Your search keyword '"KERATINOCYTE differentiation"' showing total 2,988 results

1. Cell damage shifts the microRNA content of small extracellular vesicles into a Toll-like receptor 7-activating cargo capable to propagate inflammation and immunity.

Author

Salvi, Valentina, Gaudenzi, Carolina, Mariotti, Barbara, Giongrandi, Gaia, Alacqua, Silvia, Gianello, Veronica, Schioppa, Tiziana, Tiberio, Laura, Ceribelli, Angela, Selmi, Carlo, Bergese, Paolo, Calza, Stefano, Del Prete, Annalisa, Sozzani, Silvano, Bazzoni, Flavia, and Bosisio, Daniela

Subjects

*TYPE I interferons, *GENE expression, *TOLL-like receptors, *EXTRACELLULAR vesicles, *DENDRITIC cells, *T cells, KERATINOCYTE differentiation

Abstract

Background: The physiological relevance of cell-to-cell communication mediated by small extracellular vesicle-encapsulated microRNAs (sEV-miRNAs) remains debated because of the limiting representativity of specific miRNAs within the extracellular pool. We hypothesize that sEV-miRNA non-canonical function consisting of the stimulation of Toll-like receptor 7 (TLR7) may rely on a global shift of the sEV cargo rather than on the induction of one or few specific miRNAs. Psoriasis represents an ideal model to test such hypothesis as it is driven by overt activation of TLR7-expressing plasmacytoid dendritic cells (pDCs) following keratinocyte damage. Methods: To mimic the onset of psoriasis, keratinocytes were treated with a cocktail of psoriatic cytokines or UV-irradiated. SmallRNA sequencing was performed on sEVs released by healthy and UV-treated keratinocytes. sEV-miRNAs were analyzed for nucleotide composition as well as for the presence of putative TLR7-binding triplets. Primary human pDCs where stimulated with sEVs +/- inhibitors of TLR7 (Enpatoran), of sEV release (GW4869 + manumycin) and of TLR7-mediated pDC activation (anti-BDCA-2 antibody). Secretion of type I IFNs and activation of CD8+T cells were used as readouts. qPCR on psoriatic and healthy skin biopsies was conducted to identify induced miRNAs. Results: sEV-miRNAs released by damaged keratinocytes revealed a significantly higher content of TLR7-activating sequences than healthy cells. As expected, differential expression analysis confirmed the presence of miRNAs upregulated in psoriatic skin, including miR203a. More importantly, 76.5% of induced miRNAs possessed TLR7-binding features and among these we could detect several previously demonstrated TLR7 ligands. In accordance with this in silico analysis, sEVs from damaged keratinocytes recapitulated key events of psoriatic pathogenesis by triggering pDCs to release type I interferon and activate cytotoxic CD8+T cells in a TLR7- and sEV-dependent manner. Discussion: Our results demonstrate that miR203a is just one paradigmatic TLR7-activating miRNA among the hundreds released by UV-irradiated keratinocytes, which altogether trigger pDC activation in psoriatic conditions. This represents the first evidence that cell damage shifts the miRNA content of sEVs towards a TLR7-activating cargo capable to propagate inflammation and immunity, offering strong support to the physiological role of systemic miRNA-based cell-to-cell communication. [ABSTRACT FROM AUTHOR]

Published

2024

2. Advancing skin model development: A focus on a self-assembled, induced pluripotent stem cell-derived, xeno-free approach.

Author

Dubau, Marla, Tripetchr, Tarada, Mahmoud, Lava, Kral, Vivian, and Kleuser, Burkhard

Subjects

*INDUCED pluripotent stem cells, *FIBROBLASTS, *ANIMAL experimentation, *KERATINOCYTES, *COLLAGEN, *PLURIPOTENT stem cells, KERATINOCYTE differentiation

Abstract

The demand for skin models as alternatives to animal testing has grown due to ethical concerns and the need for accurate substance evaluation. These alternatives, known as New Approach Methodologies (NAMs), are increasingly used for regulatory decisions. Current skin models from primary human cells often rely on bovine collagen, raising ethical issues. This study explores self-assembled skin models (SASM) as a new method, utilizing hair follicle-derived keratinocytes reprogrammed into induced pluripotent stem cells (iPSC) and differentiated into fibroblasts and keratinocytes. The model relies on the ability of fibroblasts to secrete collagen to produce a xeno-free dermal layer and on the differentiation of keratinocytes to create a functional epidermal layer. These layers exhibited confirmed metabolic activity and the capability to withstand test substances. The successful development of SASM underscores the significance of accurate alternatives in dermatological research, providing an ethical and reliable option for substance evaluation and regulatory testing. [ABSTRACT FROM AUTHOR]

Published

2024

3. A shorter splicing isoform antagonizes ZBP1 to modulate cell death and inflammatory responses.

Author

Nagata, Masahiro, Carvalho Schäfer, Yasmin, Wachsmuth, Laurens, and Pasparakis, Manolis

Subjects

*SKIN inflammation, *CELL death, *LIGANDS (Biochemistry), *INTERFERONS, *INFLAMMATION, KERATINOCYTE differentiation

Abstract

Z-DNA-binding protein 1 (ZBP1) is an interferon-inducible sensor of Z-DNA and Z-RNA, which has emerged as a critical regulator of cell death and inflammation. ZBP1 binds Z-DNA and Z-RNA via its Zα domains, and signals by engaging RIPK3 and RIPK1 via its RIP homotypic interaction motifs (RHIMs). Here, we show that mice express an alternatively-spliced shorter ZBP1 isoform (ZBP1-S), which harbours the Zα domains but lacks the RHIMs, and acts as an endogenous inhibitor of the full-length protein (ZBP1-L). Mice and cells expressing only ZBP1-S are resistant to ZBP1-mediated cell death and inflammation. In contrast, cells lacking ZBP1-S show increased ZBP1-L-induced death compared to cells expressing both isoforms. Moreover, loss of the short isoform accelerates and exacerbates skin inflammation induced by ZBP1-mediated necroptosis of RIPK1-deficient keratinocytes, revealing an important physiological role of ZBP1-S. Mechanistically, ZBP1-S suppresses ZBP1-L-mediated cell death by binding to Z-nucleic acids via its Zα domains. Therefore, ZBP1-S acts as an endogenous inhibitor that competes with full-length ZBP1-L for binding Z-nucleic acid ligands to fine-tune ZBP1-mediated cell death and inflammation. Synopsis: Mice express full-length protein ZBP1-L as well as an alternatively-spliced shorter isoform (ZBP1-S) containing only its two Zα domains but lacking the three RHIM motifs. This study shows that ZBP1-S acts as an endogenous inhibitor that suppresses activation of ZBP1-L-mediated necroptosis and inflammation by endogenous Z-RNA ligands. Both ZBP1-S and ZBP1-L are induced by interferons and interact with endogenous Z-RNAs via their Zα domains. ZBP1-S suppresses ZBP1-L activation in a Zα domain-dependent manner. Loss of ZBP1-S results in increased ZBP1-L-mediated cell death. Specific ablation of ZBP1-S causes exaggerated ZBP1-L-induced necroptosis and inflammation in mice lacking RIPK1 in keratinocytes. Interferons induce a ZBP1-S isoform that competitively interacts with endogenous Z-RNAs and thereby suppresses ZBP1-induced necroptosis and inflammation. [ABSTRACT FROM AUTHOR]

Published

2024

4. Streptococcus canis transcriptomic modifications in host cell entry environments of human keratinocytes.

Author

Yoshida, Haruno, Goto, Mieko, Tsuyuki, Yuzo, Kim, Jae-Seok, and Takahashi, Takashi

Subjects

*GENE expression, *AMINO acid transport, *WHOLE genome sequencing, *LATENT infection, *AMINO acid metabolism, KERATINOCYTE differentiation

