Publications by authors named "Jesselynn LaBelle"
The ability to label proteins by fusion with genetically encoded fluorescent proteins is a powerful tool for understanding dynamic biological processes. However, current approaches for expressing fluorescent protein fusions possess drawbacks, especially at the whole organism level. Expression by transgenesis risks potential overexpression artifacts while fluorescent protein insertion at endogenous loci is technically difficult and, more importantly, does not allow for tissue-specific study of broadly expressed proteins.
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- Researchers are using a split fluorescent protein system, mNeonGreen2 (split-mNG2), to label proteins in zebrafish, addressing limitations in current fluorescent labeling methods, such as overexpression and difficulty in tissue-specific studies.
- This method involves using CRISPR/Cas gene editing to insert mNG2 into specific protein-coding genes while expressing it under tissue-specific promoters, allowing for natural expression levels of proteins.
- The study shows that split-mNG2 effectively labels cytoskeleton genes across different tissues and can manipulate protein function by anchoring mNG2 to specific cellular compartments, suggesting this approach has broad research applications.
The endoderm is one of the three primary germ layers that ultimately gives rise to the gastrointestinal and respiratory epithelia and other tissues. In zebrafish and other vertebrates, endodermal cells are initially highly migratory with only transient interactions among one other, but later converge together to form an epithelial sheet. Here, we show that during their early, migratory phase, endodermal cells actively avoid each other through contact inhibition of locomotion (CIL), a characteristic response consisting of 1) actin depolymerization and membrane retraction at the site of contact, 2) preferential actin polymerization along a cell-free edge, and 3) reorientation of migration away from the other cell.
View Article and Find Full Text PDFInducible gene expression systems are an invaluable tool for studying biological processes. Optogenetic expression systems can provide precise control over gene expression timing, location, and amplitude using light as the inducing agent. In this protocol, an optogenetic expression system is used to achieve light-inducible gene expression in zebrafish embryos.
View Article and Find Full Text PDFInducible gene expression systems are valuable tools for studying biological processes. We previously developed an optogenetic gene expression system called TAEL that is optimized for use in zebrafish. When illuminated with blue light, TAEL transcription factors dimerize and activate gene expression downstream of the TAEL-responsive C120 promoter.
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