Detail
Article
Online article
FT
Medvik - BMC
  • Something wrong with this record ?

Modelling the maternal-fetal interface: An in vitro approach to investigate nutrient and drug transport across the human placenta

B. Fuenzalida, V. Basler, N. Koechli, N. Yi, F. Staud, C. Albrecht

. 2024 ; 28 (20) : e70151. [pub] -

Language English Country England, Great Britain

Document type Journal Article

Persistent link   https://www.medvik.cz/link/bmc25003972

Grant support
OC-2019-019 Swiss 3R Competence Centre
310030_197408 Swiss National Science Foundation - Switzerland

The placenta plays a critical role in maternal-fetal nutrient transport and fetal protection against drugs. Creating physiological in vitro models to study these processes is crucial, but technically challenging. This study introduces an efficient cell model that mimics the human placental barrier using co-cultures of primary trophoblasts and primary human umbilical vein endothelial cells (HUVEC) on a Transwell®-based system. Monolayer formation was examined over 7 days by determining transepithelial electrical resistance (TEER), permeability of Lucifer yellow (LY) and inulin, localization of transport proteins at the trophoblast membrane (immunofluorescence), and syncytialization markers (RT-qPCR/ELISA). We analysed diffusion-based (caffeine/antipyrine) and transport-based (leucine/Rhodamine-123) processes to study the transfer of physiologically relevant compounds. The latter relies on the adequate localization and function of the amino-acid transporter LAT1 and the drug transporter P-glycoprotein (P-gp) which were studied by immunofluorescence microscopy and application of respective inhibitors (2-Amino-2-norbornanecarboxylic acid (BCH) for LAT1; cyclosporine-A for P-gp). The formation of functional monolayer(s) was confirmed by increasing TEER values, low LY transfer rates, minimal inulin leakage, and appropriate expression/release of syncytialization markers. These results were supported by microscopic monitoring of monolayer formation. LAT1 was identified on the apical and basal sides of the trophoblast monolayer, while P-gp was apically localized. Transport assays confirmed the inhibition of LAT1 by BCH, reducing both intracellular leucine levels and leucine transport to the basal compartment. Inhibiting P-gp with cyclosporine-A increased intracellular Rhodamine-123 concentrations. Our in vitro model mimics key aspects of the human placental barrier. It represents a powerful tool to study nutrient and drug transport mechanisms across the placenta, assisting in evaluating safer pregnancy therapies.

