Simultaneous induction of vasculature and neuronal network formation on a chip reveals a dynamic interrelationship between cell types

Lotta Isosaari; Hanna Vuorenpää; Alma Yrjänäinen; Fikret Emre Kapucu; Minna Kelloniemi; Toni-Karri Pakarinen; Susanna Miettinen; Susanna Narkilahti

doi:10.1186/s12964-023-01159-4

Simultaneous induction of vasculature and neuronal network formation on a chip reveals a dynamic interrelationship between cell types

Cell Commun Signal. 2023 Jun 14;21(1):132. doi: 10.1186/s12964-023-01159-4.

Authors

Lotta Isosaari^{1

2

3}, Hanna Vuorenpää^{2

3}, Alma Yrjänäinen^{2

3}, Fikret Emre Kapucu¹, Minna Kelloniemi⁴, Toni-Karri Pakarinen⁵, Susanna Miettinen^{2

3}, Susanna Narkilahti⁶

Affiliations

¹ NeuroGroup, Faculty of Medicine and Health Technology, Tampere University, Tampere, Finland.
² Adult Stem Cell Group, Faculty of Medicine and Health Technology, Tampere University, Tampere, Finland.
³ Research, Development and Innovation Centre, Tampere University Hospital, Tampere, Finland.
⁴ Department of Plastic and Reconstructive Surgery, Tampere University Hospital, Tampere, Finland.
⁵ Regea Cell and Tissue Center, Tampere University, Tampere, Finland.
⁶ NeuroGroup, Faculty of Medicine and Health Technology, Tampere University, Tampere, Finland. susanna.narkilahti@tuni.fi.

Abstract

Background: Neuronal networks receive and deliver information to regulate bodily functions while the vascular network provides oxygen, nutrients, and signaling molecules to tissues. Neurovascular interactions are vital for both tissue development and maintaining homeostasis in adulthood; these two network systems align and reciprocally communicate with one another. Although communication between network systems has been acknowledged, the lack of relevant in vitro models has hindered research at the mechanistic level. For example, the current used in vitro neurovascular models are typically established to be short-term (≤ 7 days) culture models, and they miss the supporting vascular mural cells.

Methods: In this study, we utilized human induced pluripotent stem cell (hiPSC) -derived neurons, fluorescence tagged human umbilical vein endothelial cells (HUVECs), and either human bone marrow or adipose stem/stromal cells (BMSCs or ASCs) as the mural cell types to create a novel 3D neurovascular network-on-a-chip model. Collagen 1-fibrin matrix was used to establish long-term (≥ 14 days) 3D cell culture in a perfusable microphysiological environment.

Results: Aprotinin-supplemented endothelial cell growth medium-2 (EGM-2) supported the simultaneous formation of neuronal networks, vascular structures, mural cell differentiation, and the stability of the 3D matrix. The formed neuronal and vascular networks were morphologically and functionally characterized. Neuronal networks supported vasculature formation based on direct cell contacts and by dramatically increasing the secretion of angiogenesis-related factors in multicultures in contrast to cocultures without neurons. Both utilized mural cell types supported the formation of neurovascular networks; however, the BMSCs seemed to boost neurovascular networks to greater extent.

Conclusions: Overall, our study provides a novel human neurovascular network model that is applicable for creating in vivo-like tissue models with intrinsic neurovascular interactions. The 3D neurovascular network model on chip forms an initial platform for the development of vascularized and innervated organ-on-chip and further body-on-chip concepts and offers the possibility for mechanistic studies on neurovascular communication both under healthy and in disease conditions. Video Abstract.

Keywords: 3D cell culture; Angiogenesis; Cellular communication; Human cells; Microfluidic; Neurovascular interactions.

Publication types

Video-Audio Media
Research Support, Non-U.S. Gov't

MeSH terms

Cell Differentiation
Homeostasis
Human Umbilical Vein Endothelial Cells
Humans
Induced Pluripotent Stem Cells*
Lab-On-A-Chip Devices