Live Fluorescence Imaging of F-Actin Organization in Chick Whole Embryo Cultures Using SiR-Actin

Manuel Schmitz-Elbers; Gražvydas Lukinavičius; Theodoor H. Smit

doi:10.3390/cells10071578

Live Fluorescence Imaging of F-Actin Organization in Chick Whole Embryo Cultures Using SiR-Actin

Manuel Schmitz-Elbers
, Gražvydas Lukinavičius
, Theodoor H. Smit

University of Amsterdam
Max Planck Institute for Biophysical Chemistry (Karl Friedrich Bonhoeffer Institute)

Research output: Contribution to journal › Article › Academic › peer-review

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Abstract

Morphogenesis is a continuous process of pattern formation so complex that it requires in vivo monitoring for better understanding. Changes in tissue shape are initiated at the cellular level, where dynamic intracellular F-actin networks determine the shape and motility of cells, influence differentiation and cytokinesis and mediate mechanical signaling. Here, we stain F-actin with the fluorogenic probe SiR-actin for live fluorescence imaging of whole chick embryos. We found that 50 nM SiR-actin in the culture medium is a safe and effective concentration for this purpose, as it provides high labeling density without inducing morphological malformations.

Original language	English
Article number	1578
Journal	Cells
Volume	10
Issue number	7
DOIs	https://doi.org/10.3390/cells10071578
Publication status	Published - Jul 2021

Keywords

F-actin
Live fluorescence imaging
SiR-actin
Whole embryo culture

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title = "Live Fluorescence Imaging of F-Actin Organization in Chick Whole Embryo Cultures Using SiR-Actin",

abstract = "Morphogenesis is a continuous process of pattern formation so complex that it requires in vivo monitoring for better understanding. Changes in tissue shape are initiated at the cellular level, where dynamic intracellular F-actin networks determine the shape and motility of cells, influence differentiation and cytokinesis and mediate mechanical signaling. Here, we stain F-actin with the fluorogenic probe SiR-actin for live fluorescence imaging of whole chick embryos. We found that 50 nM SiR-actin in the culture medium is a safe and effective concentration for this purpose, as it provides high labeling density without inducing morphological malformations.",

keywords = "F-actin, Live fluorescence imaging, SiR-actin, Whole embryo culture",

author = "Manuel Schmitz-Elbers and Gra{\v z}vydas Lukinavi{\v c}ius and Smit, \{Theodoor H.\}",

year = "2021",

month = jul,

doi = "10.3390/cells10071578",

language = "English",

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journal = "Cells",

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T1 - Live Fluorescence Imaging of F-Actin Organization in Chick Whole Embryo Cultures Using SiR-Actin

AU - Schmitz-Elbers, Manuel

AU - Lukinavičius, Gražvydas

AU - Smit, Theodoor H.

PY - 2021/7

Y1 - 2021/7

N2 - Morphogenesis is a continuous process of pattern formation so complex that it requires in vivo monitoring for better understanding. Changes in tissue shape are initiated at the cellular level, where dynamic intracellular F-actin networks determine the shape and motility of cells, influence differentiation and cytokinesis and mediate mechanical signaling. Here, we stain F-actin with the fluorogenic probe SiR-actin for live fluorescence imaging of whole chick embryos. We found that 50 nM SiR-actin in the culture medium is a safe and effective concentration for this purpose, as it provides high labeling density without inducing morphological malformations.

AB - Morphogenesis is a continuous process of pattern formation so complex that it requires in vivo monitoring for better understanding. Changes in tissue shape are initiated at the cellular level, where dynamic intracellular F-actin networks determine the shape and motility of cells, influence differentiation and cytokinesis and mediate mechanical signaling. Here, we stain F-actin with the fluorogenic probe SiR-actin for live fluorescence imaging of whole chick embryos. We found that 50 nM SiR-actin in the culture medium is a safe and effective concentration for this purpose, as it provides high labeling density without inducing morphological malformations.

KW - F-actin

KW - Live fluorescence imaging

KW - SiR-actin

KW - Whole embryo culture

UR - https://www.scopus.com/pages/publications/85110371014

U2 - 10.3390/cells10071578

DO - 10.3390/cells10071578

M3 - Article

C2 - 34206626

SN - 2073-4409

VL - 10

JO - Cells

JF - Cells

IS - 7

M1 - 1578

ER -

Live Fluorescence Imaging of F-Actin Organization in Chick Whole Embryo Cultures Using SiR-Actin

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