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Regional permeability of salmon calcitonin in isolated rat gastrointestinal tracts: Transport mechanism using Caco-2 cell monolayer

机译:鲑降钙素在大鼠离体胃肠道中的区域渗透性:使用Caco-2细胞单层的转运机制

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摘要

The objective of the study was to determine the region of maximum permeation of salmon calcitonin (sCT) through the gastrointestinal tract and to investigate the mechanism of permeation. For regional permeability determination, male Sprague-Dawley rats (250–300 g) were anesthetized and the gastrointestinal tissues were isolated. Stomach, duodenum, jejunum, ileum, or colon tissues were mounted on Navicyte side-by-side diffusion apparatus. Salmon calcitonin solutions (50 μM in phosphate-buffered saline, pH 7.4, 37°C) were added to the donor side, and the samples were removed from the receiver compartment and analyzed by competitive radioimmunoassay (RIA). For mechanistic studies, Caco-2 cells were grown on Transwell inserts (0.4-μm pore size, 0.33 cm2 area) in a humidified 37°C incubator (with 5% CO2). Transport experiments were conducted for sCT solutions (50 μM in Dulbecco's modified eagle's medium [DMEM], pH 7.4) from the apical-to-basolateral (A-to-B) direction and B-to-A direction at 37°C and from the A-to-B direction at 4°C. Cell monolayer integrity was monitored by mannitol permeability and transepithelial electrical resistance (TEER) measurements. The permeability coefficients (× 10−9, cm/sec) for sCT through rat stomach, duodenum, jejunum, ileum, and colon tissues were 0.482±0.086, 0.718±0.025, 0.830±0.053, 1.537±0.32, and 0.934±0.15, respectively. The region of maximum sCT permeability is ileum followed by colon, jejunum, duodenum, and stomach. The permeability coefficients (× 10−6, cm/sec) for sCT through Caco-2 cell monolayer were 8.57±2.34 (A-to-B, 37°C), 8.01±1.22 (A-to-B, 4°C), and 6.15±1.97 (B-to-A, 37°C). The mechanism of its permeation is passive diffusion through the mucosa as determined from the Caco-2 monolayer permeability of sCT.
机译:该研究的目的是确定鲑鱼降钙素(sCT)通过胃肠道的最大渗透区域,并研究其渗透机理。为了确定区域通透性,将雄性Sprague-Dawley大鼠(250-300 g)麻醉,并分离胃肠道组织。将胃,十二指肠,空肠,回肠或结肠组织安装在Navicyte并排扩散装置上。将鲑鱼降钙素溶液(在磷酸盐缓冲液中的50μM,pH 7.4,37°C)添加到供体侧,将样品从接收器隔室中取出,并通过竞争性放射免疫分析(RIA)进行分析。为了进行机理研究,将Caco-2细胞培养在Transwell插入物上(孔径为0.4-μm,面积为0.33 cm2)在加湿的37°C恒温箱(含5%CO2)中生长。从sct溶液(在Dulbecco改良的Eagle's介质[DMEM],pH 7.4中为50μM)从顶到基底外侧(A到B)方向和B到A方向在37°C以及从在4°C下从A到B的方向。通过甘露醇渗透性和跨上皮电阻(TEER)测量来监测细胞单层完整性。 sCT通过大鼠胃,十二指肠,空肠,回肠和结肠组织的渗透系数(×10-9,cm / sec)为0.482±0.086、0.718±0.025、0.830±0.053、1.537±0.32和0.934±0.15,分别。 sCT渗透性最大的区域是回肠,其次是结肠,空肠,十二指肠和胃。 sCT通过Caco-2细胞单层的渗透系数(×10-6,cm / sec)为8.57±2.34(A-B,37°C),8.01±1.22(A-B,4°C) )和6.15±1.97(B-to-A,37°C)。根据sCT的Caco-2单层渗透性确定,其渗透机制是通过粘膜的被动扩散。

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