Abstract

Background: Streptococcus canis is a commensal bacterium in companion animals. This microorganism can infect humans who have been in deep contact with or bitten by pet dogs, suggesting that the skin/soft tissue is one of infection entry sites. To understand pathological process in human cells, we aimed to determine S. canis transcriptomic changes in invasive environments of human keratinocytes. Methods: We selected one isolate from candidates with whole-genome sequences, based on re-obtained cell invasion ability (CIA) data into human keratinocytes along with bacterial cytotoxicity. RNA-sequencing was conducted for the samples at baselines and 2 h/5 hr post-inoculation using NovaSeq 6000. Global/differential gene expression analyses [principal component analysis (PCA)/k-means clustering analysis/differentially expressed gene (DEG) analyses] were performed. We classified DEGs into their functional categories. To validate transcriptomic results, we did quantitative reverse transcription-polymerase chain reaction (qRT-PCR) assays. Results: FU1 isolate was selected from seven candidates, based on re-obtained CIA data with less cytotoxicity. Total read bases of 6.17–9.02 Gbp were obtained by RNA-sequencing. PCA and k-means clustering analysis indicated clustering according to their inoculation times. Volcano plots and Venn diagrams revealed that S. canis invasion into keratinocytes produced altered distributions of many genes. Gene ontology enrichment analysis showed most of the gene expressions were downregulated. DEG functional analysis showed the downregulated DEGs belonging to energy production and conversion/carbohydrate transport and metabolism/amino acid transport and metabolism/nucleotide transport and metabolism, with the upregulated DEGs belonging to transcription. qRT-PCR assays for downregulated/upregulated expressions of four genes (pgk–slo/opuAA–kdpB) validated transcriptomic results. Conclusion: Our observations suggest that S. canis can downregulate its metabolism-associated gene expressions in human keratinocyte environments. The observed gene expression changes can imply the latent infection in human cells. Further investigation is needed to elucidate the underlying mechanisms for the latent infection. [ABSTRACT FROM AUTHOR]

Published

2024

5. Amelioration of Systemic Amyloidosis by Blocking IL-17A and Not by IL-17F, and Arteriosclerosis by Blocking Both IL-17A and IL-17F in an Inflammatory Skin Mouse Model.

Author

Nakanishi, Takehisa, Iida, Shohei, Ichishi, Masako, Kondo, Makoto, Nishimura, Mai, Ichikawa, Ayaka, Matsushima, Yoshiaki, Iwakura, Yoichiro, Watanabe, Masatoshi, and Yamanaka, Keiichi

Subjects

*SKIN inflammation, *ATOPIC dermatitis, *CEREBRAL infarction, *MYOCARDIAL infarction, *INFLAMMATION, KERATINOCYTE differentiation

Abstract

There are comorbidities and complications in atopic dermatitis and psoriasis that often occur after the appearance of skin inflammation. Statistically, data show that patients with psoriasis and atopic dermatitis have a shorter life expectancy than patients without psoriatic dermatitis, due to the occurrence of arteriosclerosis, myocardial infarction, and cerebral infarction. Many types of skin inflammation are treated with various antibody preparations, and marked improvement in patients' quality of life can be achieved. The next theme is to understand the pathogenesis of arteriosclerosis, myocardial infarction, stroke, and other complications associated with dermatitis and to find treatments and drugs to reduce their occurrence. The skin, a crucial immune organ, generates large amounts of inflammatory cytokines in response to various stimuli, leading to systemic inflammation and potential damage to internal organs. The link between inflammatory skin conditions like psoriasis and atopic dermatitis with serious health complications such as vascular disorders and systemic amyloidosis has been increasingly recognized. In psoriasis, biological treatments targeting Interleukin (IL)-17A, a key cytokine, have shown promise in reducing cardiovascular risks. Recent developments include treatments that target both IL-17A and IL-17F in the psoriasis field, though each cytokine's impact on internal organ damage is still under debate. Among visceral complications secondary to dermatitis, systemic amyloidosis and atherosclerosis have been reported to be controlled by suppressing IL-17 in the early stages of dermatitis. Still, it remains unclear whether suppressing IL-17 prevents organ damage in the late stages of persistent severe dermatitis. A study using a long-lasting dermatitis mouse model that overexpressed human caspase-1 in keratinocytes (Kcasp1Tg) investigated the effects of deleting IL-17A and IL-17F on visceral complications. Cross-mating Kcasp1Tg with IL-17A-, IL-17F-, and IL-17AF-deficient mice assessed the skin and visceral organs histologically, and RT-PCR analysis of aortic sclerosis markers was performed. Despite less improvement in dermatitis, deletion of IL-17A in Kcasp1Tg mice showed promising results in reducing multiple organ amyloidosis. On the other hand, the effect was observed in both IL-17A and IL-17F deleted mice for aortic sclerosis. The inhibition of IL-17A and IL-17F was suggested to reduce the risk of developing comorbidities in internal organs. IL-17A and IL-17F were found to act similarly or produce very different results, depending on the organ. [ABSTRACT FROM AUTHOR]

Published

2024

6. Knockdown of Keratin 6 Within Arsenite-Transformed Human Urothelial Cells Decreases Basal/Squamous Expression, Inhibits Growth, and Increases Cisplatin Sensitivity.

Author

Nargis, Nelofar, Sens, Donald A., and Mehus, Aaron A.

Subjects

*POISONS, *CISPLATIN, *TRANSITIONAL cell carcinoma, *PROTEIN expression, *DRINKING water, KERATINOCYTE differentiation

Abstract

Urothelial carcinoma (UC) is prevalent, especially in elderly males. The high rate of recurrence, treatment regime, and follow-up monitoring make UC a global health and economic burden. Arsenic is a ubiquitous toxicant that can be found in drinking water, and it is known that exposure to arsenic is associated with UC development. Around 25% of diagnosed UC cases are muscle-invasive (MIUC) which have poor prognosis and develop chemoresistance, especially if tumors are associated with squamous differentiation (SD). The immortalized UROtsa cell line is derived from normal human urothelium and our lab has malignantly transformed these cells using arsenite (As3+). These cells represent a basal subtype model of MIUC and the tumors derived from the As3+-transformed cells histologically and molecularly resemble clinical cases of the basal subtype of MIUC that have focal areas SD and expression of the basal keratins (KRT1, 5, 6, 14, and 16). Our previous data demonstrate that KRT6 protein expression correlates to areas of SD within the tumors. For this study, we performed a lentiviral knockdown of KRT6 in As3+-transformed UROtsa cells to evaluate the effects on morphology, gene/protein expression, growth, colony formation, and cisplatin sensitivity. The knockdown of KRT6 resulted in decreased expression of the basal keratins, decreased growth, decreased colony formation, and increased sensitivity to cisplatin, the standard treatment for MIUC. The results of this study suggest that KRT6 plays a role in UC cell growth and is an exploitable target to increase cisplatin sensitivity for MIUC tumors that may have developed resistance to cisplatin treatment. [ABSTRACT FROM AUTHOR]

Published

2024

7. Foamed microemulsion nanodroplets loaded with chlorin e6 for epidermal-targeted treatment against psoriasis.

Author

Ma, Xiaolu, Bian, Qiong, Xu, Yihua, Hu, Jingyi, Hu, Weitong, Wang, Ruxuan, Zhang, Yunting, Ye, Yuxian, Sheng, Xiaoxia, Zhang, Tianyuan, and Gao, Jianqing

Subjects

TRANSDERMAL medication, PHOTODYNAMIC therapy, REACTIVE oxygen species, SKIN diseases, LABORATORY mice, KERATINOCYTE differentiation

