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Studying M1 and M2 states in adult microglia.
Gaikwad, Sadanand M; HENEKA, Michael
2013In Methods in Molecular Biology, 1041, p. 185 - 197
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Keywords :
Animals; Cells, Cultured; Flow Cytometry; Mice; Mice, Inbred C57BL; Mice, Transgenic; Microglia/metabolism; Adult microglia; Alzheimer; Cytokine; Inflammatory gene; M1/M2 phenotype; Neurodegeneration; Neuroinflammation; Molecular Biology; Genetics
Abstract :
[en] Microglial cell function receives increasing interest. To date, the majority of experiments are performed by using immortalized microglia-like cells or primary microglia prepared from pre- or postnatal rodent brain. As those may not adequately reflect the microglial biology in the adult brain, this protocol advocates a procedure which allows for the isolation, purification, and subsequent analysis of microglial cells. Once isolated, the principal state of activation, M1 or M2, can be determined in adult microglia using fluorescence-activated cell sorting, quantitative PCR, and/or Western blotting. Likewise, adult microglia generated by this protocol can be used for functional analysis through cell cultivation for a limited time.
Disciplines :
Neurology
Author, co-author :
Gaikwad, Sadanand M;  University of Bonn, Bonn, Germany
HENEKA, Michael  ;  Clinical Neuroscience Unit, Department of Neurology, University of Bonn, Bonn, Germany
External co-authors :
yes
Language :
English
Title :
Studying M1 and M2 states in adult microglia.
Publication date :
2013
Journal title :
Methods in Molecular Biology
ISSN :
1064-3745
eISSN :
1940-6029
Publisher :
Humana Press, United States
Volume :
1041
Pages :
185 - 197
Peer reviewed :
Peer Reviewed verified by ORBi
Available on ORBilu :
since 22 July 2024

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