Literature DB >> 22677164

Quantitative evaluation of MRI-based tracking of ferritin-labeled endogenous neural stem cell progeny in rodent brain.

Greetje Vande Velde1, Janaki Raman Rangarajan, Ruth Vreys, Caroline Guglielmetti, Tom Dresselaers, Marleen Verhoye, Annemie Van der Linden, Zeger Debyser, Veerle Baekelandt, Frederik Maes, Uwe Himmelreich.   

Abstract

Endogenous neural stem cells have the potential to facilitate therapy for various neurodegenerative brain disorders. To increase our understanding of neural stem and progenitor cell biology in healthy and diseased brain, methods to label and visualize stem cells and their progeny in vivo are indispensable. Iron oxide particle based cell-labeling approaches enable cell tracking by MRI with high resolution and good soft tissue contrast in the brain. However, in addition to important concerns about unspecific labeling and low labeling efficiency, the dilution effect upon cell division is a major drawback for longitudinal follow-up of highly proliferating neural progenitor cells with MRI. Stable viral vector-mediated marking of endogenous stem cells and their progeny with a reporter gene for MRI could overcome these limitations. We stably and efficiently labeled endogenous neural stem/progenitor cells in the subventricular zone in situ by injecting a lentiviral vector expressing ferritin, a reporter for MRI. We developed an image analysis pipeline to quantify MRI signal changes at the level of the olfactory bulb as a result of migration of ferritin-labeled neuroblasts along the rostral migratory stream. We were able to detect ferritin-labeled endogenous neural stem cell progeny into the olfactory bulb of individual animals with ex vivo MRI at 30 weeks post injection, but could not demonstrate reliable in vivo detection and longitudinal tracking of neuroblast migration to the OB in individual animals. Therefore, although LV-mediated labeling of endogenous neural stem and progenitor cells resulted in efficient and stable ferritin-labeling of stem cell progeny in the OB, even with quantitative image analysis, sensitivity remains a limitation for in vivo applications.
Copyright © 2012 Elsevier Inc. All rights reserved.

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Year:  2012        PMID: 22677164     DOI: 10.1016/j.neuroimage.2012.04.040

Source DB:  PubMed          Journal:  Neuroimage        ISSN: 1053-8119            Impact factor:   6.556


  28 in total

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Authors:  Anna V Naumova; Niranjan Balu; Vasily L Yarnykh; Hans Reinecke; Charles E Murry; Chun Yuan
Journal:  J Cardiovasc Pharmacol Ther       Date:  2014-03-30       Impact factor: 2.457

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Journal:  Proc Natl Acad Sci U S A       Date:  2013-12-17       Impact factor: 11.205

Review 4.  In vivo imaging of endogenous neural stem cells in the adult brain.

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Journal:  World J Stem Cells       Date:  2015-01-26       Impact factor: 5.326

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8.  PET imaging of neurogenic activity in the adult brain: Toward in vivo imaging of human neurogenesis.

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Journal:  Neurogenesis (Austin)       Date:  2017-02-06

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