Abstract

Psoriasis is a chronic skin disease characterized by the hyperproliferation of keratinocytes and an overactive autoimmune response. Photodynamic therapy (PDT) has been established as a promising intervention for alleviating psoriasis. However, the current transdermal delivery of photosensitizers is inefficient and imprecise. In this study, we developed a foamed microemulsion nanodroplets system containing chlorin e6 (Ce6 FM), exhibiting precise epidermal targeting and retention, which targeted the aberrantly proliferating epidermal cells at psoriatic skin lesions and avoided the damage to the normal cutaneous cells. Upon application in a psoriatic mouse model, Ce6 FM efficiently induced keratinocyte apoptosis by generating reactive oxygen species under laser. Furthermore, Ce6 FM-based PDT activated the cyclooxygenase-2-induced immunosuppressive pathway in keratinocytes, resulting in the amelioration of the autoimmune microenvironment in psoriatic skin. Additionally, Ce6 FM-based PDT did not induce skin damage or atrophy associated with non-targeted halometasone treatment. Overall, Ce6 FM-based PDT holds promise as an effective, safe and compliant strategy for psoriasis treatment. [ABSTRACT FROM AUTHOR]

Published

2024

8. Discovery of PANoptosis-related signatures correlates with immune cell infiltration in psoriasis.

Author

Wu, Li, Jiao, Xin-long, Jing, Ming, Zhang, Sheng-xiao, Wang, Yang, Li, Chen-long, Shi, Gao-xiang, Li, Zhuo-yang, Liu, Ge-liang, Yan, Kai, Yan, Li-xuan, Wang, Qi, He, Pei-feng, and Yu, Qi

Subjects

*CELL analysis, *CELL populations, *PLASMA cells, *IMMUNE checkpoint proteins, *REGULATORY T cells, KERATINOCYTE differentiation

Abstract

Psoriasis is an inflammatory skin disease that relapses frequently. Keratinocyte apoptosis dysregulation plays a crucial role in the pathological mechanisms of psoriasis. PANoptosis is a process with intermolecular interaction among pyroptosis, apoptosis, and necroptosis. The mechanism of PANoptosis in the occurrence and development of psoriasis is still unclear. Here we present a novel approach by identifying PANoptosis-related signatures (PANoptosis-sig) from skin tissue of psoriasis patients and healthy controls on transcriptional and protein levels. Five PANoptosis-sig (TYMP, S100A8, S100A9, NAMPT, LCN2) were identified. Enrichment analysis showed they were mainly enriched in response to leukocyte aggregation, leukocyte migration, chronic inflammatory response and IL−17 signaling pathway. Single cell transcriptome analysis showed TYMP and NAMPT were expressed in almost all cell populations, while LCN2, S100A8 and S100A9 were significantly highly expressed in keratinocyte. We then constructed predictive and diagnostic models with the PANoptosis-sig and evaluated their performance. Finally, unsupervised consensus clustering analysis was conducted to ascertain psoriasis molecular subtypes by the PANoptosis-sig. The psoriasis cohort was divided into two distinct subtypes. Immune landscape showed that the stromal score of cluster 1 was significantly higher than cluster 2, while the immune and estimate scores of cluster 2 were expressively higher than cluster 1. Cluster 1 exhibited high expression of Plasma cells, Tregs and Mast cells resting, while cluster 2 showed high expression of T cells, Macrophages M1, Dendritic cells activated, and Neutrophils in immune infiltration analysis. And cluster 2 was more sensitive to immune checkpoints. In conclusion, our findings revealed potential biomarkers and therapeutic targets for the prevention, diagnosis, and treatment of psoriasis, enhancing our understanding of the molecular mechanisms underlying PANoptosis. [ABSTRACT FROM AUTHOR]

Published

2024

9. Capsaicin attenuates the effect of inflammatory cytokines in a HaCaT cell model for basal keratinocytes.

Author

Cervantes Recalde, Maria Fernanda, Schmidt, Jana, Girardi, Cristina, Massironi, Marco, Rechl, Markus Leo, Hans, Joachim, Stuhlmann, Dominik, Somoza, Veronika, and Lieder, Barbara

Subjects

TIGHT junctions, SKIN permeability, CLAUDINS, TRPV cation channels, GENE expression, KERATINOCYTE differentiation

Abstract

Introduction: The resolution of the skin's inflammatory response is only possible if its barrier function is restored. TRPV1 channel activation plays an important role during inflammation but the effect of this activation on the skin barrier under inflammatory conditions has not been clarified. We hypothesize that it could potentially aid the keratinocyte barrier by reducing inflammatory cytokine release and promoting tight junction development. Methods: To explore the role of TRPV1 activation in inflammation, we designed and optimized an in vitro model of keratinocytes with basal epidermal layer characteristics using HaCaT cells and TNFα to induce inflammation. Results: TNFα increased the gene expression of tight junction protein claudin 1 (CLDN1) by at least 2.60 ± 0.16-fold, in a concentration-dependent manner, over a 48 h period. The administration of a capsaicin pre-treatment reduced the CLDN1 expression to 1.51 ± 0.16-fold during the first 6 h after TNFα induction, whereas IL-8 cytokine release was reduced 0.64 ± 0.17-fold. After 48 h, CLDN1 protein levels increased by a factor of 6.57 ± 1.39 compared to cells only treated with TNFα. Discussion: These results suggest that activation of TRPV1 by capsaicin can potentiate the increase in CLDN1 expression and CLDN1 protein synthesis induced by TNFα in cultured keratinocytes, while reducing the release of IL-8. [ABSTRACT FROM AUTHOR]

Published

2024

10. Non-electrophilic NRF2 activators promote wound healing in human keratinocytes and diabetic mice and demonstrate selective downstream gene targeting.

Author

Barakat, May, Han, Chen, Chen, Lin, David, Brian P., Shi, Junhe, Xu, Angela, Skowron, Kornelia J., Johnson, Tatum, Woods, Reginald A., Ankireddy, Aparna, Reddy, Sekhar P., Moore, Terry W., and DiPietro, Luisa A.

Subjects

*TRANSCRIPTION factors, *GENE targeting, *RNA sequencing, *NUCLEAR factor E2 related factor, *CELL migration, *WOUND healing, *SKIN regeneration, KERATINOCYTE differentiation

Abstract

The transcription factor NRF2 plays an important role in many biological processes and is a promising therapeutic target for many disease states. NRF2 is highly expressed in the skin and is known to play a critical role in diabetic wound healing, a serious disease process for which treatment options are limited. However, many existing NRF2 activators display off-target effects due to their electrophilic mechanism, underscoring the need for alternative approaches. In this work, we investigated two recently described non-electrophilic NRF2 activators, ADJ-310 and PRL-295, and demonstrated their efficacy in vitro and in vivo in human keratinocytes and Leprdb/db diabetic mice. We also compared the downstream targets of PRL-295 to those of the widely used electrophilic NRF2 activator CDDO-Me by RNA sequencing. Both ADJ-310 and PRL-295 maintained human keratinocyte cell viability at increasing concentrations and maintained or improved cell proliferation over time. Both compounds also increased cell migration, improving in vitro wound closure. ADJ-310 and PRL-295 enhanced the oxidative stress response in vitro, and RNA-sequencing data showed that PRL-295 activated NRF2 with a narrower transcriptomic effect than CDDO-Me. In vivo, both ADJ-310 and PRL-295 improved wound healing in Leprdb/db diabetic mice and upregulated known downstream NRF2 target genes in treated tissue. These results highlight the non-electrophilic compounds ADJ-310 and PRL-295 as effective, innovative tools for investigating the function of NRF2. These compounds directly address the need for alternative NRF2 activators and offer a new approach to studying the role of NRF2 in human disease and its potential as a therapeutic across multiple disease states. [ABSTRACT FROM AUTHOR]

Published

2024

11. FGF12 Positively Regulates Keratinocyte Proliferation by Stabilizing MDM2 and Inhibiting p53 Activity in Psoriasis.

Author

Wang, Nan, Xu, Xiejun, Guan, Fangqian, Lin, Yifan, Ye, Yizhou, Zhou, Jie, Feng, Jianjun, Li, Sihang, Ye, Junbo, Tang, Zhouhao, Gao, Wenjie, Sun, Bohao, Shen, Yingjie, Sun, Li, Song, Yonghuan, Jin, Litai, Li, Xiaokun, Cong, Weitao, and Zhu, Zhongxin

