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Adult brain isolation kit

Manufactured by Miltenyi Biotec
Sourced in Germany

The Adult Brain Isolation Kit is a laboratory product designed for the isolation of cells from adult brain tissue. The kit provides reagents and protocols to facilitate the extraction and purification of cells from adult brain samples.

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4 protocols using adult brain isolation kit

1

Isolation of Adult Mouse Neurons

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Adult mouse brain (from 6-month-old animals) tissue was dissociated with the Adult Brain Isolation Kit (Miltenyi). Dissociated cells, after removal of debris and red blood cells, neurons were separated with the Neuron Isolation Kit (Miltenyi). The identity of the isolated fraction was confirmed previously19 (link) by western blot against the neuronal marker microtubule-associated protein 2 (MAP2) and GFAP.
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2

Mouse brain cell isolation

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Adult mouse brain (from 6 months animals) tissue was dissociated with the Adult Brain Isolation Kit (Miltenyi Biotec). Neurons were separated in the dissociated cells, after removal of debris and red blood cells, and neurons were separated with the Neuron Isolation Kit (Miltenyi), according to the manufacturer’s protocol. The identity of the isolated fraction was confirmed previously (Lopez‐Fabuel et al, 2016 (link)) by Western blot against the neuronal marker microtubule‐associated protein 2 (MAP2).
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3

Isolation of Microglia from Adult Mouse Brains

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Adult mice were anesthetized and brains were harvested after heart perfusion with ice-cold Duchenne phosphate buffer. This was followed by tissue isolation, debris removal, and red blood cell removal, followed by single-cell suspension using an adult brain isolation kit (Miltenyi Biotec, Germany). Microglia were further isolated from single-cell suspensions using MACS separation columns (Miltenyi Biotec, Germany) and magnetic CD11b microbeads (Miltenyi Biotec, Germany).
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4

Microglia Isolation from Young and Aged Mice

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Primary microglia were isolated from the brains of young (3–4 months old) and aged (18–20 months old) female C57BL/6N mice as previously described16 (link). Briefly, we transcardially perfused on mice with sterile 1x PBS. Whole brain tissue was explanted and meninges were removed. Brain tissue was mechanically and enzymatically homogenized into a single cell suspension using the Miltenyi Adult Brain Isolation Kit (130–107-677) per the manufacturer’s instructions. Cell suspensions were strained with a 70 mm cell strainer and then resuspended in 6 mL of 75% stock isotonic percoll (SIP). A density gradient was then made by layering 5 mL of 35% SIP on top of the cell solution followed by 3 mL of 1x PBS. Density gradients were placed on ice for 15 minutes and then spun at 800 × g, 4°C, for 45 minutes with slow acceleration and no break. The top 2 layers were aspirated, and microglia were collected at the 75:35 SIP interface. Cells were then washed in 45 mL of sterile 1x PBS and resuspended in Dulbecco’s modified Eagle’s medium (DMEM) (11965–092 Sigma Aldrich) supplemented with 10% fetal bovine serum and 1% penicillin-streptomycin. Immediately following isolation, primary microglia were seeded in cell culture-treated chamber slides (154941, Thermo Fisher) for immunocytochemistry or 48 well cell culture plates (130187, Thermo Fisher) for flow cytometry at a density of 3×105 cells/cm2.
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