culture conditions, however, have a marked effect on both cell layer structure and function, and should be an important factor when considering Caco-2 cells as an in vitro model of enterocyte function.

摘要

将人源Caco - 2细胞(传代80至100代)接种到经胶原蛋白包被的密理博滤膜组件上,并将其置于培养环境中,培养方式分为两种:(a) 漂浮于培养基表面;(b) 浸没于培养基中。在30天的时间内进行结构和功能评估。接种后,所有细胞呈现扁平的鳞状形态,并迅速汇合。浸没于培养基中的细胞形成了具有发育良好的连接复合体、丰富的顶端微绒毛以及碱性磷酸酶活性不断升高的极化单层细胞。漂浮在培养基表面生长的细胞形成了复杂的多层结构,其中极化现象局限于表层。连接复合体和顶端微绒毛与浸没单层细胞中的相似,但碱性磷酸酶活性更高。随着细胞层汇合,跨上皮电阻从第1天开始迅速增加。单层细胞的电阻更高,短路电流和电位差比多层细胞更低。培养10天后,向所有细胞层的顶端浴液中添加D - 葡萄糖,导致短路电流和电位差迅速升高。这些变化依赖于钠离子且对根皮苷敏感。半乳糖和3 - O - 甲基葡萄糖诱导了类似的变化,这些己糖的亲和常数排序与大鼠空肠报道的顺序一致(葡萄糖Km 2.44 ± 0.52 mM;半乳糖Km 8.05 ± 1.33 mM;3 - O - 甲基葡萄糖Km 22.0 ± 5.2 mM)。培养条件对己糖最大转运速率有显著影响(葡萄糖Vmax:浸没培养为2.94 ± 0.20 μA/cm²;漂浮培养为9.94 ± 0.82 μA/cm²,P < 0.05),但亲和常数不变。用作细胞旁通透性指标的顶端到基底的甘露醇通量从第1天到第5天下降,然后保持稳定。单层细胞和多层细胞的通量没有显著差异。我们得出结论,在可渗透支持物上培养的Caco - 2细胞层中发生了依赖于钠离子的己糖转运。然而,培养条件对细胞层结构和功能都有显著影响,在将Caco - 2细胞作为肠上皮细胞功能的体外模型时,这应该是一个重要因素。

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