Bilaminar Co-culture of Primary Rat Cortical Neurons and Glia

Shimizu, Saori; Abt, Anna; Meucci, Olimpia

doi:10.3791/3257

Cited by 20 publications

(26 citation statements)

References 14 publications

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“…Neurons can be cocultured with endotheliocytes and astrocytes to mimic neurovascular units in vitro [16] for the purposes of studying the blood-brain barrier [17]. Every neurodevelopmental stage can be studied depending on the culture time [18].…”

Section: Discussionmentioning

confidence: 99%

A Modified Technique for Culturing Primary Fetal Rat Cortical Neurons

Zhong

et al. 2012

Journal of Biomedicine and Biotechnology

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The study explored a modified primary culture system for fetal rat cortical neurons. Day E18 embryos from pregnant Sprague Dawley rats were microdissected under a stereoscope. To minimize enzymatic damage to the cultured neurons, we applied a sequential digestion protocol using papain and Dnase I. The resulting sifted cell suspension was seeded at a density of 50,000 cells per cm2 onto 0.1 mg/mL L-PLL-covered vessels. After a four-hour incubation in high-glucose Dulbecco's Modified Eagle's Medium (HG-DMEM) to allow the neurons to adhere, the media was changed to neurobasal medium that was refreshed by changing half of the volume after three days followed by a complete medium change every week. The cells displayed progressively robust neurite extension, and nonneuronal-like cells could barely be detected by five days in vitro (DIV); cell growth was still substantial at 14 DIV. Neurons were identified by β-tubulin III immunofluorescence, and neuronal purity within the cultures was assessed at over 95% by both flow cytometry and by dark-field counting of β-tubulin III-positive cells. These results suggest that the protocol was successful and that the high purity of neurons in this system could be used as the basis for generating various cell models of neurological disease.

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Section: Discussionmentioning

confidence: 99%

A Modified Technique for Culturing Primary Fetal Rat Cortical Neurons

Zhong

et al. 2012

Journal of Biomedicine and Biotechnology

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“…Rat cortical neurons were cultured in the presence of a glial feeder layer, using the previously described bilaminar cell culture model (73). Due to the presence of glia, this culture system largely preserves the in vivo mechanisms of neuronal growth and differentiation, but also allows for direct studies on neurons, which were separated from glia at the time of analysis.…”

Section: Methodsmentioning

confidence: 99%

Neuronal ferritin heavy chain and drug abuse affect HIV-associated cognitive dysfunction

Pitcher¹,

Abt²,

Myers³

et al. 2014

J. Clin. Invest.

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Interaction of the chemokine CXCL12 with its receptor CXCR4 promotes neuronal function and survival during embryonic development and throughout adulthood. Previous studies indicated that μ-opioid agonists specifically elevate neuronal levels of the protein ferritin heavy chain (FHC), which negatively regulates CXCR4 signaling and affects the neuroprotective function of the CXCL12/CXCR4 axis. Here, we determined that CXCL12/CXCR4 activity increased dendritic spine density, and also examined FHC expression and CXCR4 status in opiate abusers and patients with HIV-associated neurocognitive disorders (HAND), which is typically exacerbated by illicit drug use. Drug abusers and HIV patients with HAND had increased levels of FHC, which correlated with reduced CXCR4 activation, within cortical neurons. We confirmed these findings in a nonhuman primate model of SIV infection with morphine administration. Transfection of a CXCR4-expressing human cell line with an iron-deficient FHC mutant confirmed that increased FHC expression deregulated CXCR4 signaling and that this function of FHC was independent of iron binding. Furthermore, examination of morphine-treated rodents and isolated neurons expressing FHC shRNA revealed that FHC contributed to morphine-induced dendritic spine loss. Together, these data implicate FHC-dependent deregulation of CXCL12/CXCR4 as a contributing factor to cognitive dysfunction in neuroAIDS.

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“…Support Protocol 2 describes how to prepare primary astrocyte cultures from brains of rat pups (2 to 4 days old). This protocol is adapted from Kortagere et al (2018) and Shimizu, Abt, & Meucci (2011).…”

Section: Primary Astrocyte Culturementioning

confidence: 99%

Protocols for Measuring Glutamate Uptake: Dose‐Response and Kinetic Assays in In Vitro and Ex Vivo Systems

Fontana

2018

CP Pharmacology

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This article presents detailed descriptions of procedures and troubleshooting tips for basic in vitro and ex vivo uptake assays for the functional characterization of glutamate transporters and the assessment of the effect of compounds that modulate their activity. Assays are performed in cell lines that transiently or stably express a particular transporter under investigation, in primary cultures of astrocytes, or in ex vivo synaptosomal preparations that endogenously express these transporters. Two main assays are described, including dose-response assays to measure potencies of test compounds for stimulation or inhibition of function (EC or IC values, respectively) and kinetic functional assays to calculate apparent affinity (K ) and maximal velocity (V ) of radiolabeled substrate uptake into the cells. The methods described use glutamate transporters as an example; however, the protocols can be adapted to other neurotransmitter transporters using their respective substrates (e.g., GABA uptake through GATs, serotonin uptake through SERTs, among others). © 2018 by John Wiley & Sons, Inc.

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Bilaminar Co-culture of Primary Rat Cortical Neurons and Glia

Cited by 20 publications

References 14 publications

A Modified Technique for Culturing Primary Fetal Rat Cortical Neurons

A Modified Technique for Culturing Primary Fetal Rat Cortical Neurons

Neuronal ferritin heavy chain and drug abuse affect HIV-associated cognitive dysfunction

Protocols for Measuring Glutamate Uptake: Dose‐Response and Kinetic Assays in In Vitro and Ex Vivo Systems

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