Subjects

*INHIBITION of cellular proliferation, *CELL communication, *RNA sequencing, *CELL cycle, *SKIN diseases, KERATINOCYTE differentiation

Abstract

Psoriasis is a chronic skin disease characterized by abnormal proliferation and inflammation of epidermal keratinocytes. Fibroblast growth factor 12 (FGF12) is implicated in the regulation of diverse cellular signals; however, its precise mechanism in psoriasis requires further investigation. In this study, high expression of FGF12 is observed in the epidermis of skin lesion in psoriasis patients and imiquimod (IMQ)‐induced psoriasis like‐dermatitis. Moreover, specific loss of FGF12 in keratinocytes in IMQ‐induced psoriasis model alleviates psoriasis‐like symptoms and reduces proliferation. In vitro RNA sequencing demonstrates that knockdown of FGF12 effectively arrests the cell cycle, inhibits cell proliferation, and predominantly regulates the p53 signaling pathway. Mechanistically, FGF12 is selectively bound to the RING domain of MDM2, thus partially inhibiting the binding of β‐Trcp to MDM2. This interaction inhibits β‐Trcp‐induced‐K48 ubiquitination degradation of MDM2, thereby suppressing the activity of the p53 signaling pathway, which results in excessive cell proliferation. Last, the alleviatory effect of FGF12 deficiency on psoriasis progression is reversed by p53 knockdown. In summary, these findings provide valuable insights into the mechanisms by which FGF12 suppresses p53 signaling in keratinocytes, exacerbating the development of psoriasis. This positive regulatory loop highlights the potential of FGF12 as a therapeutic target to manage psoriasis. [ABSTRACT FROM AUTHOR]

Published

2024

12. Liraglutide Promotes Diabetic Wound Healing via Myo1c/Dock5.

Author

Zhang, Qian, Zhang, Chunlin, Kang, Changjiang, Zhu, Jiaran, He, Qingshan, Li, Hongwei, Tong, Qiang, Wang, Min, Zhang, Linlin, Xiong, Xin, Wang, Yuren, Qu, Hua, Zheng, Hongting, and Zheng, Yi

Subjects

*CELL physiology, *KNOCKOUT mice, *WOUND healing, *EXTRACELLULAR matrix, *LIRAGLUTIDE, KERATINOCYTE differentiation

Abstract

Non‐healing diabetic wounds and ulcer complications, with persistent cell dysfunction and obstructed cellular processes, are leading causes of disability and death in patients with diabetes. Currently, there is a lack of guideline‐recommended hypoglycemic drugs in clinical practice, likely due to limited research and unclear mechanisms. In this study, it is demonstrated that liraglutide significantly accelerates wound closure in diabetic mouse models (db/db mice and streptozotocin‐induced mice) by improving re‐epithelialization, collagen deposition, and extracellular matrix remodeling, and enhancing the proliferation, migration, and adhesion functions of keratinocytes. However, these effects of improved healing by liraglutide are abrogated in dedicator of cytokinesis 5 (Dock5) keratinocyte‐specific knockout mice. Mechanistically, liraglutide induces cellular function through stabilization of unconventional myosin 1c (Myo1c). Liraglutide directly binds to Myo1c at arginine 93, enhancing the Myo1c/Dock5 interaction by targeting Dock5 promoter and thus promoting the proliferation, migration, and adhesion of keratinocytes. Therefore, this study provides insights into liraglutide biology and suggests it may be an effective treatment for diabetic patients with wound‐healing pathologies. [ABSTRACT FROM AUTHOR]

Published

2024

13. Shifts in keratin isoform expression activate motility signals during wound healing.

Author

Nanes, Benjamin A., Bhatt, Kushal, Azarova, Evgenia, Rajendran, Divya, Munawar, Sabahat, Isogai, Tadamoto, Dean, Kevin M., and Danuser, Gaudenz

Subjects

*INTERMEDIATE filament proteins, *CYTOPLASMIC filaments, *CELL motility, *CELL physiology, *EPITHELIUM, *WOUND healing, *WNT signal transduction, KERATINOCYTE differentiation

Abstract

Keratin intermediate filaments confer structural stability to epithelial tissues, but the reason this simple mechanical function requires a protein family with 54 isoforms is not understood. During skin wound healing, a shift in keratin isoform expression alters the composition of keratin filaments. If and how this change modulates cellular functions that support epidermal remodeling remains unclear. We report an unexpected effect of keratin isoform variation on kinase signal transduction. Increased expression of wound-associated keratin 6A, but not of steady-state keratin 5, potentiated keratinocyte migration and wound closure without compromising mechanical stability by activating myosin motors to increase contractile force generation. These results substantially expand the functional repertoire of intermediate filaments from their canonical role as mechanical scaffolds to include roles as isoform-tuned signaling scaffolds that organize signal transduction cascades in space and time to influence epithelial cell state. [Display omitted] • During skin wound healing, the isoform composition of keratin filaments changes • Wound-associated keratin isoforms organize cellular signals to activate myosin • Keratin isoform-dependent signaling is separable from canonical mechanical function Nanes et al. explore why the seemingly simple mechanical function of keratin intermediate filaments requires a protein family with 54 isoforms. They find that skin wound healing triggers a change in keratin isoform expression not to alter force resistance but to organize signals activating myosin and promoting cell motility. [ABSTRACT FROM AUTHOR]

Published

2024

14. Transcriptomic evidence for T cell‐fibroblast‐keratinocyte axis via IL‐13‐periostin‐integrin in atopic dermatitis.

Author

Tran, Nguyen Quoc Vuong, Kobayashi, Yoshiaki, Nakamura, Yuki, Ishimaru, Kayoko, Izuhara, Kenji, and Nakao, Atsuhito

Subjects

*CELL analysis, *KILLER cells, *CELL communication, *T cells, *BLAST injuries, KERATINOCYTE differentiation

Abstract

The article delves into the function of periostin in atopic dermatitis (AD) by examining cell interactions in skin biopsy samples from healthy individuals, AD patients, and psoriasis patients. It reveals that POSTN and its receptors are mainly expressed in keratinocytes and fibroblasts, with higher POSTN levels in AD compared to healthy skin and psoriasis. The study suggests a T cell-fibroblast-keratinocyte axis in AD, with periostin playing a crucial role in linking Th2-type responses to keratinocyte activation. The research underscores the significance of periostin as a key molecule in AD, hinting at the potential benefits of targeting periostin signaling for AD treatment. [Extracted from the article]

Published

2024

15. H Antigen expression modulates epidermal Keratinocyte Integrity and differentiation.

Author

Jin, Seon-Pil, Oh, Jang-Hee, Kim, Namjoo Kaylee, and Chung, Jin Ho

Subjects

BLOOD group antigens, EPIDERMAL growth factor receptors, ABO blood group system, LIGANDS (Biochemistry), ERYTHROCYTES, KERATINOCYTE differentiation

