Your search keyword '"Kim B. Jensen"' showing total 122 results

1. Detecting host responses to microbial stimulation using primary epithelial organoids

Author

Jette Bornholdt, Christina V. Müller, Maria Juul Nielsen, Jesper Strickertsson, Daria Rago, Yun Chen, Grzegorz Maciag, Jonathan Skov, Anja Wellejus, Pawel J. Schweiger, Stine L. Hansen, Christa Broholm, Ismail Gögenur, Martti Maimets, Stine Sloth, Jakob Hendel, Adam Baker, Albin Sandelin, and Kim B. Jensen

Subjects

Intestinal organoids, probiotics, microbiome, intestinal epithelium, bacterial–epithelial interactions, Diseases of the digestive system. Gastroenterology, RC799-869

Abstract

ABSTRACTThe intestinal epithelium is constantly exposed to microbes residing in the lumen. Traditionally, the response to microbial interactions has been studied in cell lines derived from cancerous tissues, e.g. Caco-2. It is, however, unclear how the responses in these cancer cell lines reflect the responses of a normal epithelium and whether there might be microbial strain-specific effects. To address these questions, we derived organoids from the small intestine from a cohort of healthy individuals. Culturing intestinal epithelium on a flat laminin matrix induced their differentiation, facilitating analysis of microbial responses via the apical membrane normally exposed to the luminal content. Here, it was evident that the healthy epithelium across multiple individuals (n = 9) demonstrates robust acute both common and strain-specific responses to a range of probiotic bacterial strains (BB-12Ⓡ, LGGⓇ, DSM33361, and Bif195). Importantly, parallel experiments using the Caco-2 cell line provide no acute response. Collectively, we demonstrate that primary epithelial cells maintained as organoids represent a valuable resource for assessing interactions between the epithelium and luminal microbes across individuals, and that these models are likely to contribute to a better understanding of host microbe interactions.

Published

2023

2. Mesenchymal-epithelial crosstalk shapes intestinal regionalisation via Wnt and Shh signalling

Author

Martti Maimets, Marianne Terndrup Pedersen, Jordi Guiu, Jes Dreier, Malte Thodberg, Yasuko Antoku, Pawel J. Schweiger, Leonor Rib, Raul Bardini Bressan, Yi Miao, K. Christopher Garcia, Albin Sandelin, Palle Serup, and Kim B. Jensen

Subjects

Science

Abstract

The small intestine forms via crosstalk between epithelial and mesenchymal cell compartments. Here, the authors show that a gradient of Wnt signalling along the anterior-posterior axis regulates Sonic Hedgehog which is required for correct formation and regionalization of the small intestine.

Published

2022

3. In Vivo Studies Should Take Priority When Defining Mechanisms of Intestinal Crypt Morphogenesis

Author

Jordi Guiu, PhD and Kim B. Jensen, PhD

Subjects

Diseases of the digestive system. Gastroenterology, RC799-869

Published

2022

4. A bioengineering perspective on modelling the intestinal epithelial physiology in vitro

Author

Maria Antfolk and Kim B. Jensen

Subjects

Science

Abstract

Maria Antfolk and Kim Jensen discuss how to model intestinal epithelial cell function in the dish and how various physiologically important environmental conditions, for example, extracellular matrix, pressure and flow, can be modelled and how this is applicable to clinical work.

Published

2020

5. Rebuttal to: Organoid vs Mouse Model: Which is a Better Research Tool to Understand the Biologic Mechanisms of Intestinal Epithelium?

Author

Jordi Guiu, PhD and Kim B. Jensen, PhD

Subjects

Diseases of the digestive system. Gastroenterology, RC799-869

Published

2022

6. Fluorescence-based tracing of transplanted intestinal epithelial cells using confocal laser endomicroscopy

Author

Fredrik Bergenheim, Jakob B. Seidelin, Marianne Terndrup Pedersen, Benjamin E. Mead, Kim B. Jensen, Jeffrey M. Karp, and Ole Haagen Nielsen

Subjects

Cell labeling, Confocal laser endomicroscopy, Colitis, Fluorescent dyes, Intestinal organoids, Intestinal stem cells, Medicine (General), R5-920, Biochemistry, QD415-436

Abstract

Abstract Background Intestinal stem cell transplantation has been shown to promote mucosal healing and to engender fully functional epithelium in experimental colitis. Hence, stem cell therapies may provide an innovative approach to accomplish mucosal healing in patients with debilitating conditions such as inflammatory bowel disease. However, an approach to label and trace transplanted cells, in order to assess engraftment efficiency and to monitor wound healing, is a key hurdle to overcome prior to initiating human studies. Genetic engineering is commonly employed in animal studies, but may be problematic in humans due to potential off-target and long-term adverse effects. Methods We investigated the applicability of a panel of fluorescent dyes and nanoparticles to label intestinal organoids for visualization using the clinically approved imaging modality, confocal laser endomicroscopy (CLE). Staining homogeneity, durability, cell viability, differentiation capacity, and organoid forming efficiency were evaluated, together with visualization of labeled organoids in vitro and ex vivo using CLE. Results 5-Chloromethylfluorescein diacetate (CMFDA) proved to be suitable as it efficiently stained all organoids without transfer to unstained organoids in co-cultures. No noticeable adverse effects on viability, organoid growth, or stem cell differentiation capacity were observed, although single-cell reseeding revealed a dose-dependent reduction in organoid forming efficiency. Labeled organoids were easily identified in vitro using CLE for a duration of at least 3 days and could additionally be detected ex vivo following transplantation into murine experimental colitis. Conclusions It is highly feasible to use fluorescent dye-based labeling in combination with CLE to trace intestinal organoids following transplantation to confirm implantation at the intestinal target site.

Published

2019

7. A Semi-automated Organoid Screening Method Demonstrates Epigenetic Control of Intestinal Epithelial Differentiation

Author

Jenny Ostrop, Rosalie T. Zwiggelaar, Marianne Terndrup Pedersen, François Gerbe, Korbinian Bösl, Håvard T. Lindholm, Alberto Díez-Sánchez, Naveen Parmar, Silke Radetzki, Jens Peter von Kries, Philippe Jay, Kim B. Jensen, Cheryl Arrowsmith, and Menno J. Oudhoff

Subjects

organoids, epigenetic modifiers, intestinal stem cell biology, bioimage analysis, PRMT1, EP300, Biology (General), QH301-705.5

Abstract

Intestinal organoids are an excellent model to study epithelial biology. Yet, the selection of analytical tools to accurately quantify heterogeneous organoid cultures remains limited. Here, we developed a semi-automated organoid screening method, which we applied to a library of highly specific chemical probes to identify epigenetic regulators of intestinal epithelial biology. The role of epigenetic modifiers in adult stem cell systems, such as the intestinal epithelium, is still undefined. Based on this resource dataset, we identified several targets that affected epithelial cell differentiation, including HDACs, EP300/CREBBP, LSD1, and type I PRMTs, which were verified by complementary methods. For example, we show that inhibiting type I PRMTs, which leads enhanced epithelial differentiation, blocks the growth of adenoma but not normal organoid cultures. Thus, epigenetic probes are powerful tools to study intestinal epithelial biology and may have therapeutic potential.

Published

2021

8. Personalized B cell response to the Lactobacillus rhamnosus GG probiotic in healthy human subjects: a randomized trial

Author

Jette Bornholdt, Christa Broholm, Yun Chen, Alfredo Rago, Stine Sloth, Jakob Hendel, Cathrine Melsæther, Christina V. Müller, Maria Juul Nielsen, Jesper Strickertsson, Lars Engelholm, Kristoffer Vitting-Seerup, Kim B. Jensen, Adam Baker, and Albin Sandelin

Subjects

lactobacillus rhamnosus gg, immediate in vivo effect, probiotics, human transcriptomics, b cell activation, Diseases of the digestive system. Gastroenterology, RC799-869

Abstract

The specific effects of administering live probiotics in the human gut are not well characterized. To this end, we investigated the immediate effect of Lactobacillus rhamnosus GG (LGG) in the jejunum of 27 healthy volunteers 2 h after ingestion using a combination of global RNA sequencing of human biopsies and bacterial DNA sequencing in a multi-visit, randomized, cross-over design (ClinicalTrials.gov number NCT03140878). While LGG was detectable in jejunum after 2 h in treated subjects, the gene expression response vs. placebo was subtle if assessed across all subjects. However, clustering analysis revealed that one-third of subjects exhibited a strong and consistent LGG response involving hundreds of genes, where genes related to B cell activation were upregulated, consistent with prior results in mice. Immunohistochemistry and single cell-based deconvolution analyses showed that this B cell signature likely is due to activation and proliferation of existing B cells rather than B cell immigration to the tissue. Our results indicate that the LGG strain has an immediate effect in the human gut in a subpopulation of individuals. In extension, our data strongly suggest that studies on in vivo probiotic effects in humans require large cohorts and must take individual variation into account.

