INVESTIGATIONS ON EPITHELIAL BIOLOGY USING ORGANOID DIFFERENTIATION AND CO-CULTURES

10.33540/182 ◽  
2021 ◽  
Author(s):  
◽  
Jens Puschhof
Keyword(s):  
Epithelial Biology

scholarly journals Functional Genomic Annotation of Genetic Risk Loci Highlights Inflammation and Epithelial Biology Networks in CKD

2014 ◽  
Vol 26 (3) ◽  
pp. 692-714 ◽  
Author(s):  
Nora Ledo ◽  
Yi-An Ko ◽  
Ae-Seo Deok Park ◽  
Hyun-Mi Kang ◽  
Sang-Youb Han ◽  
...  
Keyword(s):  
Genetic Risk ◽  
Functional Genomic ◽  
Genomic Annotation ◽  
Epithelial Biology

scholarly journals Knock-in tagging in zebrafish facilitated by insertion into non-coding regions

2021 ◽  
Author(s):  
Daniel S Levic ◽  
Naoya Yamaguchi ◽  
Siyao Wang ◽  
Holger Knaut ◽  
Michel Bagnat
Keyword(s):  
Protein Function ◽  
Cell Biology ◽  
Quantitative Imaging ◽  
Expression Patterns ◽  
Imaging Studies ◽  
Coding Regions ◽  
Fluorescent Markers ◽  
Endogenous Expression ◽  
Epithelial Biology

Zebrafish provide an excellent model for in vivo cell biology studies due to their amenability to live imaging. Protein visualization in zebrafish has traditionally relied on overexpression of fluorescently tagged proteins from heterologous promoters, making it difficult to recapitulate endogenous expression patterns and protein function. One way to circumvent this problem is to tag the proteins by modifying their endogenous genomic loci. Such an approach is not widely available to zebrafish researchers due to inefficient homologous recombination and the error-prone nature of targeted integration in zebrafish. Here, we report a simple approach for tagging proteins in zebrafish on their N- or C termini with fluorescent markers by inserting PCR-generated donor amplicons into non-coding regions of the corresponding genes. Using this approach, we generated endogenously tagged alleles for several genes critical for epithelial biology and organ development including the tight junction components ZO-1 and Cldn15la, the trafficking effector Rab11a, and the ECM receptor β1 integrin. Our approach facilitates the generation of knock-in lines in zebrafish, opening the way for accurate quantitative imaging studies.

scholarly journals Corneal epithelial biology: Lessons stemming from old to new

2020 ◽  
Vol 198 ◽  
pp. 108094 ◽  
Author(s):  
Robert M. Lavker ◽  
Nihal Kaplan ◽  
Junyi Wang ◽  
Han Peng
Keyword(s):  
Corneal Epithelial ◽  
Epithelial Biology

scholarly journals A192 DEPLETING ASCL2 IN ESOPHAGEAL ORGANOIDS TO INVESTIGATE ITS ROLE IN STEM CELLS MAINTENANCE

2020 ◽  
Vol 3 (Supplement_1) ◽  
pp. 63-64
Author(s):  
M Hamilton ◽  
D Jean ◽  
V Giroux
Keyword(s):  
Stem Cells ◽  
Cell Line ◽  
Cell Lines ◽  
Gene Target ◽  
Funding Agencies ◽  
Primary Mouse ◽  
Lentiviral Infection ◽  
Infected Cells ◽  
Epithelial Biology

Abstract Background Recently, the first population of stem cells in the esophageal epithelium was identified with the help of the Keratin 15(Krt15) marker. However, little is known about the mechanisms underlying the expansion and the function of stem cells in the esophagus. It was shown that ASCL2, a transcription factor, is upregulated in Krt15+cells compared with Krt15- cells. ASCL2 is a gene target of the Wnt/β-catenin pathway, which act as a regulator of proliferation and maintenance of the stemness state. The ultimate goal of my research project is to determine the role of ASCL2 in the maintenance of esophageal stem cells and to identify his binding partners. Aims To investigate the role of ASCL2 in esophageal epithelial biology, we aim at establishingAscl2knockout esophageal organoid lines. Methods Lentiviral infection and CRISPR/Cas9 knockout approach were optimized in mouse esophageal organoids. ASCL2was invalidated with CRISPR/Cas9 and/or inducible specific shRNAs in primary mouse esophageal cell line and organoids. Antibodies directed against ASCL2 were also tested to validate cell lines. Results First, to optimize lentiviral infection in mouse esophageal organoids, we produced GFP-expressing lentiviruses. Viruses were then concentrated and incubated with a single cell suspension of mouse organoid cells under gentle activation. Infected cells were embedded in Matrigel and grown in organoids. GFP+ cells were then selected using an antibiotic resistance strategy. Second, we used our optimized lentiviral infection protocol to express specific gRNAs in mouse esophageal organoids, which were previously screened in a primary mouse esophageal cell line. Knockout were validated using Western Blot. Invalidation of ASCL2 was performed using CRISPR/Cas9 and inducible shRNAs. We also validated three commercially available ASCL2 antibodies in WB and IF. Conclusions ASCL2 is expressed in the mouse esophagus tissue and organoids, and it can be invalidated in cell lines and organoids. Funding Agencies NSERC, CRC Tier2

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