References provided by Crossref.org

000      
00000naa a2200000 a 4500
001      
bmc25003972
003      
CZ-PrNML
005      
20250206104830.0
007      
ta
008      
250121s2024 enk f 000 0|eng||
009      
AR
024    7_
$a 10.1111/jcmm.70151 $2 doi
035    __
$a (PubMed)39422159
040    __
$a ABA008 $b cze $d ABA008 $e AACR2
041    0_
$a eng
044    __
$a enk
100    1_
$a Fuenzalida, Barbara $u Institute of Biochemistry and Molecular Medicine, Faculty of Medicine, University of Bern, Bern, Switzerland
245    10
$a Modelling the maternal-fetal interface: An in vitro approach to investigate nutrient and drug transport across the human placenta / $c B. Fuenzalida, V. Basler, N. Koechli, N. Yi, F. Staud, C. Albrecht
520    9_
$a The placenta plays a critical role in maternal-fetal nutrient transport and fetal protection against drugs. Creating physiological in vitro models to study these processes is crucial, but technically challenging. This study introduces an efficient cell model that mimics the human placental barrier using co-cultures of primary trophoblasts and primary human umbilical vein endothelial cells (HUVEC) on a Transwell®-based system. Monolayer formation was examined over 7 days by determining transepithelial electrical resistance (TEER), permeability of Lucifer yellow (LY) and inulin, localization of transport proteins at the trophoblast membrane (immunofluorescence), and syncytialization markers (RT-qPCR/ELISA). We analysed diffusion-based (caffeine/antipyrine) and transport-based (leucine/Rhodamine-123) processes to study the transfer of physiologically relevant compounds. The latter relies on the adequate localization and function of the amino-acid transporter LAT1 and the drug transporter P-glycoprotein (P-gp) which were studied by immunofluorescence microscopy and application of respective inhibitors (2-Amino-2-norbornanecarboxylic acid (BCH) for LAT1; cyclosporine-A for P-gp). The formation of functional monolayer(s) was confirmed by increasing TEER values, low LY transfer rates, minimal inulin leakage, and appropriate expression/release of syncytialization markers. These results were supported by microscopic monitoring of monolayer formation. LAT1 was identified on the apical and basal sides of the trophoblast monolayer, while P-gp was apically localized. Transport assays confirmed the inhibition of LAT1 by BCH, reducing both intracellular leucine levels and leucine transport to the basal compartment. Inhibiting P-gp with cyclosporine-A increased intracellular Rhodamine-123 concentrations. Our in vitro model mimics key aspects of the human placental barrier. It represents a powerful tool to study nutrient and drug transport mechanisms across the placenta, assisting in evaluating safer pregnancy therapies.
650    _2
$a lidé $7 D006801
650    _2
$a ženské pohlaví $7 D005260
650    _2
$a těhotenství $7 D011247
650    12
$a trofoblasty $x metabolismus $7 D014327
650    12
$a placenta $x metabolismus $7 D010920
650    12
$a maternofetální výměna látek $7 D008431
650    _2
$a biologický transport $7 D001692
650    12
$a endoteliální buňky pupečníkové žíly (lidské) $x metabolismus $7 D061307
650    _2
$a kokultivační techniky $7 D018920
650    _2
$a P-glykoprotein $x metabolismus $7 D020168
650    _2
$a biologické modely $7 D008954
650    _2
$a rhodamin 123 $x metabolismus $7 D020112
650    _2
$a leucin $x metabolismus $7 D007930
650    _2
$a inulin $x metabolismus $7 D007444
650    _2
$a isochinoliny $7 D007546
655    _2
$a časopisecké články $7 D016428
700    1_
$a Basler, Virginia $u Institute of Biochemistry and Molecular Medicine, Faculty of Medicine, University of Bern, Bern, Switzerland
700    1_
$a Koechli, Nadja $u Institute of Biochemistry and Molecular Medicine, Faculty of Medicine, University of Bern, Bern, Switzerland
700    1_
$a Yi, Nan $u Institute of Biochemistry and Molecular Medicine, Faculty of Medicine, University of Bern, Bern, Switzerland
700    1_
$a Staud, Frantisek $u Department of Pharmacology and Toxicology, Faculty of Pharmacy in Hradec Kralove, Charles University, Hradec Kralove, Czech Republic
700    1_
$a Albrecht, Christiane $u Institute of Biochemistry and Molecular Medicine, Faculty of Medicine, University of Bern, Bern, Switzerland $1 https://orcid.org/0000000278466930
773    0_
$w MED00006785 $t Journal of cellular and molecular medicine $x 1582-4934 $g Roč. 28, č. 20 (2024), s. e70151
856    41
$u https://pubmed.ncbi.nlm.nih.gov/39422159 $y Pubmed
910    __
$a ABA008 $b sig $c sign $y - $z 0
990    __
$a 20250121 $b ABA008
991    __
$a 20250206104826 $b ABA008
999    __
$a ok $b bmc $g 2263613 $s 1239979
BAS    __
$a 3
BAS    __
$a PreBMC-MEDLINE
BMC    __
$a 2024 $b 28 $c 20 $d e70151 $e - $i 1582-4934 $m Journal of cellular and molecular medicine $n J Cell Mol Med $x MED00006785
GRA    __
$a OC-2019-019 $p Swiss 3R Competence Centre
GRA    __
$a 310030_197408 $p Swiss National Science Foundation $2 Switzerland
LZP    __
$a Pubmed-20250121
Back

Find record

Citation metrics

Archiving options