Abstract

Background: ABO blood group antigens (ABH antigens) are carbohydrate chains glycosylated on epithelial and red blood cells. Recent findings suggest reduced ABH expression in psoriasis and atopic dermatitis, a chronic inflammatory skin disease with retained scale. H antigen, a precursor for A and B antigens, is synthesized by fucosyltransferase 1 (FUT1). Desmosomes, critical for skin integrity, are known to require N-glycosylation for stability. We investigate the impact of H antigens, a specific type of glycosylation, on desmosomes in keratinocytes. Method: Primary human keratinocytes were transfected with FUT1 siRNA or recombinant adenovirus for FUT1 overexpression. Cell adhesion and desmosome characteristics and their underlying mechanisms were analyzed. Result: The knockdown of FUT1, responsible for H2 antigen expression in the skin, increased cell-cell adhesive strength and desmosome size in primary cultured keratinocytes without altering the overall desmosome structure. Desmosomal proteins, including desmogleins or plakophilin, were upregulated, suggesting enhanced desmosome assembly. Reduced H2 antigen expression via FUT1 knockdown led to increased keratinocyte differentiation, evidenced by elevated expression of differentiation markers. Epidermal growth factor receptor (EGFR) has been described to be associated with FUT1 and promotes cell migration and differentiation. The effects of FUT1 knockdown were recapitulated by an EGFR inhibitor concerning desmosomal proteins and cellular differentiation. Further investigation demonstrated that the FUT1 knockdown reduced EGFR signaling by lowering the levels of EGF ligands rather than directly regulating EGFR activity. Moreover, FUT1 overexpression reversed the effects observed in FUT1 knockdown, resulting in the downregulation of desmosomal proteins and differentiation markers while increasing both mRNA and protein levels of EGFR ligands. Conclusion: The expression level of FUT1 in the epidermis appears to influence cell-cell adhesion and keratinocyte differentiation status, at least partly through regulation of H2 antigen and EGFR ligand expression. These observations imply that the fucosylation of the H2 antigen by FUT1 could play a significant role in maintaining the molecular composition and regulation of desmosomes and suggest a possible involvement of the altered H2 antigen expression in skin diseases, such as psoriasis and atopic dermatitis. [ABSTRACT FROM AUTHOR]

Published

2024

16. Autophagy-Mediated Cellular Remodeling during Terminal Differentiation of Keratinocytes in the Epidermis and Skin Appendages.

Author

Eckhart, Leopold, Gruber, Florian, and Sukseree, Supawadee

Subjects

*SEBACEOUS glands, *APOPTOSIS, *CELL differentiation, *PRODUCT differentiation, *EPITHELIAL cells, KERATINOCYTE differentiation

Abstract

The epidermis of the skin and skin appendages, such as nails, hair and sebaceous glands, depend on a balance of cell proliferation and terminal differentiation in order to fulfill their functions at the interface of the body and the environment. The differentiation of epithelial cells of the skin, commonly referred to as keratinocytes, involves major remodeling processes that generate metabolically inactive cell remnants serving as building blocks of the epidermal stratum corneum, nail plates and hair shafts. Only sebaceous gland differentiation results in cell disintegration and holocrine secretion. A series of studies performed in the past decade have revealed that the lysosome-dependent intracellular degradation mechanism of autophagy is active during keratinocyte differentiation, and the blockade of autophagy significantly alters the properties of the differentiation products. Here, we present a model for the autophagy-mediated degradation of organelles and cytosolic proteins as an important contributor to cellular remodeling in keratinocyte differentiation. The roles of autophagy are discussed in comparison to alternative intracellular degradation mechanisms and in the context of programmed cell death as an integral end point of epithelial differentiation. [ABSTRACT FROM AUTHOR]

Published

2024

17. Novel three‐dimensional live skin‐like in vitro composite for bioluminescence reporter gene assay.

Author

Tomita, Tatsunosuke, Nakajima, Yoshihiro, Ohmiya, Yoshihiro, and Miyazaki, Koyomi

Subjects

*TOPICAL drug administration, *REPORTER genes, *BIOLUMINESCENCE, *IMMUNOHISTOCHEMISTRY, *HYDROPHOBIC compounds, *CELL culture, KERATINOCYTE differentiation

Abstract

We genetically manipulated HaCaT cells, a spontaneously immortalised normal keratinocyte cell line, to stably express two different coloured luciferase reporter genes, driven by interleukin 8 (IL‐8) and ubiquitin‐C (UBC) promoters, respectively. Subsequently, we generated a three‐dimensional (3D) skin‐like in vitro composite (SLIC) utilising these cells, with the objective of monitoring bioluminescence emitted from the SLIC. This SLIC was generated on non‐woven silica fibre membranes in differentiation medium. Immunohistochemical analyses of skin differentiation markers in the SLIC revealed the expression of keratins 2 and 10, filaggrin, and involucrin, indicating mature skin characteristics. This engineered SLIC was employed for real‐time bioluminescence monitoring, allowing the assessment of time‐ and dose‐dependent responses to UV stress, as well as to hydrophilic and hydrophobic chemical loads. Notably, evaluation of responses to hydrophobic substances has been challenging with conventional 2D cell culture methods, suggesting the need for a new approach, which this technology could address. Our observations suggest that engineered SLIC with constitutively expressing reporters driven by selected promoters which are tailored to specific objectives, significantly facilitates assays exploring the physiological functions of skin cells based on genetic response mechanisms. It also highlights new avenues for evaluating the physiological impacts of various compounds designed for topical application to human skin. [ABSTRACT FROM AUTHOR]

Published

2024

18. Upregulation of keratin 15 is required for varicella-zoster virus replication in keratinocytes and is attenuated in the live attenuated vOka vaccine strain.

Author

Tommasi, Cristina, Yogev, Ohad, Yee, Michael B., Drousioti, Andriani, Jones, Meleri, Ring, Alice, Singh, Manuraj, Dry, Inga, Atkins, Oscar, Naeem, Aishath S., Kriplani, Nisha, Akbar, Arne N., Haas, Jürgen G., O'Toole, Edel A., Kinchington, Paul R., and Breuer, Judith

Subjects

*GENE expression, *VARICELLA-zoster virus, *REGULATOR genes, *HAIR follicles, *HERPES zoster, KERATINOCYTE differentiation

Abstract

Varicella-zoster virus (VZV) is the etiological agent of chickenpox and shingles, diseases characterised by epidermal virus replication in skin and mucosa and the formation of blisters. We have previously shown that VZV infection has a profound effect on keratinocyte differentiation, altering the normal pattern of epidermal gene expression. In particular, VZV infection reduces expression of suprabasal keratins 1 and 10 and desmosomal proteins, disrupting epidermal structure to promote expression of a blistering phenotype. Here, we extend these findings to show that VZV infection upregulates the expression of keratin 15 (KRT15), a marker expressed by basal epidermal keratinocytes and hair follicles stem cells. We demonstrate that KRT15 is essential for VZV replication in the skin, since downregulation of KRT15 inhibits VZV replication in keratinocytes, while KRT15 exogenous overexpression supports viral replication. Importantly, our data show that VZV upregulation of KRT15 depends on the expression of the VZV immediate early gene ORF62. ORF62 is the only regulatory gene that is mutated in the live attenuated VZV vaccine and contains four of the five fixed mutations present in the VZV Oka vaccine. Our data indicate that the mutated vaccine ORF62 is not capable of upregulating KRT15, suggesting that this may contribute to the vaccine attenuation in skin. Taken together our data present a novel association between VZV and KRT15, which may open a new therapeutic window for a topical targeting of VZV replication in the skin via modulation of KRT15. [ABSTRACT FROM AUTHOR]

Published

2024

19. Investigation into the significant role of dermal‐epidermal interactions in skin ageing utilising a bioengineered skin construct.

