In vivo longitudinal visualization of bone marrow engraftment process in mouse calvaria using two-photon microscopy

Intravital microscopy of mouse calvarial bone marrow (BM) is a powerful method for studying hematopoietic stem cells (HSCs) and the BM microenvironment at the cellular level. However, the current method used to access the mouse calvaria allows for only a few imaging times in the same mouse because o...

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Published inScientific reports Vol. 7; no. 1; p. 44097
Main Authors Le, Viet-Hoan, Lee, Seunghun, Lee, Seungwon, Wang, Taejun, Hyuk Jang, Won, Yoon, Yeoreum, Kwon, Soonjae, Kim, Hyekang, Lee, Seung-Woo, Hean Kim, Ki
Format Journal Article
LanguageEnglish
Published London Nature Publishing Group UK 09.03.2017
Nature Publishing Group
Subjects
13/100
631/1647/328/2057
631/532/1542
64/110
Animals
Bone marrow
Bone Marrow - metabolism
Bone Marrow - pathology
Calvaria
Dental cement
Dental Cements - pharmacology
Engraftment
Female
Humanities and Social Sciences
Mice
Microscopy
Microscopy, Fluorescence, Multiphoton - methods
multidisciplinary
Osteogenesis
Rodents
Science
Skull - injuries
Skull - metabolism
Skull - pathology
Stem cell transplantation
Stem cells
Transplantation
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Summary:Intravital microscopy of mouse calvarial bone marrow (BM) is a powerful method for studying hematopoietic stem cells (HSCs) and the BM microenvironment at the cellular level. However, the current method used to access the mouse calvaria allows for only a few imaging times in the same mouse because of scar formation and inflammation induced by multiple surgeries. Longitudinal imaging of the BM may help better understand its microenvironment. In this study, a mouse calvarial window model was developed for longitudinal imaging that involves attaching a cover glass window onto the mouse calvaria and sealing the surrounding exposed area with cyanoacrylate glue and dental cement. The model was used for the longitudinal two-photon microscopy (TPM) imaging of the BM engraftment process. The same BM cavity sites were imaged multiple times over 4 weeks after BM transplantation (BMT). Temporal changes in the BM microenvironment, such as the reconstitution of transplanted BM cells and the recovery of vasculature, were observed and analysed qualitatively and quantitatively. Longitudinal intravital microscopy using the mouse calvarial window model was successfully demonstrated and may be useful for further BM studies.
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ISSN:2045-2322
2045-2322
DOI:10.1038/srep44097