Development of a hollow fibre-based renal module for active transport studies

AbstractUnderstanding the active transport of substrates by the kidney in the renal proximal convoluted tubule is crucial for drug development and for studying kidney diseases. Currently, cell-based assays are applied for this this purpose, however, differences between assays and the body are common, indicating the importance of in vitro–in vivo discrepancies. Several studies have suggested that 3D cell cultures expose cells to a more physiological environments, thus, providing more accurate cell function results. To mimic the renal proximal tubule, we have developed a custom-made renal module (RM), containing a single polypropylene hollow fibre (Plasmaphan P1LX, 3M) that serves as a porous scaffold and compared to conventional Transwell cell-based bidirectional transport studies. In addition, a constant flow of media, exposed cells to a physiological shear stress of 0.2 dyne/cm2. MDCK-Mdr1a cells, overexpressing the rat Mdr1a (P-gp) transporter, were seeded onto the HF membrane surface coated with the basement membrane matrix Geltrex which facilitated cell adhesion and tight junction formation. Cells were then seeded into the HF lumen where attachment and tight junction formation were evaluated by fluorescence microscopy while epithelial barrier integrity under shear stress was shown to be achieved by day 7. qPCR results have shown significant changes in gene expression compared to cells grown on Transwells. Kidney injury marker such as KIM-1 and the hypoxia marker CA9 have been downregulated, while the CD133 (Prominin-1) microvilli marker has shown a fivefold upregulation. Furthermore, the renal transporter P-gp expression has been downregulated by 50%. Finally, bidirectional assays have shown that cells grown in the RM were able to reabsorb albumin with a higher efficiency compared to Transwell cell cultures while efflux of the P-gp-specific substrates Hoechst and Rhodamine 123 was decreased. These results further support the effect of the microenvironment and fluidic shear stress on cell function and gene expression. This can serve as the basis for the development of a microphysiological renal model for drug transport studies.

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S14.3. Glycosaminoglycan and collagen syntheses and tight junction formation of endothelial cells under shear stress

Biorheology ◽

10.1016/0006-355x(95)92024-5 ◽

1995 ◽

Vol 32 (2-3) ◽

pp. 157-157

Author(s):

M MITSUMATA ◽

T YAMANE ◽

T ARISAKA ◽

M KAWASUMI ◽

S WANG ◽

...

Keyword(s):

Endothelial Cells ◽

Shear Stress ◽

Tight Junction ◽

Tight Junction Formation ◽

Junction Formation

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Disruption of the cingulin gene does not prevent tight junction formation but alters gene expression

Journal of Cell Science ◽

10.1242/jcs.01399 ◽

2004 ◽

Vol 117 (22) ◽

pp. 5245-5256 ◽

Cited By ~ 60

Author(s):

L. Guillemot

Keyword(s):

Gene Expression ◽

Tight Junction ◽

Tight Junction Formation ◽

Junction Formation

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A novel role of Adam 10 in tight junction formation during mouse preimplantation development

Reproduction Abstracts ◽

10.1530/repabs.3.o009 ◽

2016 ◽

Author(s):

Inchul Choi ◽

Ye-lin Jeong

Keyword(s):

Tight Junction ◽

Preimplantation Development ◽

Tight Junction Formation ◽

Junction Formation

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Faculty Opinions recommendation of Adherens junctions influence tight junction formation via changes in membrane lipid composition.

Faculty Opinions – Post-Publication Peer Review of the Biomedical Literature ◽

10.3410/f.733156815.793546174 ◽

2018 ◽

Author(s):

Ronen Alon

Keyword(s):

Tight Junction ◽

Lipid Composition ◽

Adherens Junctions ◽

Membrane Lipid ◽

Membrane Lipid Composition ◽

Tight Junction Formation ◽

Junction Formation

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Faculty Opinions recommendation of LSR defines cell corners for tricellular tight junction formation in epithelial cells.

Faculty Opinions – Post-Publication Peer Review of the Biomedical Literature ◽

10.3410/f.7980962.8351066 ◽

2011 ◽

Author(s):

Asma Nusrat ◽

Stefan Koch

Keyword(s):

Epithelial Cells ◽

Tight Junction ◽

Tight Junction Formation ◽

Junction Formation

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Effect of 3D-Fibroblast Dermis Constructed by Layer-by-Layer Cell Coating Technique on Tight Junction Formation and Function in Full-Thickness Skin Equivalent

ACS Biomaterials Science & Engineering ◽

10.1021/acsbiomaterials.1c00375 ◽

2021 ◽

Author(s):

Masato Murakami ◽

Takami Akagi ◽

Yumi Sasano ◽

Mitsuru Akashi

Keyword(s):

Tight Junction ◽

Layer By Layer ◽

Full Thickness ◽

Coating Technique ◽

Layer Cell ◽

Tight Junction Formation ◽

Thickness Skin ◽

Junction Formation ◽

Cell Coating ◽

And Function

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Participation of plasma membrane proteins in the formation of tight junction by cultured epithelial cells

