Activation of multiple receptors stimulates extracellular vesicle release from trophoblast cells

被引:10
作者
Conrad, Kirk P. [1 ,2 ,3 ]
Tuna, Kubra M. [1 ]
Mestre, Cathleen T. [1 ]
Banwatt, Esha S. [1 ]
Alli, Abdel A. [1 ,4 ]
机构
[1] Univ Florida, Coll Med, Dept Physiol & Funct Genom, 1600 SW Archer Rd,Box 100274,M552, Gainesville, FL 32610 USA
[2] Univ Florida, Coll Med, Dept Obstet & Gynecol, Gainesville, FL 32610 USA
[3] Univ Florida, DH Barron Reprod & Perinatal Biol Res Program, Gainesville, FL USA
[4] Univ Florida, Coll Med, Dept Med, Div Nephrol Hypertens & Renal Transplantat, Gainesville, FL USA
来源
PHYSIOLOGICAL REPORTS | 2020年 / 8卷 / 20期
关键词
angiotensin; bitter taste receptor; calcium; cholecystokinin; exosome; GPCR; muscarinic receptor; placenta; ANGIOTENSIN-II TYPE-1; EXOSOMES; SECRETION; MATURATION;
D O I
10.14814/phy2.14592
中图分类号
Q4 [生理学];
学科分类号
071003 ;
摘要
Reports of the stimulated release of extracellular vesicles (EVs) are few, and the mechanisms incompletely understood. To our knowledge, the possibility that the activation of any one of the multitudes of G-protein-coupled receptors (GPCRs) expressed by a single cell-type might increase EV release has not been explored. Recently, we identified the expression of cholecystokinin (CCK), gastrin, gastrin/cholecystokinin types A and/or B receptors (CCKAR and/or -BR), and the bitter taste receptor, TAS2R14 in the human and mouse placenta. specifically, trophoblast. These GPCR(s) were also expressed in four different human trophoblast cell lines. The current objective was to employ two of these cell lines-JAR choriocarcinoma cells and HTR-8/SVneo cells derived from first-trimester human villous trophoblast-to investigate whether CCK, TAS2R14 agonists, and other GPCR ligands would each augment EV release. EVs were isolated from the cell-culture medium by filtration and ultracentrifugation. The preparations were enriched in small EVs (<200 nm) as determined by syntenin western blot before and after sucrose gradient purification, phycoerythrin (PE)-ADAM10 antibody labeling, and electron microscopy. Activation of TAS2R14, CCKBR, cholinergic muscarinic 1 & 3, and angiotensin II receptors, each increased EV release by 4.91-, 2.79-, 1.87-, and 3.11-fold, respectively (all p < .05 versus vehicle controls), without significantly changing EV diameter. A progressive increase of EV concentration in conditioned medium was observed over 24 hr consistent with the release of preformed EVs and de novo biogenesis. Compared to receptor-mediated stimulation, EV release by the calcium ionophore, A23187, was less robust (1.63-fold, p = .08). Diphenhydramine, a TAS2R14 agonist, enhanced EV release in JAR cells at a concentration 10-fold below that required to increase intracellular calcium. CCK activation of HTR-8/SVneo cells, which did not raise intracellular calcium, increased EV release by 2.06-fold (p < .05). Taken together, these results suggested that other signaling pathways may underlie receptor-stimulated EV release besides, or in addition to, calcium. To our knowledge, the finding that the activation of multiple GPCRs can stimulate EV release from a single cell-type is unprecedented and engenders a novel thesis that each receptor may orchestrate intercellular communication through the release of EVs containing a subset of unique cargo, thus mobilizing a specific integrated physiological response by a network of neighboring and distant cells.
引用
收藏
页数:13
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