Resolving in vivo gene expression during collective cell migration using an integrated RNAscope, immunohistochemistry and tissue clearing method

Wolfe

et al. 2017

eLife

Neural crest cells migrate throughout the embryo, but how cells move in a directed and collective manner has remained unclear. Here, we perform the first single-cell transcriptome analysis of cranial neural crest cell migration at three progressive stages in chick and identify and establish hierarchical relationships between cell position and time-specific transcriptional signatures. We determine a novel transcriptional signature of the most invasive neural crest Trailblazer cells that is consistent during migration and enriched for approximately 900 genes. Knockdown of several Trailblazer genes shows significant but modest changes to total distance migrated. However, in vivo expression analysis by RNAscope and immunohistochemistry reveals some salt and pepper patterns that include strong individual Trailblazer gene expression in cells within other subregions of the migratory stream. These data provide new insights into the molecular diversity and dynamics within a neural crest cell migratory stream that underlie complex directed and collective cell behaviors.

Section: Resultsmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

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Single-cell transcriptome analysis of avian neural crest migration reveals signatures of invasion and molecular transitions

Morrison

Wolfe

et al. 2017

eLife

“…To detect the expression of AQP-1 mRNA in vivo specifically within migrating cranial neural crest cells, we took advantage of our recently optimized integrated protocol combining RNAscope multiplexed fluorescence in situ hybridization, immunohistochemistry (IHC), and tissue clearing with FRUIT (Morrison et al, 2017b). This enabled the detection of AQP-1 mRNA expression in migrating HNK-1 labeled neural crest cells (Fig.…”

Section: Resultsmentioning

confidence: 99%

“…RNAscope on whole chick heads was performed as previously described (Morrison et al, 2017b). Briefly, HH13 chick embryos were harvested and fixed in 4% paraformaldehyde for 2 hours.…”

Section: Methodsmentioning

confidence: 99%

Neural crest cells bulldoze through the microenvironment using Aquaporin-1 to stabilize filopodia

McKinney

Teddy

et al. 2019

Preprint

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2Neural crest migration requires cells to move through an environment filled with dense 3 extracellular matrix and mesoderm to reach targets throughout the vertebrate embryo. 4 Here, we use high-resolution microscopy, computational modeling, and in vitro and in 5 vivo cell invasion assays to investigate the function of Aquaporin-1 (AQP-1) signaling. 6 We find that migrating lead cranial neural crest cells express AQP-1 mRNA and protein, 7 implicating a biological role for water channel protein function during invasion. 8 Differential AQP-1 levels affect neural crest cell speed, direction, and the length and 9 stability of cell filopodia. Further, AQP-1 enhances matrix metalloprotease (MMP) 10 activity and colocalizes with phosphorylated focal adhesion kinases (pFAK). Co-11 localization of AQP-1 expression with EphB guidance receptors in the same migrating 12 neural crest cells raises novel implications for the concept of guided bulldozing by lead 13 cells during migration. 14 15 3 1 INTRODUCTION 2 Cell migration is essential during embryogenesis to gastrulate, elongate the vertebrate 3 axis, and distribute cells into the periphery to contribute to organ development. Despite 4 the importance of cell migration to human development and disease, it is still unclear 5 what mechanisms enable cells to invade the dense ECM, mesoderm and other cell 6 types characteristic of the embryonic microenvironment. The complexity of the 7 embryonic microenvironment means that invading cells must rapidly change cell shape 8 and volume, form and sustain protrusions that penetrate different sized gaps, and attach 9 to and remodel the ECM. Thus, there is a tremendous need to identify and test the 10 function of molecules critical to embryonic cell migration and better understand their 11 mechanistic basis.12 13 Neural crest cell migration is one of the most prevalent examples of how cells efficiently 14 distribute throughout the growing vertebrate embryo to precise targets. In the head, 15 cranial neural crest cells must invade through dense ECM, loosely connected 16 mesoderm, and migrating endothelial cells. Yet, it has remained unclear how the 17 migrating neural crest cells that first encounter the embryonic microenvironment 18 penetrate small gaps between mesodermal cells and degrade the ECM to move in a 19 directed manner to peripheral targets. By combining dynamic in vivo imaging and super 20 resolution microscopy with gain-and loss-of-function experiments, we are poised to 21 examine the function of genes presumed critical to neural crest cell migration. Thus, the 22 embryonic neural crest is an attractive in vivo model to study the function of cell 23 invasion genes in mechanistic detail. 4 1 Using single cell RT-qPCR and transcriptome profiling, we discovered the enhanced 2 expression of several genes in the most invasive chick cranial neural crest cells, 3 including AQP-1 (McLennan et al., 2015a; Morrison et al., 2017a). AQP-1 is a 4 transmembrane channel protein that facilitates the flux of water across the plasma 5 5 ...

Colec12 and Trail signaling confine cranial neural crest cell trajectories and promote collective cell migration

Giniūnaitė

Hildebrand

et al. 2023

Developmental Dynamics

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Background Collective and discrete neural crest cell (NCC) migratory streams are crucial to vertebrate head patterning. However, the factors that confine NCC trajectories and promote collective cell migration remain unclear. Results Computational simulations predicted that confinement is required only along the initial one‐third of the cranial NCC migratory pathway. This guided our study of Colec12 (Collectin‐12, a transmembrane scavenger receptor C‐type lectin) and Trail (tumor necrosis factor‐related apoptosis‐inducing ligand, CD253) which we show expressed in chick cranial NCC‐free zones. NCC trajectories are confined by Colec12 or Trail protein stripes in vitro and show significant and distinct changes in cell morphology and dynamic migratory characteristics when cocultured with either protein. Gain‐ or loss‐of‐function of either factor or in combination enhanced NCC confinement or diverted cell trajectories as observed in vivo with three‐dimensional confocal microscopy, respectively, resulting in disrupted collective migration. Conclusions These data provide evidence for Colec12 and Trail as novel NCC microenvironmental factors playing a role to confine cranial NCC trajectories and promote collective cell migration.