Published

2020

9. COX-2–PGE2 Signaling Impairs Intestinal Epithelial Regeneration and Associates with TNF Inhibitor Responsiveness in Ulcerative ColitisResearch in Context

Author

Yuan Li, Christoffer Soendergaard, Fredrik Holmberg Bergenheim, David M. Aronoff, Ginger Milne, Lene Buhl Riis, Jakob Benedict Seidelin, Kim B. Jensen, and Ole Haagen Nielsen

Subjects

Medicine, Medicine (General), R5-920

Abstract

Background: Inhibition of tumor necrosis factor-α (TNF) signaling is beneficial in the management of ulcerative colitis (UC), but up to one-third of patients do not have a clinical response of relevance to TNF inhibitors during induction therapy (i.e. primary non-responders [PNRs]). Through production of prostaglandins (PGs) and thromboxanes, cyclooxygenase-2 (COX-2) affects inflammation and epithelial regeneration and may in this way be implicated in treatment resistance to TNF inhibitors. Methods: In this study, COX-2 expression was analyzed in human intestinal biopsies and patient-derived monocytes, and the downstream consequences of COX-2 activity was evaluated by assessing the influence of the down-stream effector, PGE2, on intestinal epithelial stem cell self-renewal and differentiation using primary human intestinal organoids (“mini-guts”). Findings: We found that TNF stimulation induced COX-2 expression in monocytes isolated from responders (Rs), whereas COX-2 expression was constitutively high and non-inducible in monocytes from PNRs. Additionally, PGE2 in combination with proliferative signals transformed human intestinal epithelial cells to a proinflammatory state akin to flaring UC, whereas PGE2 in combination with differentiation signals supported robust mucin induction. Interpretation: Our work indicates that COX-2-PGE2 signaling could be a novel target for the management of PNRs to TNF inhibitors. We additionally demonstrate that COX-2–PGE2 signaling has dual functions during tissue repair and normal lineage differentiation, explaining in part the lack of response to TNF inhibitors among PNRs. Fund: This work was funded by grants from the Novo Nordisk Foundation, the Lundbeck Foundation, the Vanderbilt Digestive Disease Research Center, NIH Grants, Aase and Ejnar Danielsen's Foundation and the A.P. Møller Foundation. Keywords: COX-2, Intestinal epithelial cells, Monocytes, Prostaglandin E2, Ulcerative colitis

Published

2018

10. Maintenance of high-turnover tissues during and beyond homeostasis

Author

Isidora Banjac, Martti Maimets, and Kim B. Jensen

Subjects

Genetics, Molecular Medicine, Cell Biology

Published

2023

11. Transcriptional and epigenomic profiling identifies YAP signaling as a key regulator of intestinal epithelium maturation

Author

Laura M. Pikkupeura, Raul B. Bressan, Jordi Guiu, Yun Chen, Martti Maimets, Daniela Mayer, Pawel J. Schweiger, Stine L. Hansen, Grzegorz J. Maciag, Hjalte L. Larsen, Kadi Lõhmussaar, Marianne Terndrup Pedersen, Joji M. Yap Teves, Jette Bornholdt, Vladimir Benes, Albin Sandelin, and Kim B. Jensen

Abstract

During intestinal organogenesis, equipotent epithelial progenitors mature into phenotypically distinct stem cells that are responsible for life-long maintenance of the tissue. While the morphological changes associated with the transition are well-characterized, the molecular mechanisms underpinning the maturation process are not fully understood. Here, we leverage intestinal organoid cultures to profile transcriptional, chromatin accessibility, DNA methylation and 3D chromatin conformation landscapes defining fetal and adult epithelial cells. We observed prominent differences in gene expression and enhancer activity, accompanied by changes in 3D organization and local changes in DNA accessibility and methylation, between the two cellular states. Using integrative analyses, we identified sustained YAP transcriptional activity as a major gatekeeper of the immature fetal state. We found the YAP-associated transcriptional network to be regulated at various levels of chromatin organization, and likely to be coordinated by changes in extracellular matrix composition. Altogether, our work highlights the value of unbiased profiling of regulatory landscapes for the identification of key mechanisms underlying tissue maturation.

Published

2023

12. Reprogramming cellular identity during intestinal regeneration

Author

Hjalte List Larsen and Kim B. Jensen

Subjects

0303 health sciences, Regeneration (biology), Identity (social science), Epithelial Cells, Biology, Cellular Reprogramming, Intestinal epithelium, Cell biology, Intestines, Organoids, 03 medical and health sciences, Crosstalk (biology), 0302 clinical medicine, Genetics, Organoid, Animals, Humans, Regeneration, Intestinal Mucosa, Reprogramming, 030217 neurology & neurosurgery, Vital organ, Homeostasis, 030304 developmental biology, Developmental Biology

Abstract

The intestine is a vital organ mediating absorption of nutrients and water. Following tissue damage, the intestine mounts a remarkable regenerative response by reprogramming cellular identity to facilitate reinstatement of homeostasis. Here we review recent advances within intestinal regenerative biology and the emerging concept of fetal-like reprogramming, in which the adult intestinal epithelium transiently enters a repair-associated state reminiscent of ontologically pre-existing stages. We focus on molecular mechanisms governing reprogramming of cellular identity via epithelial-mesenchymal crosstalk, and how novel approaches in organoid technologies enable identification and characterisation of cell-autonomous repair responses within epithelial cells. Transitioning from the single-cell level to tissue scale, we discuss clonal selection following regeneration and associated pathological repurcussions such as cancer and chronic inflammatory diseases.

Published

2021

13. A biomechanical switch regulates the transition towards homeostasis in oesophageal epithelium

Author

Kata Krizic, Kim B. Jensen, Maria P. Alcolea, Kevin J. Chalut, Seungmin Han, Svetlana Ulyanchenko, Christophe M. Verstreken, Ramiro Iglesias-Bartolome, Jamie McGinn, Adrien Hallou, Benjamin D. Simons, and Frances J. England

Subjects

Esophageal Mucosa, Period (gene), Population, Cell, Biology, Article, Epithelium, Kruppel-Like Factor 4, Mice, 03 medical and health sciences, 0302 clinical medicine, medicine, Animals, Homeostasis, Humans, education, Cell Proliferation, 030304 developmental biology, 0303 health sciences, education.field_of_study, Cell growth, Mechanism (biology), Stem Cells, Cell Differentiation, Epithelial Cells, Cell Biology, Cell biology, medicine.anatomical_structure, KLF4, 030220 oncology & carcinogenesis

Abstract

Epithelial cells rapidly adapt their behaviour in response to increasing tissue demands. However, the processes that finely control these cell decisions remain largely unknown. The postnatal period covering the transition between early tissue expansion and the establishment of adult homeostasis provides a convenient model with which to explore this question. Here, we demonstrate that the onset of homeostasis in the epithelium of the mouse oesophagus is guided by the progressive build-up of mechanical strain at the organ level. Single-cell RNA sequencing and whole-organ stretching experiments revealed that the mechanical stress experienced by the growing oesophagus triggers the emergence of a bright Krüppel-like factor 4 (KLF4) committed basal population, which balances cell proliferation and marks the transition towards homeostasis in a yes-associated protein (YAP)-dependent manner. Our results point to a simple mechanism whereby mechanical changes experienced at the whole-tissue level are integrated with those sensed at the cellular level to control epithelial cell fate.

Published

2021

14. Selective N-Terminal Acylation of Peptides and Proteins with Tunable Phenol Esters

Author

Jesper H. Mikkelsen, Magnus B. F. Gustafsson, Troels Skrydstrup, and Kim B. Jensen

Subjects

Pharmacology, Biological Products, NATIVE PEPTIDES, Phenol, Acylation, Organic Chemistry, Biomedical Engineering, Proteins, Pharmaceutical Science, EFFICIENT, Esters, Bioengineering, Glucagon-Like Peptide 1, RESIDUES, Humans, Insulin, BIOTINYLATION, Amino Acid Sequence, Peptides, Biotechnology

Abstract

Selective modification of peptides and proteins is of foremost importance for the development of biopharmaceuticals and exploring biochemical pathways, as well as other applications. Here, we present a study on the development of a general and easily applicable selective method for N-terminal acylation of biomolecules, applying a new type of phenol esters. Key to the success was the development of highly tunable phenol activators bearing in the ortho-position, sulfonic acid or sulfonamide, acting as a steric shield for hydrolysis, and electron-withdrawing groups in the other ortho- and para-position for controlling the reactivity of the activated phenol esters. A library of heptapeptides, testing all 20 natural amino acids positioned at the N-terminal, were acylated in a selective manner at the N-terminus. The majority showed high conversion and excellent N α-selectivity. Several biologically relevant biomolecules, including DesB30 insulin and human growth hormone, could also be modified at the N-terminal in a highly selective way, exemplified by either a fluorophore or a fatty acid sidechain. Finally, taking advantage of the possibility to accurately adjust the reactivity of the phenol esters, we present a potential strategy for the construction of dual active biopharmaceuticals through the employment of a bifunctional acylation linker and demonstrate its use in the creation of a GLP-1 insulin analogue, coupled through the lysine residue of GLP-1 and the N-terminal Phe B1amine of DesB30 insulin.

Published

2022

15. Author Reply to Peer Reviews of Fibronectin meshwork controls epithelial stem cell fate

Author

Chloé C. Féral, Kim B Jensen, Ludovic Cervera, Laurence Cailleteau, Floriane S. Tissot, Lionel Tosello, and Soline Estrach

Published

2022

16. Lrig1 expression identifies airway basal cells with high proliferative capacity and restricts lung squamous cell carcinoma growth

Author

Kim B. Jensen, Sandra Gómez-López, Adam Pennycuick, Ahmed S. N. Alhendi, Laura Succony, Derek Davies, Kate H.C. Gowers, Nicholas A. Wright, Sam M. Janes, and Sarah E. Clarke

Subjects

Pulmonary and Respiratory Medicine, Cell of origin, Immunology, 03 medical and health sciences, Basal (phylogenetics), 0302 clinical medicine, medicine, 030212 general & internal medicine, Progenitor cell, Lung cancer, Human Biology & Physiology, business.industry, Stem Cells, FOS: Clinical medicine, Cancer, Cell Biology, Tumour Biology, medicine.disease, 3. Good health, 030228 respiratory system, Cancer research, Respiratory epithelium, Cell Cycle & Chromosomes, business, Airway, Homeostasis

Abstract

BackgroundLung squamous cell carcinoma (LUSC) accounts for a significant proportion of cancer deaths worldwide, and is preceded by the appearance of progressively disorganised pre-invasive lesions in the airway epithelium. Yet the biological mechanisms underlying progression of pre-invasive lesions into invasive LUSC are not fully understood. LRIG1 (leucine-rich repeats and immunoglobulin-like domains 1) is downregulated in pre-invasive airway lesions and invasive LUSC tumours and this correlates with decreased lung cancer patient survival.Methods and resultsUsing an Lrig1 knock-in reporter mouse and human airway epithelial cells collected at bronchoscopy, we show that during homeostasis LRIG1 is heterogeneously expressed in the airway epithelium. In basal airway epithelial cells, the suspected cell of origin of LUSC, LRIG1 identifies a subpopulation of progenitor cells with higher in vitro proliferative and self-renewal potential in both the mouse and human. Using the N-nitroso-tris-chloroethylurea (NTCU)-induced murine model of LUSC, we find that Lrig1 loss-of-function leads to abnormally high cell proliferation during the earliest stages of pre-invasive disease and to the formation of significantly larger invasive tumours, suggesting accelerated disease progression.ConclusionTogether, our findings identify LRIG1 as a marker of basal airway progenitor cells with high proliferative potential and as a regulator of pre-invasive lung cancer progression. This work highlights the clinical relevance of LRIG1 and the potential of the NTCU-induced LUSC model for functional assessment of candidate tumour suppressors and oncogenes.