Author

Costello, Lydia, Goncalves, Kirsty, De Los Santos Gomez, Paola, Hulette, Ben, Dicolandrea, Teresa, Flagler, Michael J., Isfort, Robert, Oblong, John, Bascom, Charlie, and Przyborski, Stefan

Subjects

*TISSUE differentiation, *MOLECULAR dynamics, *POPULATION aging, *FIBROBLASTS, *SKIN aging, KERATINOCYTE differentiation

Abstract

Increased prevalence of skin ageing is a growing concern due to an ageing global population and has both sociological and psychological implications. The use of more clinically predictive in vitro methods for dermatological research is becoming commonplace due to initiatives and the cost of clinical testing. In this study, we utilise a well‐defined and characterised bioengineered skin construct as a tool to investigate the cellular and molecular dynamics involved in skin ageing from a dermal perspective. Through incorporation of ageing fibroblasts into the dermal compartment we demonstrate the significant impact of dermal‐epidermal crosstalk on the overlying epidermal epithelium. We characterise the paracrine nature of dermal‐epidermal communication and the impact this has during skin ageing. Soluble factors, such as inflammatory cytokines released as a consequence of senescence associated secretory phenotype (SASP) from ageing fibroblasts, are known to play a pivotal role in skin ageing. Here, we demonstrate their effect on epidermal morphology and thickness, but not keratinocyte differentiation or tissue structure. Through a novel in vitro strategy utilising bioengineered tissue constructs, this study offers a unique reductionist approach to study epidermal and dermal compartments in isolation and tandem. [ABSTRACT FROM AUTHOR]

Published

2024

20. Stratum corneum hydration levels are negatively correlated with HbA1c levels in the elderly Chinese.

Author

Lai, Qingsong, Wang, Xiaohua, Lai, Zebin, Lai, Yulin, Ye, Li, Liu, Sha, Yang, Bin, and Man, Mao‐Qiang

Subjects

*TYPE 2 diabetes, *PEARSON correlation (Statistics), *TYPE 1 diabetes, *BLOOD sugar, KERATINOCYTE differentiation

Abstract

The study published in the Journal of Diabetes explores the relationship between stratum corneum hydration levels and HbA1c levels in elderly Chinese individuals. The research indicates a negative correlation between stratum corneum hydration and HbA1c levels, with individuals with type 2 diabetes showing lower hydration levels. The findings suggest that improving stratum corneum hydration could be an alternative approach in managing type 2 diabetes, as low hydration levels may increase proinflammatory cytokines linked to the disease's pathogenesis. Further studies are needed to understand the interaction between stratum corneum hydration and type 2 diabetes. [Extracted from the article]

Published

2024

21. Pharmacological Impacts of Mucopolysacccharide Polyphosphates in the Epidermis Involves Inhibition of Amphiregulin‐Mediated Signals in Keratinocytes.

Author

Hirase, Ryo, Fujita, Tomoyuki, Miyai, Tomohiro, Kawasaki, Hiroshi, and Koseki, Haruhiko

Subjects

*EPIDERMAL growth factor, *EPIDERMAL growth factor receptors, *TIGHT junctions, *MEMBRANE proteins, KERATINOCYTE differentiation

Abstract

The epidermis, the most superficial layer of the human skin, serves a critical barrier function, protecting the body from external pathogens and allergens. Dysregulation of epidermal differentiation contributes to barrier dysfunction and has been implicated in the pathology of various dermatological diseases, including atopic dermatitis (AD). Mucopolysaccharide polysulphate (MPS) is a moisturising agent used to treat xerosis in patients with AD. However, its mechanism of action on keratinocytes, the main constituents of the epidermis, remains unclear. In this study, we investigated the effect of MPS on keratinocytes by subjecting adult human epidermal and three‐dimensional cultured keratinocytes to MPS treatment, followed by transcriptome analysis. The analysis revealed that MPS treatment enhances keratinocyte differentiation and suppresses proliferation. We focused on amphiregulin (AREG), a membrane protein that belongs to the epidermal growth factor (EGF) family and possesses a heparin‐binding domain, as a significant target among the genes altered by MPS. MPS exerted an inhibitory effect directly on AREG, rather than on EGF receptors or other members of the EGF family. Furthermore, AREG leads to a reduction in epidermal barrier function, whereas MPS contributes to barrier enhancement via AREG inhibition. Collectively, these findings suggest that MPS modulates barrier function through AREG inhibition, offering insights into potential therapeutic strategies for skin barrier restoration. [ABSTRACT FROM AUTHOR]

Published

2024

22. Fibroblast stromal support model for predicting human papillomavirus-associated cancer drug responses.

Author

James, Claire D., Lewis, Rachel L., Fakunmoju, Alexis L., Witt, Austin J., Youssef, Aya H., Xu Wang, Rais, Nabiha M., Prabhakar, Apurva T., Machado, J. Mathew, Otoa, Raymonde, and Bristol, Molly L.

Subjects

*SELECTIVE estrogen receptor modulators, *HUMAN papillomavirus, *DRUG discovery, *OROPHARYNGEAL cancer, *THERAPEUTICS, KERATINOCYTE differentiation

Abstract

Currently, there are no specific antiviral therapeutic approaches targeting Human papillomaviruses (HPVs), which cause around 5% of all human cancers. Specific antiviral reagents are particularly needed for HPV-related oropharyngeal cancers (HPV+OPCs) whose incidence is increasing and for which there are no early diagnostic tools available. We and others have demonstrated that the estrogen receptor alpha (ERα) is overexpressed in HPV+OPCs, compared to HPV-negative cancers in this region, and that these elevated levels are associated with an improved disease outcome. Utilizing this HPV+-specific overexpression profile, we previously demonstrated that estrogen attenuates the growth and cell viability of HPV+ keratinocytes and HPV+ cancer cells in vitro. Expansion of this work in vivo failed to replicate this sensitization. The role of stromal support from the tumor microenvironment (TME) has previously been tied to both the HPV lifecycle and in vivo therapeutic responses. Our investigations revealed that in vitro co-culture with fibroblasts attenuated HPV+-specific estrogen growth responses. Continuing to monopolize on the HPV+-specific overexpression of ERα, our co-culture models then assessed the suitability of the selective estrogen receptor modulators (SERMs), raloxifene and tamoxifen, and showed growth attenuation in a variety of our models to one or both of these drugs in vitro. Utilization of these SERMs in vivo closely resembled the sensitization predicted by our co-culture models. Therefore, the in vitro fibroblast co-culture model better predicts in vivo responses. We propose that utilization of our co-culture in vitro model can accelerate cancer therapeutic drug discovery. [ABSTRACT FROM AUTHOR]

Published

2024

23. Piperonylic Acid Promotes Hair Growth by Activation of EGFR and Wnt/β-Catenin Pathway.

Author

Han, Seung Hyun, Jo, Kyung Won, Kim, Younghyun, and Kim, Kyong-Tai

Subjects

*EPIDERMAL growth factor receptors, *ALKALINE phosphatase, *SMALL molecules, *CELLULAR signal transduction, *BALDNESS, *HAIR growth, *HAIR follicles, KERATINOCYTE differentiation

Abstract

Dermal papilla cells (DPCs) are located at the bottom of the hair follicle and play a critical role in hair growth, shape, and cycle. Epidermal growth factor receptor (EGFR) and Wnt/β-catenin signaling pathways are essential in promoting keratinocyte activation as well as hair follicle formation in DPCs. Piperonylic acid is a small molecule that induces EGFR activation in keratinocytes. However, the effects of piperonylic acid on DPCs in regard to the stimulation of hair growth have not been studied. In the present study, piperonylic acid was shown to activate the Wnt/β-catenin signaling pathway in addition to the EGFR signaling pathway in DPCs. Piperonylic acid suppressed DKK1 expression, which presumably promoted the accumulation of β-catenin in the nucleus. In addition, piperonylic acid promoted cyclin D upregulation and cell growth and increased the expression of alkaline phosphatase (ALP), a DPC marker. In a clinical study, the group that applied a formulation containing piperonylic acid had a significantly higher number of hairs per unit area than the placebo group. These results identify piperonylic acid as a promising new candidate for hair loss treatment. [ABSTRACT FROM AUTHOR]

Published

2024

24. Epidermal RORα Maintains Barrier Integrity and Prevents Allergic Inflammation by Regulating Late Differentiation and Lipid Metabolism.

