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Published September 24, 2010 | Supplemental Material + Published
Journal Article Open

Multispectral fingerprinting for improved in vivo cell dynamics analysis

Abstract

Background: Tracing cell dynamics in the embryo becomes tremendously difficult when cell trajectories cross in space and time and tissue density obscure individual cell borders. Here, we used the chick neural crest (NC) as a model to test multicolor cell labeling and multispectral confocal imaging strategies to overcome these roadblocks. Results: We found that multicolor nuclear cell labeling and multispectral imaging led to improved resolution of in vivo NC cell identification by providing a unique spectral identity for each cell. NC cell spectral identity allowed for more accurate cell tracking and was consistent during short term time-lapse imaging sessions. Computer model simulations predicted significantly better object counting for increasing cell densities in 3-color compared to 1-color nuclear cell labeling. To better resolve cell contacts, we show that a combination of 2-color membrane and 1-color nuclear cell labeling dramatically improved the semi-automated analysis of NC cell interactions, yet preserved the ability to track cell movements. We also found channel versus lambda scanning of multicolor labeled embryos significantly reduced the time and effort of image acquisition and analysis of large 3D volume data sets. Conclusions: Our results reveal that multicolor cell labeling and multispectral imaging provide a cellular fingerprint that may uniquely determine a cell's position within the embryo. Together, these methods offer a spectral toolbox to resolve in vivo cell dynamics in unprecedented detail.

Additional Information

© 2010 Kulesa et al; licensee BioMed Central Ltd. This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited. Received: 28 May 2010 Accepted: 24 September 2010. Published: 24 September 2010. We would like to thank Hua Li for consultation on statistical analysis of data and Winfried Wiegraebe and Joel Schwartz for helpful technical discussions. This work was funded by NIH grant 1R01HD057922 and the Stowers Institute for Medical Research. Authors' contributions RM, JMT, and MS performed all the embryo labeling, sample preparation, multispectral imaging, and image analysis in the DiI, GFP, and multi-color H2B-labeling experiments and cell tracking. CHJC and JMT performed all the embryo labeling, sample preparation, multispectral imaging, and image analysis in the multi-color cell membrane labeling experiments. RA designed and carried out the computational model simulations. RL provided many of the fluorescent protein constructs and participated in discussions of the experimental design strategy. PMK designed the research, analyzed data and wrote the paper. All authors read and approved the final manuscript.

Attached Files

Published - Kulesa2010p11724BMC_Dev_Biol.pdf

Supplemental Material - 1471-213x-10-101-s1.doc

Supplemental Material - 1471-213x-10-101-s2.avi

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Supplemental Material - 1471-213x-10-101-s5.tiff

Supplemental Material - 1471-213x-10-101-s6.tiff

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Created:
August 19, 2023
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