Published

2022

17. Extracellular matrix interactions provide tumor cells with an escape mechanism for commitment to differentiation

Author

Pawel J. Schweiger, Marie Le Bouteiller, Shiro Yui, Malte Thodberg, Ditte Clement, and Kim B. Jensen

Subjects

Hepatology, Gastroenterology, Humans, Cell Count, Cell Differentiation, Extracellular Matrix

Published

2022

18. Transplantation of intestinal organoids into a mouse model of colitis

Author

Satoshi Watanabe, Sakurako Kobayashi, Nobuhiko Ogasawara, Ryuichi Okamoto, Tetsuya Nakamura, Mamoru Watanabe, Kim B. Jensen, and Shiro Yui

Subjects

Intestines, Organoids, Mice, Animals, Intestinal Mucosa, Colitis, General Biochemistry, Genetics and Molecular Biology

Abstract

Intestinal organoids are fundamental in vitro tools that have enabled new research opportunities in intestinal stem cell research. Organoids can also be transplanted in vivo, which enables them to probe stem cell potential and be used for disease modeling and as a preclinical tool in regenerative medicine. Here we describe in detail how to orthotopically transplant epithelial organoids into the colon of recipient mice. In this assay, epithelial injury is initiated at the distal part of colon by the administration of dextran sulfate sodium, and organoids are infused into the luminal space via the anus. The infused organoids subsequently attach to the injured region and rebuild a donor-derived epithelium. The steps for cell infusion can be completed in 10 min. The assay has been applied successfully to organoids derived from both wild-type and genetically altered epithelial cells from adult colonic and small intestinal epithelium, as well as fetal small intestine. This is a versatile protocol, providing the technical basis for transplantation following alternative colonic injury models. It has been used previously for functional assays to probe cellular potential, and formed the basis for the first in-human clinical trial using colonic organoid transplantation therapy for intractable cases of ulcerative colitis.

Published

2022

19. New Phenol Esters for Efficient pH-Controlled Amine Acylation of Peptides, Proteins, and Sepharose Beads in Aqueous Media

Author

Kim B. Jensen, Jesper H. Mikkelsen, Simon P. Jensen, Steffen Kidal, Gitte Friberg, Troels Skrydstrup, and Magnus B. F. Gustafsson

Subjects

Pharmacology, Phenol, Organic Chemistry, Biomedical Engineering, Pharmaceutical Science, Bioengineering, Biotechnology

Abstract

This paper describes the discovery, synthesis, and use of novel water-soluble acylation reagents for efficient and selective modification, cross-linking, and labeling of proteins and peptides, as well as for their use in the effective modification of sepharose beads under pH control in aqueous media. The reagents are based on a 2,4-dichloro-6-sulfonic acid phenol ester core combined with a variety of linker structures. The combination of these motifs leads to an ideal balance between hydrolytic stability and reactivity. At high pH, good to excellent conversions (up to 95%) and regioselectivity (up to 99:1 Nϵ/Nα amine ratio) in the acylation were realized, exemplified by the chemical modification of incretin peptides and insulin. At neutral pH, an unusually high preference toward the N-terminal phenylalanine in an insulin derivative was observed (>99:1 Nα/Nϵ), which is up until now unprecedented in the literature for more elaborate reagents. In addition, the unusually high hydrolytic stability of these reagents and their ability to efficiently react at low concentrations (28 μM or 0.1 mg/mL) are exemplified with a hydroxy linker-based reagent and are a unique feature of this work.

Published

2021

20. TGF-β modulates cell fate in human ES cell-derived foregut endoderm by inhibiting multiple endogenous signaling pathways

Author

Kim B. Jensen, M. S. Hansen, Palle Serup, J. v. C. Kuylenstierna, N. S. Funa, K. H. de Lichtenberg, Kenan Christopher Garcia, and Yi Miao

Subjects

Directed differentiation, medicine.anatomical_structure, Chemistry, Wnt signaling pathway, medicine, Foregut, Cell fate determination, Endoderm, Signal transduction, Induced pluripotent stem cell, Embryonic stem cell, Cell biology

Abstract

SummaryGenetic differences between pluripotent stem cell lines causes variable activity of extra-cellular signaling pathways, which limits the reproducibility of directed differentiation protocols. Here we used human embryonic stem cells (hESCs) to interrogate how exogenously provided factors modulate endogenous signaling events during specification of foregut endoderm lineages. We find that TGF-β1 activates an OTX2/LHX1 gene regulatory network that promotes anterior fate by antagonizing endogenous Wnt signaling. In contrast to Porcupine inhibition, the effects of TGF-β1 cannot be reversed by exogenous Wnt ligands, suggesting that induction of SHISA proteins and intracellular accumulation of Fzd receptors make TGF-β1 treated cells refractory to Wnt signaling. Subsequently, TGF-β1-mediated inhibition of Bmp- and Wnt-signaling suppresses liver- and promotes pancreas fate. However, pancreas differentiation is delayed by TGF-β1-induced CYP26A1 expression and inhibition of RA signaling. Our study thus identifies multiple mechanisms of crosstalk between major developmental signaling pathways during foregut patterning.

Published

2021

21. Fetal-like reversion in the regenerating intestine is regulated by mesenchymal Asporin

Author

Menno J. Oudhoff, Nalle Pentinmikko, Kirsi H. Pietiläinen, Alessandro Ori, Tuure Saarinen, Simon Andersson, Anne Juuti, Sharif Iqbal, Anna Taylor Webb, Markku Varjosalo, Pekka Katajisto, Nestaite E, Ashwini Kumar, Kim B. Jensen, and Borshagovski D

Subjects

0303 health sciences, Decellularization, Mesenchyme, Regeneration (biology), Asporin, Biology, Epithelium, Cell biology, Extracellular matrix, 03 medical and health sciences, 0302 clinical medicine, medicine.anatomical_structure, 030220 oncology & carcinogenesis, medicine, Reprogramming, Tissue homeostasis, 030304 developmental biology

Abstract

Epithelial tissues undergo fetal-like cellular reprogramming to regenerate after damage1,2. Although the mesenchyme and the extracellular matrix (ECM) play critical roles in tissue homeostasis and regeneration2–5, their role in repurposing developmental programs in epithelium is unknown. To model epithelial regeneration, we culture intestinal epithelium on decellularized small intestinal scaffold (iECM), and identify Asporin (Aspn), an ECM bound proteoglycan, as a critical mediator of cellular reprogramming. Aspn is produced by the mesenchyme, and we show that its effect on epithelial Tgfβ-signalling via CD44 is critical for fetal-like conversion. Furthermore, we demonstrate that Aspn is transiently increased upon chemotherapy-induced damage and pivotal for a timely induction of the fetal-like state and tissue regeneration. In summary, we establish a platform for modelling epithelial injury responses ex vivo, and show that the mesenchymal Aspn-producing niche controls tissue repair by regulating epithelial fetal-like reprogramming.

Published

2021

22. Fibronectin meshwork controls epithelial stem cell fate

Author

Cervera L, Floriane S. Tissot, Kim B. Jensen, Lionel Tosello, Laurence Cailleteau, Chloé C. Féral, and Soline Estrach

Subjects

Extracellular matrix, Fibronectin, biology, Chemistry, Regeneration (biology), Integrin, biology.protein, Compartment (development), Stem cell, Wound healing, Cell biology, Adult stem cell

Abstract

Adult stem cell fate is tightly balanced by the local microenvironment called niche and sustain tissue regeneration1–4. How niche signals are integrated and regulate regeneration remains largely unexplored. The extracellular matrix and integrin ligand fibronectin is a crucial and well-characterized wound healing actor that has never been involved in skin regeneration. Here, we show that fibronectin displays a highly specific enrichment in hair follicle stem cells (HFSC) at the onset of regeneration. Conditional deletion of fibronectin in HFSC compartment (Lrig1, K19) leads to hair regeneration blockade, impaired stem cell location and fate. Dermal injection of exogenous fibronectin rescues these phenotypes. To elucidate molecular mechanism underlying fibronectin function, we used conditional deletion models of SLC3A2, the main integrin coreceptor. We show that, via its role in integrin-dependent assembly of fibronectin matrix, SLC3A2 acts as molecular relay of niche signals. Thus, fibronectin-integrin-SLC3A2 cascade finely tunes HFSC fate and tissue regenerative power.

Published

2021

23. A Nickel(II)-Mediated Thiocarbonylation Strategy for Carbon Isotope Labeling of Aliphatic Carboxamides

Author

Troels Skrydstrup, Kim B. Jensen, Magnus Gustafsson, Aske S. Donslund, Florian Papp, Simon S. Pedersen, Jesper H. Mikkelsen, and Oskar S. Bakholm

Subjects

chemistry.chemical_classification, thioesters, Sulfide, aminocarbonylation, 010405 organic chemistry, Organic Chemistry, General Chemistry, aliphatic carboxamides, 010402 general chemistry, Thioester, 01 natural sciences, Combinatorial chemistry, Small molecule, Catalysis, Reductive elimination, 0104 chemical sciences, Acylation, chemistry.chemical_compound, nickel, chemistry, Isotopes of carbon, TheoryofComputation_ANALYSISOFALGORITHMSANDPROBLEMCOMPLEXITY, isotope labeling, Alkyl, Carbon monoxide

Abstract

A series of pharmaceutically relevant small molecules and biopharmaceuticals bearing aliphatic carboxamides have been successfully labeled with carbon-13. Key to the success of this novel carbon isotope labeling technique is the observation that 13C-labeled NiII-acyl complexes, formed from a 13CO insertion step with NiII-alkyl intermediates, rapidly react in less than one minute with 2,2’-dipyridyl disulfide to quantitatively form the corresponding 2-pyridyl thioesters. Either the use of 13C-SilaCOgen or 13C-COgen allows for the stoichiometric addition of isotopically labeled carbon monoxide. Subsequent one-pot acylation of a series of structurally diverse amines provides the desired 13C-labeled carboxamides in good yields. A single electron transfer pathway is proposed between the NiII-acyl complexes and the disulfide providing a reactive NiIII-acyl sulfide intermediate, which rapidly undergoes reductive elimination to the desired thioester. By further optimization of the reaction parameters, reaction times down to only 11 min were identified, opening up the possibility of exploring this chemistry for carbon-11 isotope labeling. Finally, this isotope labeling strategy could be adapted to the synthesis of 13C-labeled liraglutide and insulin degludec, representing two antidiabetic drugs.

