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小溶质在生长于可渗透支持物上的MDCK细胞上皮细胞间侧间隙中的扩散。

Diffusion of small solutes in the lateral intercellular spaces of MDCK cell epithelium grown on permeable supports.

作者信息

Kovbasnjuk O N, Bungay P M, Spring K R

机构信息

Laboratory of Kidney and Electrolyte Metabolism, National Heart, Lung and Blood Institute, Bethesda, MD 20892-5766, USA.

出版信息

J Membr Biol. 2000 May 1;175(1):9-16. doi: 10.1007/s002320001050.

Abstract

The diffusion coefficients of four solutes ranging in molecular weight from 238 to 10,000 in the lateral intercellular spaces (LIS) of cultured kidney cells (MDCK) grown on permeable supports were determined from the spread of fluorescence produced after the release of caged compounds by a pulse from a UV laser. Two types of experiments were performed: measurement of the rate of change of fluorescence after releasing a caged fluorophore, and measurement of the change in fluorescence of a relatively static fluorescent dye produced by the diffusion of an uncaged ligand for the dye. Fluorescence intensity was determined by photon-counting the outputs of a multichannel photomultiplier tube. Diffusion coefficients were determined in free solution as well as in the LIS of MDCK cells grown on permeable supports and the hindrance factor, theta, determined from the ratio of the free solution diffusivity to that in the LIS. The hindrance factors for 3000-MW dextran, 8-hydroxypyrene-1,3,6-trisulfonic acid (HPTS, MW 524) and N-2-hydroxyethylpiperazine-N'-2-ethanesulfonic acid (HEPES, MW 238) were not significantly different from 1. The diffusion of 10,000-MW dextran was substantially reduced in the LIS with a theta of 5.6 +/- 0.3. Enzymatic digestion by neuraminidase of the sialic acid residues of the glycosylation groups in the LIS increased the diffusivity of the 10,000-MW dextran 1.8-fold indicating hindrance by the glycocalyx. We conclude that small solutes, such as Na(+) and Cl(-), would not be significantly restricted in their diffusion in the LIS and that solute concentration gradients could not develop along the LIS under physiologic conditions.

摘要

利用紫外激光脉冲释放笼形化合物后产生的荧光扩散,测定了在可渗透支持物上培养的肾细胞(MDCK)侧向细胞间隙(LIS)中分子量范围为238至10,000的四种溶质的扩散系数。进行了两种类型的实验:释放笼形荧光团后荧光变化速率的测量,以及由染料的未笼形配体扩散产生的相对静态荧光染料荧光变化的测量。通过对多通道光电倍增管的输出进行光子计数来确定荧光强度。在游离溶液以及在可渗透支持物上生长的MDCK细胞的LIS中测定扩散系数,并根据游离溶液扩散率与LIS中扩散率的比值确定阻碍因子θ。3000分子量葡聚糖、8-羟基芘-1,3,6-三磺酸(HPTS,分子量524)和N-2-羟乙基哌嗪-N'-2-乙磺酸(HEPES,分子量238)的阻碍因子与1没有显著差异。10,000分子量葡聚糖在LIS中的扩散显著降低,θ为5.6±0.3。用神经氨酸酶对LIS中糖基化基团的唾液酸残基进行酶消化,使10,000分子量葡聚糖的扩散率增加了1.8倍,表明糖萼起到了阻碍作用。我们得出结论,小溶质,如Na(+)和Cl(-),在LIS中的扩散不会受到显著限制,并且在生理条件下溶质浓度梯度不会沿LIS形成。

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