Author

Hua, Xiangmei, Ficaro, Maria K., Wallace, Nicole L., and Dai, Jun

Subjects

*WESTERN immunoblotting, *LIPID metabolism, *CONTACT dermatitis, *DELETION mutation, *KERATINIZATION, KERATINOCYTE differentiation

Abstract

The skin epidermis provides a barrier that is imperative for preventing transepidermal water loss (TEWL) and protecting against environmental stimuli. The underlying molecular mechanisms for regulating barrier functions and sustaining its integrity remain unclear. RORα is a nuclear receptor highly expressed in the epidermis of normal skin. Clinical studies showed that the epidermal RORα expression is significantly reduced in the lesions of multiple inflammatory skin diseases. In this study, we investigate the central roles of RORα in stabilizing skin barrier function using mice with an epidermis-specific Rora gene deletion (RoraEKO). While lacking spontaneous skin lesions or dermatitis, RoraEKO mice exhibited an elevated TEWL rate and skin characteristics of barrier dysfunction. Immunostaining and Western blot analysis revealed low levels of cornified envelope proteins in the RoraEKO epidermis, suggesting disturbed late epidermal differentiation. In addition, an RNA-seq analysis showed the altered expression of genes related to "keratinization" and "lipid metabolism" in RORα deficient epidermis. A lipidomic analysis further uncovered an aberrant ceramide composition in the RoraEKO epidermis. Importantly, epidermal Rora ablation greatly exaggerated percutaneous allergic inflammatory responses to oxazolone in an allergic contact dermatitis (ACD) mouse model. Our results substantiate the essence of epidermal RORα in maintaining late keratinocyte differentiation and normal barrier function while suppressing cutaneous inflammation. [ABSTRACT FROM AUTHOR]

Published

2024

25. Radiofrequency Currents Modulate Inflammatory Processes in Keratinocytes.

Author

Toledano-Macías, Elena, Martínez-Pascual, María Antonia, Cecilia-Matilla, Almudena, Bermejo-Martínez, Mariano, Pérez-González, Alfonso, Jara, Rosa Cristina, Sacristán, Silvia, and Hernández-Bule, María Luisa

Subjects

*EPIDERMAL growth factor receptors, *ELECTRIC currents, *KERATINOCYTES, *MATRIX metalloproteinases, *RADIO frequency therapy, KERATINOCYTE differentiation

Abstract

Keratinocytes play an essential role in the inflammatory phase of wound regeneration. In addition to migrating and proliferating for tissue regeneration, they produce a large amount of cytokines that modulate the inflammatory process. Previous studies have shown that subthermal treatment with radiofrequency (RF) currents used in capacitive resistive electric transfer (CRET) therapy promotes the proliferation of HaCat keratinocytes and modulates their cytokine production. Although physical therapies have been shown to have anti-inflammatory effects in a variety of experimental models and in patients, knowledge of the biological basis of these effects is still limited. The aim of this study was to investigate the effect of CRET on keratinocyte proliferation, cytokine production (IL-8, MCP-1, RANTES, IL-6, IL-11), TNF-α secretion, and the expression of MMP9, MMP1, NF-κB, ERK1/2, and EGFR. Human keratinocytes (HaCat) were treated with an intermittent 448 kHz electric current (CRET signal) in subthermal conditions and for different periods of time. Cell proliferation was analyzed by XTT assay, cytokine and TNF-α production by ELISA, NF-κB expression and activation by immunofluorescence, and MMP9, MMP1, ERK1/2, and EGF receptor expression and activation by immunoblot. Compared to a control, CRET increases keratinocyte proliferation, increases the transient release of MCP-1, TNF-α, and IL-6 while decreasing IL-8. In addition, it modifies the expression of MMPs and activates EGFR, NF-κB, and ERK1/2 proteins. Our results indicate that CRET reasonably modifies cytokine production through the EGF receptor and the ERK1/2/NF-κB pathway, ultimately modulating the inflammatory response of human keratinocytes. [ABSTRACT FROM AUTHOR]

Published

2024

26. 3D Approaches to Culturing Bovine Skin: Explant Culture versus Organotypic Skin Model.

Author

Baumbach, Christina-Marie, Anantama, Nadia Ayurini, Savkovic, Vuk, Mülling, Christoph K.W., Schinköthe, Jan, and Michler, Jule Kristin

Subjects

*MICROPHYSIOLOGICAL systems, *CELL communication, *TISSUE engineering, *ANIMAL experimentation, *CELLULAR signal transduction, KERATINOCYTE differentiation

Abstract

Introduction: Digital dermatitis (DD) in cattle appears with high prevalence; nevertheless, the knowledge on its pathogenesis is still limited. In this context, in vitro skin models represent a valuable tool to facilitate the study of DD. Methods: Two in vitro skin models were established using bovine distal limb skin: a skin explant model and an organotypic skin model. For the skin explant model, skin samples were cultured with an air-liquid interface for up to 7 days. Besides routine histopathological examination, readout parameters were Ki-67 and cleaved Caspase-3 stainings. For the organotypic model, primary keratinocytes were layered on top of a dermal equivalent containing mainly mitotically inactive fibroblasts and maintained for up to 21 days. At regular intervals (days 7, 14, and 21), cultured skin samples were taken for (immuno)histological analysis. Results: Both cultures could be maintained for the entire duration of the intended culture period. In the histopathological assessment, explant skin cultures showed ballooning degeneration of keratinocytes and segmental necrosis starting at day 5 of culturing. Initially, basal keratinocytes in the organotypic model differentiated as demonstrated by positive Keratin 14, Desmoglein-1, Loricrin, and Involucrin immunofluorescent stainings. Ki-67 was observed occasionally and suprabasally still after 21 days of culture. Conclusion: Both in vitro models proved dependable and constitute a viable option for replacing experiments on live animals, each with its own benefits. Whereas skin explants include all cell types available in vivo and can therefore reflect realistic cell-cell interactions and signaling pathways, the organotypic model offers a higher standardization and reproducibility. Depending on the focus of future studies, both models can be used for specific experimental purposes of bovine dermatological research in general or specialized questions concerning (infectious) claw diseases as, e.g., DD. [ABSTRACT FROM AUTHOR]

Published

2024

27. Facial pore refining by targeting dermal and epidermal functions: Assessment across age and gender.

Author

De Tollenaere, Morgane, Meunier, Marie, Durduret, Anaïs, Chapuis, Emilie, Auriol, Pascale, Auriol, Daniel, Scandolera, Amandine, and Reynaud, Romain

Subjects

*CELL proliferation, *ASIANS, *EXTRACELLULAR matrix, *COLLAGEN, KERATINOCYTE differentiation

Abstract

Background: Conspicuous facial pores are benign but represent a cosmetic concern for men and women. Recent works described dermal and epidermal impairments as clinical causes of enlarged pores. Morphological modifications of skin at the site of pores were associated with collagen density loss, possible alteration of extracellular matrix and abnormal differentiation of keratinocytes. Aims: A composition containing mannose‐6‐phosphate (Active Complex) was designed to address these different aspects of pore enlargement. In vitro and ex vivo evaluations were conducted in different models mimicking disturbance of dermal and epidermal functions. The pore refining activity of Active Complex was assessed in two clinical trials studying a Caucasian women cohort and an Asian men cohort. Results: At the dermal level, Active Complex upregulated collagen I and decorin synthesis, and genes encoding collagens I, III, V, VII, XVII; suggesting its ability to favor collagen fiber organization and anchorage. The downregulation of matrix metalloprotease, involved in extracellular matrix degradation, reinforced the protective effect of Active Complex in the dermis. Active Complex down modulated differentiation markers in keratinocytes as well as genes involved in cell renewal. Study of reconstructed human epidermis modeling keratinocyte hyperproliferation revealed that Active Complex mitigated two markers of this state: number of nuclei in the stratum corneum and involucrin expression. Clinical trials confirmed the pore refining activity of Active Complex on men and women of different ages and ethnicities; −24% total skin pore area after 56 days of application on women, and −30.2% on men after 7 days. Conclusions: This work demonstrates the interest to target dermal and epidermal modifications described in conspicuous pore area, especially dermis fiber organization, to address this cosmetic concern. [ABSTRACT FROM AUTHOR]

Published

2024

28. Transcriptional responses consistent with perturbation in dermo-epidermal homeostasis in septic sole ulceration.

Author

Reeder, T.L., Zarlenga, D.S., Ziegler, A.L., and Dyer, R.M.

