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Urea transport by cotransporters

机译:共同运输者进行尿素运输

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class="enumerated" style="list-style-type:decimal">The rabbit Na+-glucose cotransporter (rbSGLT1) was expressed in Xenopus laevis oocytes and urea transport in rbSGLT1 and non-injected (control) oocytes was studied using [14C]urea as a tracer. The level of rbSGLT1 expression in these batches of oocytes was monitored by measuring the uptake of α-methyl-d-[14C]glucopyranoside ([14C]αMDG).In rbSGLT1-expressing oocytes, there was a 4-fold increase in urea transport in the absence of sugar relative to that in control oocytes. Urea uptake was not Na+ dependent and was linear with both time of incubation (5–120 min) and increasing urea concentration (50 μm to 100 mm) in the bathing medium. rbSGLT1 urea uptake was blocked by the rbSGLT1-specific inhibitor phlorizin (Ki 1 μm) in 100 mm NaCl buffer, but was not affected in 100 mm choline chloride buffer. Phloretin inhibited rbSGLT1 urea uptake with a low affinity (Ki > 1 mm) in the presence and absence of Na+. The uptake of 55 μm urea through rbSGLT1 was not blocked by 100 mm urea analogues including thiourea, 1,3-dimethyl urea, 1,1-dimethyl urea and acetamide.The activation energies (Ea) of urea transport for control and rbSGLT1-expressing oocytes were 14 ± 3 and 6 ± 1 kcal mol−1, respectively. The low Ea for urea transport through rbSGLT1 is comparable to the Ea of passive water transport through rbSGLT1.Urea transport through rbSGLT1 was further increased when the cotransporter was activated by the addition of sugar to the external medium. The rate of sugar-dependent urea uptake was directly proportional to the rate of Na+-glucose-H2O cotransport such that the amount of urea transport was approximately proportional to the molar concentration ratio of urea to H2O (55 μm/55 m).The low affinity Na+-glucose (pSGLT3), the Na+-iodide (rNIS) and the Na+-Cl-GABA (hGAT1) cotransporters expressed in oocytes demonstrated similar urea transport properties.These observations suggest that cotransporters behave as urea channels in the absence of substrates. Furthermore, under substrate-transporting conditions, the same cotransporters serve as urea cotransporters. This could account for urea transport in cells that appear not to have urea uniporters or channels.
机译:class =“ enumerated” style =“ list-style-type:decimal”> <!-list-behavior =枚举前缀-word = mark-type = decimal max-label-size = 0-> 兔Na + -葡萄糖共转运蛋白(rbSGLT1)在非洲爪蟾卵母细胞中表达,尿素转运在rbSGLT1中,未注射的(对照)卵母细胞使用[ 14 C]研究尿素作为示踪剂。通过测量α-甲基-d-[ 14 C]葡萄糖吡喃糖苷([ 14 C]αMDG)的摄取来监测这些批次卵母细胞中rbSGLT1表达的水平。 在表达rbSGLT1的卵母细胞中,在无糖的情况下尿素转运相对于对照卵母细胞增加了4倍。尿素的吸收与Na + 无关,并且与孵育时间(5-120分钟)和沐浴介质中尿素浓度(50μm至100 mm)的增加呈线性关系。在100 mm NaCl缓冲液中,rbSGLT1特异性抑制剂phlorizin(Ki 1μm)阻止了rbSGLT1尿素的吸收,但在100 mm氯化胆碱缓冲液中并未受到影响。在存在和不存在Na + 的情况下,球蛋白均以低亲和力(Ki> 1 mm)抑制rbSGLT1尿素吸收。通过rbSGLT1吸收55μm尿素不会被100 mm尿素类似物(包括硫脲,1,3-二甲基尿素,1,1-二甲基尿素和乙酰胺)阻止。 尿素的活化能(Ea)对照和表达rbSGLT1的卵母细胞的转运分别为14±3和6±1 kcal mol -1 。通过rbSGLT1进行尿素转运的Ea值与通过rbSGLT1进行被动水转运的Ea值相当。 当通过向外部介质中添加糖激活共转运蛋白时,通过rbSGLT1进行尿素转运的数量进一步增加。糖依赖性尿素的吸收速率与Na + -葡萄糖-H2O共转运的速率成正比,因此尿素转运的量大约与尿素与H2O的摩尔浓度比成正比(55 μm/ 55 m)。 低亲和力Na + -葡萄糖(pSGLT3),Na + -碘化物(rNIS)和Na <在卵母细胞中表达的sup> + -Cl - -GABA(hGAT1)共转运蛋白表现出相似的尿素转运特性。 这些观察结果表明,共转运蛋白在卵母细胞中表现为尿素通道。没有底物。此外,在底物运输条件下,相同的共转运蛋白用作尿素共转运蛋白。这可以解释尿素在似乎没有尿素单向转运蛋白或通道的细胞中的迁移。

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