Brain stem cell division and maintenance studied using multi-isotope imaging mass spectrometry (MIMS)

G Enikolopov; C Guillermier; M Wang; L Trakimas; M Steinhauser; C Lechene

doi:10.1002/sia.5675

Brain stem cell division and maintenance studied using multi-isotope imaging mass spectrometry (MIMS)

Surf Interface Anal. 2014 Nov 1;46(Suppl 1):140-143. doi: 10.1002/sia.5675.

Authors

G Enikolopov¹, C Guillermier², M Wang³, L Trakimas⁴, M Steinhauser⁵, C Lechene²

Affiliations

¹ Cold Spring Harbor Laboratory, Cold Spring Harbor, NY USA.
² Division of Genetics, Brigham and Women's Hospital and Harvard Medical School, Boston, MA USA ; National Resource for Imaging Mass Spectrometry (NRIMS), Cambridge, MA USA.
³ National Resource for Imaging Mass Spectrometry (NRIMS), Cambridge, MA USA.
⁴ Department of Cell Biology, Harvard Medical School, Boston, MA USA.
⁵ Division of Genetics, Brigham and Women's Hospital and Harvard Medical School, Boston, MA USA ; Division of Cardiovascular Medicine, Brigham and Women's Hospital, Boston, MA USA.

Abstract

New neurons are continuously produced from neural stem cells in specific regions of the adult brain of animals and humans. In the hippocampus, a region crucial for cognitive function, neurogenesis responds to a multitude of extrinsic stimuli; emerging evidence indicates that it may be important for behavior, pathophysiology, brain repair, and response to drugs. We have developed an approach to identify and quantify the cellular targets of pro- and anti-neurogenic stimuli, based on reporter transgenic mouse lines in which neural stem and progenitor cells or their progeny are marked by fluorescent proteins. Here, we demonstrate the feasibility of using MIMS for studying adult neurogenesis.

Keywords: Hippocampus; MIMS; Multi-isotope Imaging Mass Spectrometry; Stem cell division.

Abstract

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