Published

2021

24. A biomechanical switch regulates the transition towards homeostasis in esophageal epithelium

Author

Jamie McGinn, Maria P. Alcolea, Frances J. England, Christophe M. Verstreken, Svetlana Ulyanchenko, Seungmin Han, Kevin J. Chalut, Adrien Hallou, Ramiro Iglesias-Bartolome, Kim B. Jensen, Kata Krizic, and Benjamin D. Simons

Subjects

education.field_of_study, Mechanism (biology), Cell, Population, RNA, Biology, Epithelium, Cell biology, medicine.anatomical_structure, medicine, Compartment (development), education, Homeostasis, Progenitor

Abstract

Epithelial cells are highly dynamic and can rapidly adapt their behavior in response to tissue perturbations and increasing tissue demands. However, the processes that finely control these responses and, particularly, the mechanisms that ensure the correct switch to and from normal tissue homeostasis are largely unknown. Here we explore changes in cell behavior happening at the interface between postnatal development and homeostasis in the epithelium of the mouse esophagus, as a physiological model exemplifying a rapid but controlled tissue growth transition. Single cell RNA sequencing and histological analysis of the mouse esophagus reveal significant mechanical changes in the epithelium upon tissue maturation. Organ stretching experiments further indicate that tissue strain caused by the differential growth of the mouse esophagus relative to the entire body promotes the emergence of a defined committed population in the progenitor compartment as homeostasis is established. Our results point to a simple mechanism whereby the mechanical changes experienced at the whole tissue level are integrated with those “sensed” at the cellular level to control epithelial cell behavior and tissue maintenance.

Published

2021

25. A semi-automated organoid screening method demonstrates epigenetic control of intestinal epithelial maturation

Author

Marianne Terndrup Pedersen, Cheryl H. Arrowsmith, Menno J. Oudhoff, Naveen Parmar, Rosalie T. Zwiggelaar, Kim B. Jensen, Jenny Ostrop, Håvard T. Lindholm, Alberto Díez-Sánchez, François Gerbe, Silke Radetzki, Jens Peter von Kries, Philippe Jay, and Korbinian Bösl

Subjects

LGR5, Organoid, Epigenetics, Stem cell, Biology, Embryonic stem cell, Intestinal epithelium, Epithelium, Cell biology, Adult stem cell

Abstract

The intestinal epithelium maintains an important barrier throughout life. It consists of several epithelial cell lineages that are derived from LGR5+ intestinal stem cells. Although epigenetic regulation of embryonic stem cell differentiation is well established, its role in adult stem cell systems such as the intestinal epithelium is still undefined. Yet, targeting of epigenetic regulatory enzymes may be relevant for new therapeutics, for example in cancer treatment. Here, we combine a newly established organoid toolbox with an epigenetic probe library to identify epigenetic regulators of intestinal epithelial biology. We discover several probes that alter intestinal epithelial biology including those targeting HDACs, EP300/CREBBP, LSD1, and type I PRMTs. We conclude that epigenetic modifiers are primarily involved in mediating maturation of the epithelium rather than dictating specific cell lineage differentiation. Furthermore, we show that inhibiting type I PRMTs, which leads to epithelial maturation, blocks the growth of adenoma but not normal organoid cultures. Thus, epigenetic probes are a powerful tool in defining biological processes and demonstrate therapeutic potential.

Published

2020

26. Mucosal vitamin D signaling in inflammatory bowel disease

Author

Kim B. Jensen, Ole Haagen Nielsen, Alan C. Moss, Lauge Kellermann, Fredrik Bergenheim, John Gubatan, and Naomi D. Chou

Subjects

0301 basic medicine, Cell signaling, Immunology, Inflammation, Calcitriol receptor, Inflammatory bowel disease, Tight Junctions, Pathogenesis, 03 medical and health sciences, 0302 clinical medicine, Immune system, Vitamin D and neurology, medicine, Immunology and Allergy, Humans, Intestinal Mucosa, Vitamin D, 030203 arthritis & rheumatology, business.industry, medicine.disease, Inflammatory Bowel Diseases, Gastrointestinal Microbiome, 030104 developmental biology, medicine.symptom, business, Hormone, Signal Transduction

Abstract

Epidemiological studies have identified vitamin D (25(OH)D) deficiency to be highly prevalent among patients with inflammatory bowel disease (IBD), and low serum levels correlate with a higher disease activity and a more complicated disease course. The link to IBD pathogenesis has been subject of investigations, primarily due to the distinct immunological functions of vitamin D signaling, including anti-inflammatory and anti-fibrotic actions. Vitamin D is a pleiotropic hormone that executes its actions on cells through the vitamin D receptor (VDR). A leaky gut, i.e. an insufficient intestinal epithelial barrier, is thought to be central for the pathogenesis of IBD, and emerging data support the concept that vitamin D/VDR signaling in intestinal epithelial cells (IECs) has an important role in controlling barrier integrity. Here we review the latest evidence on how vitamin D promotes the interplay between IECs, the gut microbiome, and immune cells and thereby regulate the intestinal immune response. On the cellular level, vitamin D signaling regulates tight junctional complexes, apoptosis, and autophagy, leading to increased epithelial barrier integrity, and promotes expression of antimicrobial peptides as part of its immunomodulating functions. Further, intestinal VDR expression is inversely correlated with the severity of inflammation in patients with IBD, which might compromise the positive effects of vitamin D signaling in patients with flaring disease. Efforts to reveal the role of vitamin D in the pathophysiology of IBD will pave the road for the invention of more rational treatment strategies of this debilitating disease in the future.

Published

2020

27. Managing vitamin D deficiency in inflammatory bowel disease

Author

Ole Haagen Nielsen, Lars Rejnmark, Kim B. Jensen, Thomas Irgens Hansen, and John Gubatan

Subjects

medicine.medical_specialty, vitamin D, Disease, digestive system, Inflammatory bowel disease, vitamin D deficiency, inflammatory bowel disease, Internal medicine, medicine, Vitamin D and neurology, biologics, In patient, Vitamin D, therapy, Hepatology, Vitamin d supplementation, business.industry, Gastroenterology, clinical control, medicine.disease, Ulcerative colitis, digestive system diseases, Clinical trial, Small bowel and Nutrition, business

Abstract

Management of inflammatory bowel disease (IBD), including ulcerative colitis and Crohn’s disease, is generally cumbersome for patients and is a massive health-economic burden. In recent years, the immunomodulating effects of vitamin D have gained a huge interest in its possible pathogenic influence on the pathophysiology of IBD. Vitamin D deficiency is frequent among patients with IBD. Several clinical studies have pointed to a critical role for vitamin D in ameliorating disease outcomes. Although causation versus correlation unfortunately remains an overwhelming issue in the illusive chicken versus egg debate regarding vitamin D and IBD, here we summarise the latest knowledge of the immunological effects of vitamin D in IBD and recommend from available evidence that physicians regularly monitor serum 25(OH)D levels in patients with IBD. Moreover, we propose an algorithm for optimising vitamin D status in patients with IBD in clinical practice. Awaiting well-powered controlled clinical trials, we consider vitamin D supplementation to be an affordable and widely accessible therapeutic strategy to ameliorate IBD clinical outcomes.

Published

2019

28. Dietary Control of Skin Lipid Composition and Microbiome

Author

Yun Chen, Kim B. Jensen, Kasper S. Moestrup, Troels Schepeler, and Pawel J. Schweiger

Subjects

0301 basic medicine, Microbiota, 030106 microbiology, Dietary control, High fat diet, Cell Biology, Dermatology, Biology, Diet, High-Fat, Lipids, Biochemistry, 030207 dermatology & venereal diseases, 03 medical and health sciences, 0302 clinical medicine, High fat, Animals, Humans, Composition (visual arts), Microbiome, Food science, Skin lipid, Molecular Biology, Adiposity, Skin

Published

2018

29. Loss of PACS-2 delays regeneration in DSS-induced colitis but does not affect the ApcMin model of colorectal cancer

Author

Jeanette Schwarz, Marie Kveiborg, Jacob Samsøe-Petersen, Kim B. Jensen, Gary Thomas, Reidar Albrechtsen, and Sarah Louise Dombernowsky

Subjects

0301 basic medicine, medicine.medical_specialty, PACS-2, Proliferative index, Colorectal cancer, Cell, 03 medical and health sciences, Medicine, Colitis, DSS-induced colitis, ApcMin model, ADAM17, business.industry, Regeneration (biology), General surgery, medicine.disease, Intestinal epithelium, humanities, Epithelium, Colon cancer, 3. Good health, 030104 developmental biology, medicine.anatomical_structure, Oncology, colon cancer, Cancer research, Apc model, Stem cell, business, Priority Research Paper

Abstract

// Sarah L. Dombernowsky 1,* , Jeanette Schwarz 1,* , Jacob Samsoe-Petersen 1 , Reidar Albrechtsen 1 , Kim B. Jensen 1,2 , Gary Thomas 3 and Marie Kveiborg 1 1 Biotech Research and Innovation Centre, University of Copenhagen, Copenhagen, Denmark 2 Novo Nordisk Foundation Center for Stem Cell Biology, University of Copenhagen, Copenhagen, Denmark 3 Department of Microbiology and Molecular Genetics, University of Pittsburgh School of Medicine, Pittsburgh, PA, USA * These authors have contributed equally to this work Correspondence to: Marie Kveiborg, email: // Keywords : DSS-induced colitis; colon cancer; ApcMin model; PACS-2; ADAM17 Received : May 07, 2017 Accepted : October 28, 2017 Published : November 26, 2017 Abstract PACS-2 is a multifunctional sorting protein that mediates cell homeostasis. We recently identified PACS-2 in a functional genome-wide siRNA screen for novel regulators of the metalloproteinase ADAM17, the main sheddase for ligands of the ErbB receptor family. Of note, we showed that Pacs2 -/- mice have significantly reduced EGFR activity and proliferative index in the intestinal epithelium. As EGFR signaling is highly mitogenic for intestinal epithelial stem cells, and plays essential roles in intestinal epithelial regeneration and tumor development, we have now examined the role of PACS-2 in these processes. Specifically, we analyzed the role of Pacs 2-deficiency in a DSS-induced colitis model as well as in the genetic Apc Min colon cancer model. We now report that loss of PACS-2 delays tissue regeneration after colonic injury with little effect on key inflammatory parameters. We did however not observe any apparent effects on tumor formation driven by excessive proliferative signaling downstream from APC-deficiency. Our findings reveal that the role of PACS-2 in regulating ADAM17-mediated shedding is not an obligate requirement for the epithelium to respond to the strong inflammatory or tumorigenic inducers in the models assessed here.

