Abstract
Astrocytes are a major cell type in the mammalian CNS. Astrocytes are now known to play a number of essential roles in processes including synapse formation and function, as well as blood-brain barrier formation and control of cerebral blood flow. However, our understanding of the molecular mechanisms underlying astrocyte development and function is still rudimentary. This lack of knowledge is at least partly due to the lack of tools currently available for astrocyte biology. ACSA-2 is a commercially available antibody originally developed for the isolation of astrocytes from young postnatal mouse brain, using magnetic cell-sorting methods, but its utility in isolating cells from adult tissue has not yet been published. Using a modified protocol, we now show that this tool can also be used to isolate ultrapure astrocytes from the adult brain. Furthermore, using a variety of techniques (including single-cell sequencing, overexpression and knockdown assays, immunoblotting, and immunohistochemistry), we identify the ACSA-2 epitope for the first time as ATP1B2 and characterize its distribution in the CNS. Finally, we show that ATP1B2 is stably expressed in multiple models of CNS injury and disease. Hence, we show that the ACSA-2 antibody possesses the potential to be an extremely valuable tool for astrocyte research, allowing the purification and characterization of astrocytes (potentially including injury and disease models) without the need for any specialized and expensive equipment. In fact, our results suggest that ACSA-2 should be a first-choice method for astrocyte isolation and characterization.
Highlights
Astrocytes are a major cell type in the mammalian central nervous system (CNS)
ACSA-2 is a commercial antibody from Miltenyi Biotec, which is marketed for the one-step isolation of astrocytes from young mice
We decided to test the utility of ACSA-2 as a general tool for astrocyte biology
Summary
A major step forward in astrocyte research would be the ability to label and characterize astrocytes from both young postnatal and adult brain (including through immunoisolation). We found that additional myelin/oligodendrocyte depletion using a Miltenyi myelin removal kit solved this issue and that cell yield, viability, and purity was broadly comparable with that obtained from young brain (with the exception of a higher level of chondroitin sulfate proteoglycan (Cspg4) (which is a marker for oligodendrocyte precursors) To determine whether ACSA-2 labels all cortical astrocytes (or just a defined subset), we prepared a suspension of adult cortical cells from the Aldh1l1-EGFP mouse line, which is widely reported to express EGFP in all astrocytes [9]. This cell suspension was labeled with an ACSA-2-phycoerythrin (PE) conjugate and used for subsequent flow cytometry. Is it a commonly used astrocyte marker (such as GLT-1 or aquaporin 4) or a more “exotic” protein, which would give an additional, alternative option for astrocyte labeling and purification, depending on its distribu-
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