TAAR8 Mediates Increased Migrasome Formation by Cadaverine in RPE Cells

Author:

Kim Joon Bum1,Bae Ji-Eun2,Park Na Yeon1,Kim Yong Hwan1,Kim Seong Hyun1,Hyung Hyejin1,Yeom Eunbyul1,Choi Dong Kyu1,Jeong Kwiwan3,Cho Dong-Hyung14

Affiliation:

1. School of Life Sciences, BK21 FOUR KNU Creative BioResearch Group, Kyungpook National University, Daegu 41566, Republic of Korea

2. KNU G-LAMP Research Group, KNU Institute of Basic Sciences, College of Natural Sciences, Kyungpook National University, Daegu 41566, Republic of Korea

3. Bio Industry Department, Gyeonggido Business & Science Accelerator, Suwon 16229, Republic of Korea

4. Organelle Institute, Kyungpook National University, Daegu 41566, Republic of Korea

Abstract

Migrasomes, the newly discovered cellular organelles that form large vesicle-like structures on the retraction fibers of migrating cells, are thought to be involved in communication between neighboring cells, cellular content transfer, unwanted material shedding, and information integration. Although their formation has been described previously, the molecular mechanisms of migrasome biogenesis are largely unknown. Here, we developed a cell line that overexpresses GFP-tetraspanin4, enabling observation of migrasomes. To identify compounds that regulate migrasome activity in retinal pigment epithelial (RPE) cells, we screened a fecal chemical library and identified cadaverine, a biogenic amine, as a potent migrasome formation inducer. Compared with normal migrating cells, those treated with cadaverine had significantly more migrasomes. Putrescine, another biogenic amine, also increased migrasome formation. Trace amine-associated receptor 8 (TAAR8) depletion inhibited migrasome increase in cadaverine-treated RPE cells, and cadaverine also inhibited protein kinase A phosphorylation. In RPE cells, cadaverine triggers migrasome formation via a TAAR8-mediated protein kinase A signaling pathway.

Funder

Kyungpook National University Research Fund

Publisher

MDPI AG

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