Published

2017

30. Intestinal Organoids: A Tool for Modelling Diet–Microbiome–Host Interactions

Author

Kim B. Jensen, Fulvio Mattivi, Kieran Tuohy, Pawel J. Schweiger, Andrea Lunardi, and Josep Rubert

Subjects

Multi-Omics, Colorectal cancer, Endocrinology, Diabetes and Metabolism, microbiome, single cell analysis, 030209 endocrinology & metabolism, Computational biology, Biology, 03 medical and health sciences, 0302 clinical medicine, Endocrinology, Single-cell analysis, gut microbial metabolites, medicine, Metabolomics, Animals, Humans, Microbiome, Settore CHIM/10 - CHIMICA DEGLI ALIMENTI, Host (biology), Intestinal Organoids, Diet, Gut Microbial Metabolites, Microbiota, Intestinal organoids, medicine.disease, phytochemicals, In vitro, 3. Good health, Gastrointestinal Microbiome, Organoids, intestinal organoids, Single-Cell Analysis, Dysbiosis, Homeostasis

Abstract

Dietary patterns, microbiome dysbiosis, and gut microbial metabolites (GMMs) have a pivotal role in the homeostasis of intestinal epithelial cells and in disease progression, such as that of colorectal cancer (CRC). Although GMMs and microorganisms have crucial roles in many biological activities, models for deciphering diet–microbiome–host relationships are largely limited to animal models. Thus, intestinal organoids (IOs) have provided unprecedented opportunities for the generation of in vitro platforms with the sufficient level of complexity to model physiological and pathological diet–microbiome–host conditions. Overall, IO responses to GMM metabolites and microorganisms can provide new insights into the mechanisms by which those agents may prevent or trigger diseases, significantly extending our knowledge of diet–microbiome–host interactions.

Published

2020

31. Tissue-Engineering the Intestine: The Trials before the Trials

Author

Matthias P. Lutolf, Vivian S. W. Li, Kim B. Jensen, Ryan K. Conder, Paolo De Coppi, Sarah Chan, Tracy C. Grikscheit, Ludovic Vallier, Hans Clevers, and Hubrecht Institute for Developmental Biology and Stem Cell Research

Subjects

Short Bowel Syndrome, Scaffold, media_common.quotation_subject, Organogenesis, Induced Pluripotent Stem Cells, Cell Culture Techniques, Design strategy, Biology, 03 medical and health sciences, 0302 clinical medicine, Tissue scaffolds, Tissue engineering, Genetics, medicine, Animals, Humans, Function (engineering), 030304 developmental biology, media_common, Cell Proliferation, 0303 health sciences, Tissue Engineering, Tissue Scaffolds, Cell Differentiation, Cell Biology, Short bowel syndrome, medicine.disease, Intestines, Organoids, Risk analysis (engineering), Molecular Medicine, 030217 neurology & neurosurgery

Abstract

Building complex tissues requires the development of innovative interdisciplinary engineering solutions. In this Forum, the INTENS Consortium discuss experimental considerations and challenges for generating a tissue-engineered intestine for the treatment of short bowel syndrome, taking into account cell source, scaffold choice, and design strategy for achieving proper assembly and function.

Published

2019

32. Tracing the origin of adult intestinal stem cells

Author

Kristine J. Hare, Svetlana Ulyanchenko, Agnete Larsen, Lea Langhoff Thuesen, Anne Jørgensen, Jordi Guiu, Rasmus H. Olesen, Shiro Yui, Signe Perlman, Edouard Hannezo, Tune H. Pers, Martti Maimets, Samuel Demharter, Benjamin D. Simons, Kim B. Jensen, Konstantin Khodosevich, Lene Lundvall, Linn Salto Mamsen, Claus Yding Andersen, Simons, Benjamin [0000-0002-3875-7071], and Apollo - University of Cambridge Repository

Subjects

Male, 0301 basic medicine, Cellular differentiation, Fetus/cytology, Biology, digestive system, Article, Receptors, G-Protein-Coupled, Mice, 03 medical and health sciences, Fetus, 0302 clinical medicine, Intestinal mucosa, Stem Cells/cytology, Animals, Regeneration, Cell Lineage, Intestinal Mucosa, Stem Cell Niche, Intestinal Mucosa/cytology, Multidisciplinary, Stem Cells, LGR5, Cell Differentiation, Receptors, G-Protein-Coupled/metabolism, Cellular Reprogramming, Intestinal epithelium, Cell biology, Transplantation, Intestines, 030104 developmental biology, Female, Stem cell, Reprogramming, 030217 neurology & neurosurgery, Intestines/cytology, Adult stem cell

Abstract

Adult intestinal stem cells are located at the bottom of crypts of Lieberkuhn, where they express markers such as LGR51,2 and fuel the constant replenishment of the intestinal epithelium1. Although fetal LGR5-expressing cells can give rise to adult intestinal stem cells3,4, it remains unclear whether this population in the patterned epithelium represents unique intestinal stem-cell precursors. Here we show, using unbiased quantitative lineage-tracing approaches, biophysical modelling and intestinal transplantation, that all cells of the mouse intestinal epithelium—irrespective of their location and pattern of LGR5 expression in the fetal gut tube—contribute actively to the adult intestinal stem cell pool. Using 3D imaging, we find that during fetal development the villus undergoes gross remodelling and fission. This brings epithelial cells from the non-proliferative villus into the proliferative intervillus region, which enables them to contribute to the adult stem-cell niche. Our results demonstrate that large-scale remodelling of the intestinal wall and cell-fate specification are closely linked. Moreover, these findings provide a direct link between the observed plasticity and cellular reprogramming of differentiating cells in adult tissues following damage5–9, revealing that stem-cell identity is an induced rather than a hardwired property. Lineage tracing, biophysical modelling and intestinal transplantation approaches are used to demonstrate that, in the mouse fetal intestinal epithelium, cells are highly plastic with respect to cellular identity and, independent of LGR5 expression and cell position, can contribute to the adult stem cell compartment.

Published

2019

33. Cover Feature: A Nickel(II)‐Mediated Thiocarbonylation Strategy for Carbon Isotope Labeling of Aliphatic Carboxamides (Chem. Eur. J. 24/2021)

Author

Jesper H. Mikkelsen, Kim B. Jensen, Troels Skrydstrup, Oskar S. Bakholm, Florian Papp, Aske S. Donslund, Simon S. Pedersen, and Magnus Gustafsson

Subjects

Nickel, chemistry, Feature (computer vision), Isotopes of carbon, Organic Chemistry, chemistry.chemical_element, Organic chemistry, Cover (algebra), General Chemistry, Catalysis

Published

2021

34. Tu1266 IMPAIRED VITAMIN D RECEPTOR EXPRESSION AND SIGNALING IN ULCERATIVE COLITIS INTESTINAL EPITHELIAL CELLS

Author

Lauge Kellermann, Marianne Terndrup Pedersen, Stine Lund Hansen, Grzegorz Maciag, Lene Riis, Fredrik Bergenheim, Ole Haagen Nielsen, and Kim B. Jensen

Subjects

Hepatology, business.industry, Gastroenterology, Cancer research, Medicine, business, medicine.disease, Calcitriol receptor, Ulcerative colitis

Published

2020

35. IL-17R–EGFR axis links wound healing to tumorigenesis in Lrig1 + stem cells

Author

Liang Zhu, Junjie Zhao, Shlomo A. Koyfman, Brian R. Gastman, Xing Chen, Caini Liu, Cun-jin Zhang, Chunfang Gu, Ling Wu, Gang Cai, Thomas A. Hamilton, Xiaoxia Li, Jun Qin, Jennifer S. Ko, Kim B. Jensen, and Allison T. Vidimos

Subjects

0301 basic medicine, education.field_of_study, TRAF4, Epidermis (botany), Immunology, Population, Signal transducing adaptor protein, Biology, medicine.disease_cause, Cell biology, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, medicine, Immunology and Allergy, Stem cell, Signal transduction, Carcinogenesis, Wound healing, education, 030215 immunology

Abstract

Lrig1 marks a distinct population of stem cells restricted to the upper pilosebaceous unit in normal epidermis. Here we report that IL-17A–mediated activation of EGFR plays a critical role in the expansion and migration of Lrig1 + stem cells and their progenies in response to wounding, thereby promoting wound healing and skin tumorigenesis. Lrig1-specific deletion of the IL-17R adaptor Act1 or EGFR in mice impairs wound healing and reduces tumor formation. Mechanistically, IL-17R recruits EGFR for IL-17A–mediated signaling in Lrig1 + stem cells. While TRAF4, enriched in Lrig1 + stem cells, tethers IL-17RA and EGFR, Act1 recruits c-Src for IL-17A–induced EGFR transactivation and downstream activation of ERK5, which promotes the expansion and migration of Lrig1 + stem cells. This study demonstrates that IL-17A activates the IL-17R–EGFR axis in Lrig1 + stem cells linking wound healing to tumorigenesis.

