PUBLICATION

Mesoderm is required for coordinated cell movements within zebrafish neural plate in vivo

Authors

Araya, C., Tawk, M., Girdler, G.C., Costa, M., Carmona-Fontaine, C., and Clarke, J.D.

ID

ZDB-PUB-140428-1

Date

2014

Source

Neural Development 9(1): 9 (Journal)

Registered Authors

Araya Garcia, Claudio, Clarke, Jon, Tawk, Marcel

Keywords

none

MeSH Terms

Neural Plate/embryology*
Nodal Signaling Ligands/metabolism
Zebrafish/embryology*
Body Patterning
Neural Tube/embryology*
Animals
Mesoderm/embryology*
Cell Movement*

(all 8)

PubMed

24755297 Full text @ Neural Dev.

Abstract

Background

Morphogenesis of the zebrafish neural tube requires the coordinated movement of many cells in both time and space. A good example of this is the movement of the cells in the zebrafish neural plate as they converge towards the dorsal midline before internalizing to form a neural keel. How these cells are regulated to ensure that they move together as a coherent tissue is unknown. Previous work in other systems has suggested that the underlying mesoderm may play a role in this process but this has not been shown directly in vivo.

Results

Here we analyze the roles of subjacent mesoderm in the coordination of neural cell movements during convergence of the zebrafish neural plate and neural keel formation. Live imaging demonstrates that the normal highly coordinated movements of neural plate cells are lost in the absence of underlying mesoderm and the movements of internalization and neural tube formation are severely disrupted. Despite this, neuroepithelial polarity develops in the abnormal neural primordium but the resulting tissue architecture is very disorganized.

Conclusions

We show that the movements of cells in the zebrafish neural plate are highly coordinated during the convergence and internalization movements of neurulation. Our results demonstrate that the underlying mesoderm is required for these coordinated cell movements in the zebrafish neural plate in vivo.

Genes / Markers

Marker	Marker Type	Name
egr2b	GENE	early growth response 2b
foxc1a	GENE	forkhead box C1a
lft1	GENE	lefty1
ndr2	GENE	nodal-related 2
pitx2	GENE	paired-like homeodomain 2
sox32	GENE	SRY-box transcription factor 32
tbx16	GENE	T-box transcription factor 16
tbxta	GENE	T-box transcription factor Ta
tdgf1	GENE	teratocarcinoma-derived growth factor 1

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Figures

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Expression

Gene	Fish	Conditions	Stage	Qualifier	Anatomy	Assay	Figure
EGFP	knu3Tg	standard conditions	Prim-5		neuron	IHC	Fig. 1
EGFP	knu3Tg	chemical treatment: pharmaceutical	Prim-5		neuron	IHC	Fig. 1
EGFP	tdgf1^tz257/tz257; knu3Tg	chemical treatment: pharmaceutical	Prim-5		neural tube	IHC	Fig. 2
GFP	kca66Tg; kca6Tg	standard conditions	20-25 somites		whole organism nucleus	IFL	Fig. 6
GFP	kca66Tg; kca6Tg	standard conditions	1-4 somites		whole organism nucleus	IFL	Fig. 6
GFP	kca66Tg; kca6Tg	standard conditions	5-9 somites		whole organism nucleus	IFL	Fig. 6
GFP	kca66Tg; kca6Tg	standard conditions	10-13 somites		whole organism nucleus	IFL	Fig. 6
lft1	WT	standard conditions	20-25 somites		zebrafish anatomical entity	ISH	Fig. 4
lft1	WT	chemical treatment: pharmaceutical	20-25 somites	Not Detected	zebrafish anatomical entity	ISH	Fig. 4
pitx2	WT	chemical treatment: pharmaceutical	26+ somites	Not Detected	zebrafish anatomical entity	ISH	Fig. 4

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Phenotype

Fish	Conditions	Stage	Phenotype	Figure
WT	chemical treatment: pharmaceutical	20-25 somites	nodal signaling pathway decreased process quality, abnormal	Fig. 4
WT	chemical treatment: pharmaceutical	26+ somites	nodal signaling pathway decreased process quality, abnormal	Fig. 4
WT	chemical treatment: pharmaceutical	Prim-5	neural tube morphology, abnormal	Fig. 4
WT	chemical treatment: pharmaceutical	Prim-5	neural tube morphology, abnormal	Fig. 1
WT + MO1-tbx16 + MO2-tbx16	standard conditions	Prim-5	mesoderm decreased amount, abnormal	Fig. 3
knu3Tg	chemical treatment: pharmaceutical	Prim-5	neural tube morphology, abnormal	Fig. 1
tdgf1^tz257/tz257	control	Bud to 20-25 somites	neural plate cell migration process quality, abnormal	Fig. 7
tdgf1^tz257/tz257	control	Bud to 20-25 somites	neural plate morphogenesis process quality, abnormal	Fig. 7
tdgf1^tz257/tz257	standard conditions	Bud to 20-25 somites	neural keel malformed, abnormal	Fig. 8
tdgf1^tz257/tz257	standard conditions	Bud to 20-25 somites	neural plate cell motility process quality, abnormal	Fig. 8

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Mutations / Transgenics

Allele	Construct	Type	Affected Genomic Region
b160		Indel	tbxta
kca6Tg	Tg(h2az2a:h2az2a-GFP)	Transgenic Insertion
kca66Tg	Tg(h2az2a:h2az2a-GFP)	Transgenic Insertion
knu3Tg	Tg(elavl3:EGFP)	Transgenic Insertion
m294		Point Mutation	ndr2
sox32_unspecified		Unspecified	sox32
t4		Deficiency	shha
tz257		Point Mutation	tdgf1

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Human Disease / Model

Sequence Targeting Reagents

Target	Reagent	Reagent Type
tbx16	MO1-tbx16	MRPHLNO
tbx16	MO2-tbx16	MRPHLNO

Fish

Fish
Df(Chr07)t4
kca66Tg; kca6Tg
knu3Tg
ndr2^m294/m294
sox32^{unspecified/unspecified}
tbxta^b160/b160
tdgf1^tz257/tz257
tdgf1^tz257/tz257
tdgf1^tz257/tz257; knu3Tg
tdgf1^tz257/tz257 + MO1-tbx16 + MO2-tbx16

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Antibodies

Name	Type	Antigen Genes	Isotypes	Host Organism
Ab1-prkca	polyclonal	prkcaa	IgG	Rabbit
Ab1-tjp1	monoclonal	tjp1a tjp1b	IgG1	Mouse
Ab1-tuba	monoclonal		IgG2b	Mouse
Ab2-gfap	polyclonal	gfap		Rabbit
Ab-MF20	monoclonal		IgG2b	Mouse

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Orthology

Engineered Foreign Genes

Marker	Marker Type	Name
EGFP	EFG	EGFP
GFP	EFG	GFP

Mapping

Araya et al., 2014 ZDB-PUB-140428-1 PMID:24755297

Mesoderm is required for coordinated cell movements within zebrafish neural plate in vivo

Background

Results

Conclusions

Araya et al., 2014

ZDB-PUB-140428-1
PMID:24755297