The Journal of Cell Biology ◽

10.1083/jcb.96.3.693 ◽

1983 ◽

Vol 96 (3) ◽

pp. 693-702 ◽

Cited By ~ 62

Author(s):

EB Griepp ◽

WJ Dolan ◽

ES Robbins ◽

DD Sabatini

Keyword(s):

Protein Synthesis ◽

Steady State ◽

Tight Junction ◽

Messenger Rna ◽

Freeze Fracture ◽

Epithelial Cell Line ◽

Experimental Conditions ◽

Tight Junction Formation ◽

Junction Formation ◽

Spinner Culture

Measurements of the transepithelial electrical resistance correlated with freeze-fracture observations have been used to study the process of tight junction formation under various experimental conditions in monolayers of the canine kidney epithelial cell line MDCK. Cells derived from previously confluent cultures and plated immediately after trypsin- EDTA dissociation develop a resistance that reaches its maximum value of several hundred ohms-cm(2) after approximately 24 h and falls to a steady-state value of 80-150 ohms- cm(2) by 48 h. The rise in resistance and the development of tight junctions can be completely and reversibly prevented by the addition of 10 μg/ml cycloheximide at the time of plating, but not when this inhibitor is added more than 10 h after planting. Thus tight junction formation consists of separable synthetic and assembly phases. These two phases can also be dissociated and the requirement for protein synthesis after plating eliminated if, following trypsinization, the cells are maintained in spinner culture for 24 h before plating. The requirement for protein synthesis is restored, however, if cells maintained in spinner culture are treated with trypsin before plating. Actinomycin D prevents development of resistance only in monolayers formed from cells derived from sparse rather than confluent cultures, but new mRNA synthesis is not required if cells obtained from sparse cultures are maintained for 24 h in spinner culture before plating. Once a steady-state resistance has been reached, its maintenance does not require either mRNA or protein synthesis; in fact, inhibition of protein synthesis causes a rise in the resistance over a 30-h period. Following treatments that disrupt the junctions in steady- state monolayers recovery of resistance also does not require protein synthesis. These observations suggest that proteins are involved in tight junction formation. Such proteins, which do not turn over rapidly under steady-state conditions, are destroyed by trypsinization and can be resynthesized in the absence of stable cell-cell or cell-substratum contact. Messenger RNA coding for proteins involved in tight junction formation is stable except when cells are sparsely plated, and can also be synthesized without intercellular contacts or cell-substratum attachment.

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Tight junction protein cingulin is expressed by maternal and embryonic genomes during early mouse development

Development ◽

10.1242/dev.117.3.1145 ◽

1993 ◽

Vol 117 (3) ◽

pp. 1145-1151 ◽

Cited By ~ 3

Author(s):

Q. Javed ◽

T.P. Fleming ◽

M. Hay ◽

S. Citi

Keyword(s):

Tight Junction ◽

Cell Mass ◽

Preimplantation Embryos ◽

Cell Contact ◽

Mouse Development ◽

Early Cleavage ◽

Cell Stage ◽

Tight Junction Formation ◽

Junction Protein ◽

Junction Formation

The expression of the tight junction peripheral membrane protein, cingulin (140 × 10(3) M(r), was investigated in mouse eggs and staged preimplantation embryos by immunoblotting and immunoprecipitation. Polyclonal antibody to chicken brush cingulin detected a single 140 × 10(3) M(r) protein in immunoblots of unfertilised eggs and all preimplantation stages. Relative protein levels were high in eggs and early cleavage stages, declined during later cleavage and increased again in expanding blastocysts. Quantitative immunoprecipitation of metabolically labelled eggs and staged embryos also revealed a biphasic pattern for cingulin synthesis with relative net levels being high in unfertilised eggs, minimal during early cleavage, rising 2.3-fold specifically at the onset of compaction (8-cell stage, when tight junction formation begins), and increasing further at a linear rate during morula and blastocyst stages. Cingulin synthesis in eggs is not influenced by fertilisation (or aging, if unfertilised), but this level declines sharply after first cleavage. These results indicate that cingulin is expressed by both maternal and embryonic genomes. The turnover of maternal cingulin (unfertilised eggs) and embryonic cingulin at a stage before tight junction formation begins (4-cell stage) is higher (t1/2 approximately 4 hours) than cingulin synthesised after tight junction formation (blastocysts; t1/2 approximately 10 hours). This increase in cingulin stability is reversed in the absence of extracellular calcium. Cingulin synthesis is also tissue-specific in blastocysts, being up-regulated in trophectoderm and down-regulated in the inner cell mass. Taken together, the results suggest that (i) cingulin may have a role during oogenesis and (ii) cell-cell contact patterns regulate cingulin biosynthesis during early morphogenesis, contributing to lineage-specific epithelial maturation.

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