Published

2019

36. Tracing the cellular dynamics of sebaceous gland development in normal and perturbed states

Author

Marianne S. Andersen, Soline Estrach, Kim B. Jensen, Kim E Boonekamp, Jens Vilstrup Johansen, Sarah Sendrup, Sabrina Pisano, Ditte L. Clement, Edouard Hannezo, Yasuko Antoku, Benjamin D. Simons, Marianne Terndrup Pedersen, Chloé C. Féral, Svetlana Ulyanchenko, Martti Maimets, Institute of Science and Technology [Austria] (IST Austria), Biologie et physiopathologie cutanées : expression génique, signalisation et thérapie, Université Nice Sophia Antipolis (... - 2019) (UNS), COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-IFR50-Institut National de la Santé et de la Recherche Médicale (INSERM), CNRS UMR7284, INSERM U1081, Institute for Research on Cancer and Aging, Nice (IRCAN), Université Côte d'Azur (UCA), University of Copenhagen = Københavns Universitet (KU), Régulation des gènes et signalisation cellulaire, Institut National de la Santé et de la Recherche Médicale (INSERM), University of Cambridge [UK] (CAM), Department of Materials and Production [Aalborg], Aalborg University [Denmark] (AAU), Andersen, Marianne Stemann [0000-0001-6751-5453], Hannezo, Edouard [0000-0001-6005-1561], Ulyanchenko, Svetlana [0000-0003-3124-9178], Estrach, Soline [0000-0003-2088-5988], Pisano, Sabrina [0000-0002-2452-4736], Maimets, Martti [0000-0001-7343-2769], Feral, Chloe C [0000-0001-9756-2082], Simons, Benjamin D [0000-0002-3875-7071], Jensen, Kim B [0000-0001-6569-1664], and Apollo - University of Cambridge Repository

Subjects

Sebaceous gland, Cell division, Mice, Transgenic, Biology, Cell fate determination, Article, 03 medical and health sciences, 0302 clinical medicine, Stroma, Fate mapping, medicine, Animals, Homeostasis, Progenitor cell, [SDV.BDD]Life Sciences [q-bio]/Development Biology, ComputingMilieux_MISCELLANEOUS, 030304 developmental biology, Cell Proliferation, Regulation of gene expression, 0303 health sciences, [SDV.BA.MVSA]Life Sciences [q-bio]/Animal biology/Veterinary medicine and animal Health, Oncogene, Stem Cells, Gene Expression Regulation, Developmental, [SDV.BDD.MOR]Life Sciences [q-bio]/Development Biology/Morphogenesis, Cell Biology, Cell biology, medicine.anatomical_structure, 030220 oncology & carcinogenesis, Disease Progression

Abstract

The sebaceous gland (SG) is an essential component of the skin, and SG dysfunction is debilitating(1, 2). Yet, the cellular bases for its origin, development and subsequent maintenance remain poorly understood. Here, we apply large-scale quantitative fate mapping to define the patterns of cell fate behaviour during SG development and maintenance. We show that the SG develops from a defined number of lineage-restricted progenitors that undergo a programme of independent and stochastic cell fate decisions. Following an expansion phase, equipotent progenitors transition into a phase of homeostatic turnover, which is correlated with changes in the mechanical properties of the stroma and spatial restrictions on gland size. Expression of the oncogene KrasG12D results in a release from these constraints and unbridled gland expansion. Quantitative clonal fate analysis reveals that, during this phase, the primary effect of the Kras-oncogene is to drive a constant fate bias with little effect on cell division rates. These findings provide insight into the developmental programme of the SG, as well as the mechanisms that drive tumour progression and gland dysfunction.

Published

2019

37. Lrig1 marks a population of gastric epithelial cells capable of long-term tissue maintenance and growth in vitro

Author

Gabor Sirokmány, Troels Schepeler, Pawel J. Schweiger, Mahalia E. Page, Xiangang Zou, Kim B. Jensen, Fiona M. Watt, and Ditte L. Clement

Subjects

0301 basic medicine, Cellular differentiation, Population, lcsh:Medicine, Mice, Transgenic, Nerve Tissue Proteins, Biology, Article, Mice, 03 medical and health sciences, Gastric glands, medicine, Organoid, Animals, lcsh:Science, education, Cells, Cultured, Cell Proliferation, education.field_of_study, Membrane Glycoproteins, Multidisciplinary, Stomach, lcsh:R, Cell Differentiation, Epithelial Cells, Cell Dedifferentiation, Pylorus, Epithelium, In vitro, Cell biology, Mice, Inbred C57BL, 030104 developmental biology, medicine.anatomical_structure, Gastric Mucosa, lcsh:Q, Biomarkers

Abstract

The processes involved in renewal of the epithelium that lines the mouse stomach remain unclear. Apart from the cells in the isthmus, several other populations located deeper in the gastric glands have been suggested to contribute to the maintenance of the gastric epithelium. Here, we reveal that Lrig1 is expressed in the basal layer of the forestomach and the lower part of glands in the corpus and pylorus. In the glandular epithelium of the stomach, Lrig1 marks a heterogeneous population comprising mainly non-proliferative cells. Yet, fate-mapping experiments using a knock-in mouse line expressing Cre specifically in Lrig1+ cells demonstrate that these cells are able to contribute to the long-term maintenance of the gastric epithelium. Moreover, when cultured in vitro, cells expressing high level of Lrig1 have much higher organoid forming potential than the corresponding cellular populations expressing lower levels of Lrig1. Taken together, these observations show that Lrig1 is expressed primarily by differentiated cells, but that these cells can be recruited to contribute to the maintenance of the gastric epithelium. This confirms previous observations that cells located in the lower segments of gastric glands can participate in tissue replenishment.

Published

2018

38. From Definitive Endoderm to Gut—a Process of Growth and Maturation

Author

Jordi Guiu and Kim B. Jensen

Subjects

Mesoderm, Cell signaling, Cellular differentiation, Morphogenesis, Biology, Inflammatory bowel disease, medicine, Animals, Humans, Intestinal Mucosa, Endoderm, Gastrulation, Cell Differentiation, Cell Biology, Hematology, medicine.disease, Intestines, medicine.anatomical_structure, Immunology, Neuroscience, Developmental Biology, Definitive endoderm

Abstract

The intestine and colon carries out vital functions, and their lifelong maintenance is of the upmost importance. Research over the past decades has carefully addressed bowel function, how it is maintained and begun to unravel how disorders such as cancer and inflammatory bowel disease form. In contrast, very little is known about the molecular mechanisms that trigger tissue maturation during development. With this review, our aim is to carefully provide a critical appraisal of the literature to give a state-of-the-art view of intestinal development. Starting from definitive endoderm at gastrulation to the emergence of a structure with mature properties, the tissue undergoes complex morphogenetic processes that rely on both biophysical changes and secreted signaling molecules. We will also discuss how new and exciting developments using in vitro models are likely to provide new insights into this process and potential therapeutic strategies for gastrointestinal disorders.

Published

2015

39. YAP/TAZ-Dependent Reprogramming of Colonic Epithelium Links ECM Remodeling to Tissue Regeneration

Author

Jens Vilstrup Johansen, Pawel J. Schweiger, Stine Lund Hansen, Robert P. Fordham, Ole Haagen Nielsen, Chris D. Madsen, Mariana R. P. Alves, Shiro Yui, Hjalte List Larsen, Marianne Terndrup Pedersen, Tetsuya Nakamura, Luca Azzolin, Stefano Piccolo, Mamoru Watanabe, Jordi Guiu, Kim B. Jensen, Yuan Li, Martti Maimets, Carsten Friis Rundsten, Maimets, Martti [0000-0001-7343-2769], Pedersen, Marianne Terndrup [0000-0003-3808-0352], Hansen, Stine L [0000-0002-5967-286X], Guiu, Jordi [0000-0003-0297-2543], Alves, Mariana RP [0000-0002-0796-2101], Madsen, Chris D [0000-0001-6838-2103], Nielsen, Ole H [0000-0003-4612-8635], Jensen, Kim B [0000-0001-6569-1664], and Apollo - University of Cambridge Repository

Subjects

Transcriptional Activation, 0301 basic medicine, Transcription, Genetic, Cellular differentiation, Cell Cycle Proteins, Biology, Cell fate determination, Mechanotransduction, Cellular, mechano-sensing, Extracellular matrix, 03 medical and health sciences, intestinal stem cells, regeneration, reprogramming, YAP/TAZ, Molecular Medicine, Genetics, Cell Biology, Fetus, medicine, Animals, Humans, Regeneration, Intestinal Mucosa, Mechano-sensing, Adaptor Proteins, Signal Transducing, Regeneration (biology), Intestinal stem cells, Wnt signaling pathway, YAP-Signaling Proteins, Reprogramming, Cellular Reprogramming, Phosphoproteins, Epithelium, Extracellular Matrix, Cell biology, Mice, Inbred C57BL, 030104 developmental biology, medicine.anatomical_structure, Cell culture, Biomarkers, Signal Transduction

Abstract

Tissue regeneration requires dynamic cellular adaptation to the wound environment. It is currently unclear how this is orchestrated at the cellular level and how cell fate is affected by severe tissue damage. Here we dissect cell fate transitions during colonic regeneration in a mouse dextran sulfate sodium (DSS) colitis model, and we demonstrate that the epithelium is transiently reprogrammed into a primitive state. This is characterized by de novo expression of fetal markers as well as suppression of markers for adult stem and differentiated cells. The fate change is orchestrated by remodeling the extracellular matrix (ECM), increased FAK/Src signaling, and ultimately YAP/TAZ activation. In a defined cell culture system recapitulating the extracellular matrix remodeling observed in vivo, we show that a collagen 3D matrix supplemented with Wnt ligands is sufficient to sustain endogenous YAP/TAZ and induce conversion of cell fate. This provides a simple model for tissue regeneration, implicating cellular reprogramming as an essential element. The mechanism that governs tissue regeneration following severe damage to the colonic epithelium remains poorly understood. Jensen and colleagues show that the colonic epithelium undergoes a profound reprogramming into a more primitive state with fetal-like properties. Moreover, they demonstrate that YAP and TAZ operate as essential mechano-sensors during tissue reprogramming.

