Methodology for reconstructing early zebrafish development from in vivo multiphoton microscopy

Miguel A. Luengo-Oroz; Jose L. Rubio-Guivernau; Emmanuel Faure; Thierry Savy; Louise Duloquin; Nicolas Olivier; David Pastor; Maria Ledesma-Carbayo; Delphine Débarre; Paul Bourgine; Emmanuel Beaurepaire; Nadine Peyriéras; Andres Santos

doi:10.1109/TIP.2011.2177911

Methodology for reconstructing early zebrafish development from in vivo multiphoton microscopy

Miguel A. Luengo-Oroz
, Jose L. Rubio-Guivernau
, Emmanuel Faure
, Thierry Savy
, Louise Duloquin
, Nicolas Olivier
, David Pastor
, Maria Ledesma-Carbayo
, Delphine Débarre
, Paul Bourgine
, Emmanuel Beaurepaire
, Nadine Peyriéras
, Andres Santos

Universidad Politécnica de Madrid
Biomaterials and Nanomedicine (CIBER-BBN)
CNRS
Institut Polytechnique de Paris

Résultats de recherche: Contribution à un journal › Article › Revue par des pairs

Résumé

Investigating cell dynamics during early zebrafish embryogenesis requires specific image acquisition and analysis strategies. Multiharmonic microscopy, i.e., second- and third-harmonic generations, allows imaging cell divisions and cell membranes in unstained zebrafish embryos from 1- to 1000-cell stage. This paper presents the design and implementation of a dedicated image processing pipeline (tracking and segmentation) for the reconstruction of cell dynamics during these developmental stages. This methodology allows the reconstruction of the cell lineage tree including division timings, spatial coordinates, and cell shape until the 1000-cell stage with minute temporal accuracy and micrometer spatial resolution. Data analysis of the digital embryos provides an extensive quantitative description of early zebrafish embryogenesis.

langue originale	Anglais
Numéro d'article	6093965
Pages (de - à)	2335-2340
Nombre de pages	6
journal	IEEE Transactions on Image Processing
Volume	21
Numéro de publication	4
Les DOIs	https://doi.org/10.1109/TIP.2011.2177911
état	Publié - 1 avr. 2012

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10.1109/TIP.2011.2177911

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Luengo-Oroz, M. A., Rubio-Guivernau, J. L., Faure, E., Savy, T., Duloquin, L., Olivier, N., Pastor, D., Ledesma-Carbayo, M., Débarre, D., Bourgine, P., Beaurepaire, E., Peyriéras, N., & Santos, A. (2012). Methodology for reconstructing early zebrafish development from in vivo multiphoton microscopy. IEEE Transactions on Image Processing, 21(4), 2335-2340. Article 6093965. https://doi.org/10.1109/TIP.2011.2177911

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title = "Methodology for reconstructing early zebrafish development from in vivo multiphoton microscopy",

abstract = "Investigating cell dynamics during early zebrafish embryogenesis requires specific image acquisition and analysis strategies. Multiharmonic microscopy, i.e., second- and third-harmonic generations, allows imaging cell divisions and cell membranes in unstained zebrafish embryos from 1- to 1000-cell stage. This paper presents the design and implementation of a dedicated image processing pipeline (tracking and segmentation) for the reconstruction of cell dynamics during these developmental stages. This methodology allows the reconstruction of the cell lineage tree including division timings, spatial coordinates, and cell shape until the 1000-cell stage with minute temporal accuracy and micrometer spatial resolution. Data analysis of the digital embryos provides an extensive quantitative description of early zebrafish embryogenesis.",

keywords = "Cell lineage tree, in vivo 4-D imaging, multiphoton microscopy, viscous watershed, zebrafish",

author = "Luengo-Oroz, \{Miguel A.\} and Rubio-Guivernau, \{Jose L.\} and Emmanuel Faure and Thierry Savy and Louise Duloquin and Nicolas Olivier and David Pastor and Maria Ledesma-Carbayo and Delphine D{\'e}barre and Paul Bourgine and Emmanuel Beaurepaire and Nadine Peyri{\'e}ras and Andres Santos",

year = "2012",

month = apr,

day = "1",

doi = "10.1109/TIP.2011.2177911",

language = "English",

volume = "21",

pages = "2335--2340",

journal = "IEEE Transactions on Image Processing",

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Luengo-Oroz, MA, Rubio-Guivernau, JL, Faure, E, Savy, T, Duloquin, L, Olivier, N, Pastor, D, Ledesma-Carbayo, M, Débarre, D, Bourgine, P, Beaurepaire, E, Peyriéras, N & Santos, A 2012, 'Methodology for reconstructing early zebrafish development from in vivo multiphoton microscopy', IEEE Transactions on Image Processing, VOL. 21, Numéro 4, 6093965, p. 2335-2340. https://doi.org/10.1109/TIP.2011.2177911

TY - JOUR

T1 - Methodology for reconstructing early zebrafish development from in vivo multiphoton microscopy

AU - Luengo-Oroz, Miguel A.

AU - Rubio-Guivernau, Jose L.

AU - Faure, Emmanuel

AU - Savy, Thierry

AU - Duloquin, Louise

AU - Olivier, Nicolas

AU - Pastor, David

AU - Ledesma-Carbayo, Maria

AU - Débarre, Delphine

AU - Bourgine, Paul

AU - Beaurepaire, Emmanuel

AU - Peyriéras, Nadine

AU - Santos, Andres

PY - 2012/4/1

Y1 - 2012/4/1

N2 - Investigating cell dynamics during early zebrafish embryogenesis requires specific image acquisition and analysis strategies. Multiharmonic microscopy, i.e., second- and third-harmonic generations, allows imaging cell divisions and cell membranes in unstained zebrafish embryos from 1- to 1000-cell stage. This paper presents the design and implementation of a dedicated image processing pipeline (tracking and segmentation) for the reconstruction of cell dynamics during these developmental stages. This methodology allows the reconstruction of the cell lineage tree including division timings, spatial coordinates, and cell shape until the 1000-cell stage with minute temporal accuracy and micrometer spatial resolution. Data analysis of the digital embryos provides an extensive quantitative description of early zebrafish embryogenesis.

AB - Investigating cell dynamics during early zebrafish embryogenesis requires specific image acquisition and analysis strategies. Multiharmonic microscopy, i.e., second- and third-harmonic generations, allows imaging cell divisions and cell membranes in unstained zebrafish embryos from 1- to 1000-cell stage. This paper presents the design and implementation of a dedicated image processing pipeline (tracking and segmentation) for the reconstruction of cell dynamics during these developmental stages. This methodology allows the reconstruction of the cell lineage tree including division timings, spatial coordinates, and cell shape until the 1000-cell stage with minute temporal accuracy and micrometer spatial resolution. Data analysis of the digital embryos provides an extensive quantitative description of early zebrafish embryogenesis.

KW - Cell lineage tree

KW - in vivo 4-D imaging

KW - multiphoton microscopy

KW - viscous watershed

KW - zebrafish

UR - https://www.scopus.com/pages/publications/84859025936

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DO - 10.1109/TIP.2011.2177911

M3 - Article

C2 - 22155959

AN - SCOPUS:84859025936

SN - 1057-7149

VL - 21

SP - 2335

EP - 2340

JO - IEEE Transactions on Image Processing

JF - IEEE Transactions on Image Processing

IS - 4

M1 - 6093965

ER -

Methodology for reconstructing early zebrafish development from in vivo multiphoton microscopy

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