| Literature DB >> 31091456 |
Marieke Meijer1, Kristina Rehbach2, Jessie W Brunner3, Jessica A Classen3, Hanna C A Lammertse1, Lola A van Linge3, Desiree Schut1, Tamara Krutenko4, Matthias Hebisch4, L Niels Cornelisse1, Patrick F Sullivan5, Michael Peitz6, Ruud F Toonen3, Oliver Brüstle7, Matthijs Verhage8.
Abstract
Synaptic dysfunction is associated with many brain disorders, but robust human cell models to study synaptic transmission and plasticity are lacking. Instead, current in vitro studies on human neurons typically rely on spontaneous synaptic events as a proxy for synapse function. Here, we describe a standardized in vitro approach using human neurons cultured individually on glia microdot arrays that allow single-cell analysis of synapse formation and function. We show that single glutamatergic or GABAergic forebrain neurons differentiated from human induced pluripotent stem cells form mature synapses that exhibit robust evoked synaptic transmission. These neurons show plasticity features such as synaptic facilitation, depression, and recovery. Finally, we show that spontaneous events are a poor predictor of synaptic maturity and do not correlate with the robustness of evoked responses. This methodology can be deployed directly to evaluate disease models for synaptic dysfunction and can be leveraged for drug development and precision medicine.Entities:
Keywords: NGN2; forward programming; human neuron; iPSC; single-cell model; synapse; synaptic dysfunction; synaptic plasticity; synaptic transmission; synaptopathy
Year: 2019 PMID: 31091456 DOI: 10.1016/j.celrep.2019.04.058
Source DB: PubMed Journal: Cell Rep Impact factor: 9.423