Published

2018

40. Characterization of the enhancer and promoter landscape of inflammatory bowel disease from human colon biopsies

Author

Katja Dahlgaard, Nicolas Rapin, Mette Boyd, Jacob Tveiten Bjerrum, Bobby Lo, Yuan Li, Pawel J. Schweiger, Pia Klausen, Andreas Petersen, Morana Vitezic, Albin Sandelin, Kristoffer Vitting-Seerup, Jesper T. Troelsen, Robin Andersson, Berit Lilje, Peter Thielsen, Yun Chen, Jakob Benedict Seidelin, Malte Thodberg, Thilde Terkelsen, Kerstin Skovgaard, Ole Haagen Nielsen, Mehmet Coşkun, Jette Bornholdt, Kim B. Jensen, Ismail Gögenur, and Anders Gorm Pedersen

Subjects

Adult, Male, 0301 basic medicine, Colon, Biopsy, Science, General Physics and Astronomy, Regulatory Sequences, Nucleic Acid, Biology, Polymorphism, Single Nucleotide, Inflammatory bowel disease, digestive system, Article, General Biochemistry, Genetics and Molecular Biology, Descending colon, Cohort Studies, 03 medical and health sciences, 0302 clinical medicine, Crohn Disease, Intestinal mucosa, SDG 3 - Good Health and Well-being, medicine, Humans, Intestinal Mucosa, lcsh:Science, Enhancer, Regulation of gene expression, Multidisciplinary, Sequence Analysis, RNA, Molecular pathology, Promoter, Colonoscopy, General Chemistry, Middle Aged, medicine.disease, Ulcerative colitis, digestive system diseases, Up-Regulation, 3. Good health, 030104 developmental biology, medicine.anatomical_structure, Case-Control Studies, Cancer research, lcsh:Q, Colitis, Ulcerative, Female, 030211 gastroenterology & hepatology

Abstract

Inflammatory bowel disease (IBD) is a chronic intestinal disorder, with two main types: Crohn’s disease (CD) and ulcerative colitis (UC), whose molecular pathology is not well understood. The majority of IBD-associated SNPs are located in non-coding regions and are hard to characterize since regulatory regions in IBD are not known. Here we profile transcription start sites (TSSs) and enhancers in the descending colon of 94 IBD patients and controls. IBD-upregulated promoters and enhancers are highly enriched for IBD-associated SNPs and are bound by the same transcription factors. IBD-specific TSSs are associated to genes with roles in both inflammatory cascades and gut epithelia while TSSs distinguishing UC and CD are associated to gut epithelia functions. We find that as few as 35 TSSs can distinguish active CD, UC, and controls with 85% accuracy in an independent cohort. Our data constitute a foundation for understanding the molecular pathology, gene regulation, and genetics of IBD., Many SNPs associated with inflammatory bowel disease are located in non-coding genomic regions. Here, the authors perform CAGE-sequencing on descending colon biopsies of Crohn’s disease and ulcerative colitis patients to map transcription start sites and enhancer activity for analysis of regulatory regions.

Published

2018

41. A genetically inducible porcine model of intestinal cancer

Author

Mai-Britt Worm Ørntoft, Martin F. Berthelsen, Kim B. Jensen, Claus L. Andersen, Søren Laurberg, Torben F. Ørntoft, Ying Liu, Martin K. Thomsen, Frederik Dagnæs-Hansen, Rong Li, Henrik Callesen, Søren Høyer, Morten M. Callesen, Iben Lyskjær, Pawel J. Schweiger, Mads Rasmussen, Jannik Ejnar Elverløv-Jakobsen, and Sigrid S. Árnadóttir

Subjects

0301 basic medicine, Cancer Research, Nuclear Transfer Techniques, Swine, Transgene, Cloning, Organism, Biology, Metastasis, Animals, Genetically Modified, Embryo Culture Techniques, 03 medical and health sciences, 0302 clinical medicine, transgenic porcine model, In vivo, Intestinal Neoplasms, Genetics, medicine, Carcinoma, Animals, Humans, Intestinal Mucosa, Research Articles, tissue‐specific activation, Oncogene, General Medicine, medicine.disease, Embryo Transfer, idducible intestinal cancer, tissue-specific activation, Molecular biology, In vitro, Intestines, Disease Models, Animal, 030104 developmental biology, Oncology, 030220 oncology & carcinogenesis, Molecular Medicine, Swine, Miniature, oncopig, Female, inducible intestinal cancer, Tamoxifen, Ex vivo, Inducible intestinal cancer, medicine.drug, Research Article

Abstract

Transgenic porcine cancer models bring novel possibilities for research. Their physical similarities with humans enable the use of surgical procedures and treatment approaches used for patients, which facilitates clinical translation. Here, we aimed to develop an inducible oncopig model of intestinal cancer. Transgenic (TG) minipigs were generated using somatic cell nuclear transfer by handmade cloning. The pigs encode two TG cassettes: (a) an Flp recombinase-inducible oncogene cassette containing KRAS-G12D, cMYC, SV40LT - which inhibits p53 - and pRB and (b) a 4-hydroxytamoxifen (4-OHT)-inducible Flp recombinase activator cassette controlled by the intestinal epithelium-specific villin promoter. Thirteen viable transgenic minipigs were born. The ability of 4-OHT to activate the oncogene cassette was confirmed in vitro in TG colonic organoids and ex vivo in tissue biopsies obtained by colonoscopy. In order to provide proof of principle that the oncogene cassette could also successfully be activated in vivo, three pigs were perorally treated with 400 mg tamoxifen for 2 × 5 days. After two months, one pig developed a duodenal neuroendocrine carcinoma with a lymph node metastasis. Molecular analysis of the carcinoma and metastasis confirmed activation of the oncogene cassette. No tumor formation was observed in untreated TG pigs or in the remaining two treated pigs. The latter indicates that tamoxifen delivery can probably be improved. In summary, we have generated a novel inducible oncopig model of intestinal cancer, which has the ability to form metastatic disease already two months after induction. The model may be helpful in bridging the gap between basic research and clinical usage. It opens new venues for longitudinal studies of tumor development and evolution, for preclinical assessment of new anticancer regimens, for pharmacology and toxicology assessments, as well as for studies into biological mechanisms of tumor formation and metastasis.

Published

2017

42. IL-17R-EGFR axis links wound healing to tumorigenesis in Lrig1

Author

Xing, Chen, Gang, Cai, Caini, Liu, Junjie, Zhao, Chunfang, Gu, Ling, Wu, Thomas A, Hamilton, Cun-Jin, Zhang, Jennifer, Ko, Liang, Zhu, Jun, Qin, Allison, Vidimos, Shlomo, Koyfman, Brian R, Gastman, Kim B, Jensen, and Xiaoxia, Li

Subjects

Mice, Knockout, Wound Healing, Membrane Glycoproteins, Receptors, Interleukin-17, Carcinogenesis, Stem Cells, Nerve Tissue Proteins, Article, CSK Tyrosine-Protein Kinase, ErbB Receptors, Mice, src-Family Kinases, Animals, Humans, Epidermis, Research Articles, Adaptor Proteins, Signal Transducing, HeLa Cells, Signal Transduction

Abstract

This study provides mechanistic insight into how IL-17 receptor adopts EGFR to activate ERK5 axis in Lrig1+ stem cells for their proliferation and migration during wounding healing and tumorigenesis., Lrig1 marks a distinct population of stem cells restricted to the upper pilosebaceous unit in normal epidermis. Here we report that IL-17A–mediated activation of EGFR plays a critical role in the expansion and migration of Lrig1+ stem cells and their progenies in response to wounding, thereby promoting wound healing and skin tumorigenesis. Lrig1-specific deletion of the IL-17R adaptor Act1 or EGFR in mice impairs wound healing and reduces tumor formation. Mechanistically, IL-17R recruits EGFR for IL-17A–mediated signaling in Lrig1+ stem cells. While TRAF4, enriched in Lrig1+ stem cells, tethers IL-17RA and EGFR, Act1 recruits c-Src for IL-17A–induced EGFR transactivation and downstream activation of ERK5, which promotes the expansion and migration of Lrig1+ stem cells. This study demonstrates that IL-17A activates the IL-17R–EGFR axis in Lrig1+ stem cells linking wound healing to tumorigenesis.

Published

2017

43. Reconstruction of the mouse extrahepatic biliary tree using primary human extrahepatic cholangiocyte organoids

Author

Kim B. Jensen, Nicholas R.F. Hannan, Johannes Bargehr, Olivia C. Tysoe, William Gelson, Ludovic Vallier, Edmund Godfrey, María J Gómez-Vázquez, Susan E. Davies, Sanjay Sinha, Negar Pirmadjid, Casey A. Rimland, Mariëlle C. F. Zonneveld, Marianne Terndrup Pedersen, Kirsten E. Snijders, Athina E. Markaki, N.L. Berntsen, Ingrid Simonic, Kourosh Saeb-Parsy, Laura Valestrand, Nikitas Georgakopoulos, Stephanie Brown, Richard L. Gieseck, Thomas A. Wynn, Pedro Madrigal, Graeme J.M. Alexander, Daniel Ortmann, Matthias Zilbauer, Fotios Sampaziotis, Alessandro Bertero, Tom H. Karlsen, Miguel Cardoso de Brito, Stephen J. Sawiak, Wenmiao Shu, Sara Upponi, Paulina M. Materek, Alexander W. Justin, Espen Melum, Alexander Ross, Loukia Yiangou, Matthias Pawlowski, Gregor Skeldon, and John Casey

Subjects

0301 basic medicine, Pathology, medicine.medical_specialty, Cell Transplantation, Cystic Fibrosis Transmembrane Conductance Regulator, In Vitro Techniques, Regenerative medicine, General Biochemistry, Genetics and Molecular Biology, Cholangiocyte, 03 medical and health sciences, Mice, Cholestasis, Secretin, Biliary atresia, Bile Ducts, Extrahepatic, TA164, medicine, Journal Article, Animals, Humans, Regeneration, Video-Audio Media, Biliary Tract, Keratin-19, Common bile duct, Tissue Engineering, Tissue Scaffolds, business.industry, Gallbladder, Keratin-7, Epithelial Cells, General Medicine, gamma-Glutamyltransferase, medicine.disease, Transplantation, Organoids, 030104 developmental biology, medicine.anatomical_structure, Biliary tract, business, Somatostatin

Abstract

The treatment of common bile duct (CBD) disorders, such as biliary atresia or ischemic strictures, is restricted by the lack of biliary tissue from healthy donors suitable for surgical reconstruction. Here we report a new method for the isolation and propagation of human cholangiocytes from the extrahepatic biliary tree in the form of extrahepatic cholangiocyte organoids (ECOs) for regenerative medicine applications. The resulting ECOs closely resemble primary cholangiocytes in terms of their transcriptomic profile and functional properties. We explore the regenerative potential of these organoids $\textit{in vivo}$ and demonstrate that ECOs self-organize into bile duct–like tubes expressing biliary markers following transplantation under the kidney capsule of immunocompromised mice. In addition, when seeded on biodegradable scaffolds, ECOs form tissue-like structures retaining biliary characteristics. The resulting bioengineered tissue can reconstruct the gallbladder wall and repair the biliary epithelium following transplantation into a mouse model of injury. Furthermore, bioengineered artificial ducts can replace the native CBD, with no evidence of cholestasis or occlusion of the lumen. In conclusion, ECOs can successfully reconstruct the biliary tree, providing proof of principle for organ regeneration using human primary cholangiocytes expanded $\textit{in vitro}$.

Published

2017

44. Heterogeneity and plasticity of epidermal stem cells

Author

Kim B. Jensen, Troels Schepeler, and Mahalia E. Page

Subjects

Tissue homeostasis, Epidermis (botany), Regeneration (biology), Stem Cells, Reviews, Plasticity, Biology, Epithelium, Cell biology, medicine.anatomical_structure, Cell Transformation, Neoplastic, Epidermal Cells, Immunology, medicine, Regeneration, Homeostasis, Humans, Stem cell, Epidermis, Molecular Biology, Hair Follicle, Function (biology), Developmental Biology

Abstract

The epidermis is an integral part of our largest organ, the skin, and protects us against the hostile environment. It is a highly dynamic tissue that, during normal steady-state conditions, undergoes constant turnover. Multiple stem cell populations residing in autonomously maintained compartments facilitate this task. In this Review, we discuss stem cell behaviour during normal tissue homeostasis, regeneration and disease within the pilosebaceous unit, an integral structure of the epidermis that is responsible for hair growth and lubrication of the epithelium. We provide an up-to-date view of the pilosebaceous unit, encompassing the heterogeneity and plasticity of multiple discrete stem cell populations that are strongly influenced by external cues to maintain their identity and function.

Published

2014

45. Fondation René Touraine

Author

Cédric Blanpain, Marcella del Rio, Fiona M. Watt, Selim Aractingi, Viljar Jaks, Katsuto Tamai, Geoges Cotsarellis, Ian Chambers, and Kim B. Jensen

Subjects

business.industry, Medicine, Dermatology, business, Molecular Biology, Biochemistry

Published

2013

46. Isolation and In Vitro Characterization of Epidermal Stem Cells

Author

Kasper S, Moestrup, Marianne S, Andersen, and Kim B, Jensen

Subjects

Keratinocytes, Stem Cells, Fluorescent Antibody Technique, Cell Differentiation, Cell Separation, Fibroblasts, Coculture Techniques, Cell Line, Immunophenotyping, Colony-Forming Units Assay, Mice, Phenotype, Epidermal Cells, Microscopy, Fluorescence, Animals, Epidermis, Biomarkers

Abstract

Colony-forming assays represent prospective methods, where cells isolated from enzymatically dissociated tissues or from tissue cultures are assessed for their proliferative capacity in vitro. Complex tissues such as the epithelial component of the skin (the epidermis) are characterized by a substantial cellular heterogeneity. Analysis of bulk populations of cells by colony-forming assays can consequently be convoluted by a number of factors that are not controlled for in population wide studies. It is therefore advantageous to refine in vitro growth assays by sub-fractionation of cells using flow cytometry. Using markers that define the spatial origin of epidermal cells, it is possible to interrogate the specific characteristics of subpopulations of cells based on their in vivo credentials. Here, we describe how to isolate, culture, and characterize keratinocytes from murine back and tail skin sorted by surface antigens associated with adult stem cell characteristics.

Published

2017

47. Intestinal barrier integrity and inflammatory bowel disease: Stem cell-based approaches to regenerate the barrier

Author

Jannie Pedersen, Kim B. Jensen, Peter L. Jørgensen, Fredrik Eo Holmberg, Christoffer Soendergaard, and Ole Haagen Nielsen

Subjects

0301 basic medicine, Pluripotent Stem Cells, Tight junction, Biomedical Engineering, Medicine (miscellaneous), Biology, medicine.disease, Inflammatory Bowel Diseases, Inflammatory bowel disease, Biomaterials, Pathogenesis, Transplantation, 03 medical and health sciences, 030104 developmental biology, Directed differentiation, Immunology, medicine, Animals, Humans, Stem cell, Intestinal Mucosa, Induced pluripotent stem cell, Barrier function, Stem Cell Transplantation

Abstract

Disruption of normal barrier function is a fundamental factor in the pathogenesis of inflammatory bowel disease, which includes increased epithelial cell death, modified mucus configuration, altered expression and distribution of tight junction proteins, along with a decreased expression of antimicrobial peptides. Inflammatory bowel disease is associated with life-long morbidity for affected patients, and both the incidence and prevalence is increasing globally, resulting in substantial economic strain for society. Mucosal healing and re-establishment of barrier integrity are associated with clinical remission, as well as with an improved patient outcome. Hence, these factors are vital treatment goals, which conventionally are achieved by a range of medical treatments, although none are effective in all patients, resulting in several patients still requiring surgery at some point. Therefore, novel treatment strategies to accomplish mucosal healing and to re-establish normal barrier integrity in inflammatory bowel disease are warranted, and luminal stem cell-based approaches might have an intriguing potential. Transplantation of in vitro expanded intestinal epithelial stem cells derived either directly from mucosal biopsies or from directed differentiation of human pluripotent stem cells may constitute complementary treatment options for patients with mucosal damage, as intestinal epithelial stem cells are multipotent and may give rise to all epithelial cell types of the intestine. This review provides the reader with a comprehensive state-of-the-art overview of the intestinal barrier's role in healthy and diseased states, discussing the clinical application of stem cell-based approaches to accomplish mucosal healing in inflammatory bowel disease.

Published

2017

48. Isolation and In Vitro Characterization of Epidermal Stem Cells

Author

Kim B. Jensen, Marianne S. Andersen, and Kasper S. Moestrup

Subjects

0301 basic medicine, education.field_of_study, Epidermis (botany), medicine.diagnostic_test, Population, Biology, In vitro, Cell biology, Flow cytometry, 03 medical and health sciences, Tissue culture, 030104 developmental biology, medicine.anatomical_structure, medicine, Stem cell, Keratinocyte, education, Adult stem cell

Abstract

Colony-forming assays represent prospective methods, where cells isolated from enzymatically dissociated tissues or from tissue cultures are assessed for their proliferative capacity in vitro. Complex tissues such as the epithelial component of the skin (the epidermis) are characterized by a substantial cellular heterogeneity. Analysis of bulk populations of cells by colony-forming assays can consequently be convoluted by a number of factors that are not controlled for in population wide studies. It is therefore advantageous to refine in vitro growth assays by sub-fractionation of cells using flow cytometry. Using markers that define the spatial origin of epidermal cells, it is possible to interrogate the specific characteristics of subpopulations of cells based on their in vivo credentials. Here, we describe how to isolate, culture, and characterize keratinocytes from murine back and tail skin sorted by surface antigens associated with adult stem cell characteristics.

Published

2017

49. Replacement of the murine common bile duct with a bioengineered conduit incorporating primary human cholangiocyte organoids

Author

William Gelson, Olivia C. Tysoe, Casey A. Rimland, F. Sampaziotis, Stephen J. Sawiak, N. Pirmadjid, N.L. Berntsen, Stephanie Brown, Richard L. Gieseck, Kim B. Jensen, Paulina M. Materek, Alexander W. Justin, Tom H. Karlsen, M.C. de Brito, Daniel Ortmann, Nikitas Georgakopoulos, Marianne Terndrup Pedersen, Ludovic Vallier, Athina E. Markaki, Mariëlle C. F. Zonneveld, Alessandro Bertero, Kirsten E. Snijders, Ingrid Simonic, Sanjay Sinha, Graeme J.M. Alexander, Espen Melum, Thomas A. Wynn, Wenmiao Shu, Nicholas R.F. Hannan, Johannes Bargehr, Susan E. Davies, Kourosh Saeb-Parsy, Loukia Yiangou, Matthias Pawlowski, Edmund Godfrey, M.J. Gomez-Vazquez, and Gregor Skeldon

Subjects

Pathology, medicine.medical_specialty, medicine.anatomical_structure, Electrical conduit, Hepatology, Common bile duct, business.industry, medicine, Organoid, business, Cholangiocyte

Published

2017

50. Bimodal skin progenitors-a matter of place and time

Author

Kim B. Jensen and Svetlana Ulyanchenko

Subjects

0301 basic medicine, Interfollicular epidermis, General Immunology and Microbiology, integumentary system, General Neuroscience, Growth phase, Stem Cells, Anatomy, Articles, Biology, General Biochemistry, Genetics and Molecular Biology, Epithelium, Cell biology, 03 medical and health sciences, 030104 developmental biology, medicine.anatomical_structure, medicine, Humans, Progenitor cell, Molecular Biology, Skin

Abstract

Interfollicular epidermal (IFE) homeostasis is a major physiological process allowing maintenance of the skin barrier function. Despite progress in our understanding of stem cell populations in different hair follicle compartments, cellular mechanisms of IFE maintenance, in particular, whether a hierarchy of progenitors exists within this compartment, have remained controversial. We here used multicolour lineage tracing with Brainbow transgenic labels activated in the epidermis to track individual keratinocyte clones. Two modes of clonal progression could be observed in the adult murine dorsal skin. Clones attached to hair follicles showed rapid increase in size during the growth phase of the hair cycle. On the other hand, clones distant from hair follicles were slow cycling, but could be mobilized by a proliferative stimulus. Reinforced by mathematical modelling, these data support a model where progenitor cycling characteristics are differentially regulated in areas surrounding or away from growing hair follicles. Thus, while IFE progenitors follow a non‐hierarchical mode of development, spatiotemporal control by their environment can change their potentialities, with far‐reaching implications for epidermal homeostasis, wound repair and cancer development.

Published

2016