Subjects

*AP-1 transcription factor, *NITRIC-oxide synthases, *TUMOR necrosis factors, *MATRIX metalloproteinases, KERATINOCYTE differentiation

Abstract

The list of standard abbreviations for JDS is available at adsa.org/jds-abbreviations-24. Nonstandard abbreviations are available in the Notes. The aim of this study was to evaluate transcriptional changes in the sole epidermis and dermis of bovine claws with septic sole ulceration of the lateral claw. Assessment included changes in transcripts orchestrating epidermal homeostatic processes, including epidermal proliferation, differentiation, inflammation, and cell signaling. Sole epidermis and dermis samples were removed from region 4 of lesion-bearing lateral and lesion-free medial claws of pelvic limbs in multiparous, lactating Holstein cows. Control sole epidermis and dermis samples were obtained from region 4 of lateral claws of normal pelvic limbs. Transcript abundances were evaluated by real-time PCR, and relative expression analyzed by ANOVA. Relative to normal lateral claws, sole epidermis and dermis in ulcer-bearing claws exhibited downregulation of genes associated with growth factors, growth factor receptors, activator protein 1 (AP-1) and proto-oncogene (CMYC) transcription components, cell cycle elements, lateral cell-to-cell signaling elements, and structures of early and late keratinocyte differentiation. These changes were accompanied by upregulation of proinflammatory transcripts interleukin 1 α (IL1A), interleukin1 β (IL1B), interleukin 1 receptor 1 (IL1R1), inducible nitric oxide synthase (NOS2), the inflammasome components NOD-like receptor protein 3 (NLRP3), pyrin and caspase recruitment domain (PYCARD), caspase-1 interleukin converting enzyme (CASPASE), the matrix metalloproteinases (MMP2 and MMP9), and the anti-inflammatory genes interleukin 1 receptor antagonist (IL1RN) and interleukin1 receptor 2 (IL1R2). Transcript abundance varied across epidermis and dermis from the ulcer center, margin, and epidermis and dermis adjacent to the lesion. Sole epidermis and dermis of lesion-free medial claws exhibited changes paralleling those in the adjacent lateral claws in an environment lacking inflammatory transcripts and downregulated IL1A , interleukin 18 (IL18), tumor necrosis factor α (TNFA), and NOS2. These data imply perturbations in signal pathways driving epidermal proliferation and differentiation are associated with, but not inevitably linked to epidermis and dermis inflammation. Further work is warranted to better define the role of crushing tissue injury, sepsis, metalloproteinase activity, and inflammation in sole ulceration. [ABSTRACT FROM AUTHOR]

Published

2024

29. Molecular evidence of sterile tissue damage during pathogenesis of the pododermatitis aseptica hemorrhagica circumscripta is associated with disturbed epidermal-dermal homeostasis.

Author

Reeder, T.L., Zarlenga, D.S., and Dyer, R.M.

Subjects

*DERMIS, *CELLULAR signal transduction, *CLAWS, *GROWTH factors, *EPIDERMIS, KERATINOCYTE differentiation

Abstract

The list of standard abbreviations for JDS is available at adsa.org/jds-abbreviations-24. Nonstandard abbreviations are available in the Notes. Pododermatitis aseptica hemorrhagica circumscripta is associated with metalloproteinase 2 weakening of distal phalangeal suspensory structures and sinkage of the distal phalanx in the claw capsule. Pressure from the tuberculum flexorium on the sole epidermis and dermis produces hemorrhagic tissue injury and defective horn production appearing as yellow-red, softened claw horn in region 4 of the sole. A model of the MAPK/ERK signal cascade orchestrating epidermal-dermal homeostasis was employed to determine if sterile inflammatory responses are linked to disturbed signal transduction for epidermal homeostasis in sole epidermis and dermis. The objective was to assess shifts in target genes of inflammation, up- and downstream MAPK/ERK signal elements, and targeted genes supporting epidermal proliferation and differentiation. Sole epidermis and dermis were removed from lateral claws bearing lesions of PAHC, medial claws from the same limb and lateral claws from completely normal limbs of multiparous, lactating Holstein cows. The abundance levels of targeted transcripts were evaluated by real-time PCR. Lesion effects were assessed by ANOVA, and mean comparisons were performed with t -tests to assess variations between mean expression in ulcer-bearing or medial claw dermis and epidermis and completely normal lateral claw dermis and epidermis or between ulcer-bearing dermis and epidermis and medial claw dermis and epidermis. The lesions were sterile and showed losses across multiple growth factors, their receptors, several downstream AP1 transcription components, CMYC, multiple cell-cycle and terminal differentiation elements conducted by MAPK/ERK signals and β 4, α 6, and collagen 17A hemidesmosome components. These losses coincided with increased cytokeratin 6, β 1 integrin, proinflammatory metalloproteinases 2 and 9, IL1B and physiologic inhibitors of IL1B, the decoy receptor, and receptor antagonist. Medial claw epidermis and dermis from limbs with lateral claws bearing PAHC showed reductions in upstream MAPK/ERK signal elements and downstream targets that paralleled those in hemorrhagic lesions. Inhibitors of IL1B increased in the absence of real increases in inflammatory targets in the medial claw dermis and epidermis. Losses across multiple signal path elements and downstream targets were associated with negative effects on targeted transcripts supporting claw horn production and wound repair across lesion-bearing lateral claws and lesion-free medial claw dermis and epidermis. It was unclear if the sterile inflammation was causative or a consequence of these perturbations. [ABSTRACT FROM AUTHOR]

Published

2024

30. Keratinocyte derived extracellular vesicles mediated crosstalk between epidermis and dermis in UVB-induced skin inflammation.

Author

Li, Yubin, Baniel, Avital, Diaz, DeAnna, Ogawa-Momohara, Mariko, Ricco, Cristina, Eldaboush, Ahmed, Bashir, Muhammad, Sharma, Meena, Liu, Ming-Lin, and Werth, Victoria P.

Subjects

*KNOCKOUT mice, *EXTRACELLULAR vesicles, *SKIN inflammation, *KERATINOCYTES, *DERMIS, *IRRADIATION, KERATINOCYTE differentiation

Abstract

Background and rationale: Ultraviolet-B (UVB) light induces dermal inflammation, although it is mostly absorbed in the epidermis. Recent reports suggest extracellular vesicles (EVs) act as a mediator of photodamage signaling. Melatonin is reported to be a protective factor against UV-induced damage. We hypothesized that EVs derived from UVB-irradiated keratinocytes might trigger proinflammatory responses in dermal cells and tested whether melatonin can ameliorate UVB-induced inflammation. Methods: We used UVB-irradiated HaCaT cells, primary keratinocytes and STING knock-out mice to model production of EVs under photodamaging conditions and performed immunoblotting and ELISA to measure their effect on dermal macrophages. Results: UVB-irradiated keratinocytes produce an increased number of EVs that contain higher concentrations of DNA and protein compared with controls. KC-derived EVs (KEVs) induced a STING- and inflammasome-mediated proinflammatory response in macrophages in vitro, and a pronounced inflammatory infiltrate in mouse dermis in vivo. Melatonin ameliorated KEVs inflammatory effect both in vitro and in vivo. Conclusions: This data suggests EVs are mediators in a crosstalk that takes place between keratinocytes and their neighboring cells as a result of photodamage. Further studies exploring EVs induced by damaging doses of UVB, and their impact on other cells will provide insight into photodamage and may help develop targeted therapeutic approaches. [ABSTRACT FROM AUTHOR]

Published

2024

31. Ethosomes-mediated tryptanthrin delivery as efficient anti-psoriatic nanotherapy by enhancing topical drug absorption and lipid homeostasis.

Author

Wang, Pengyu, Hong, Shihao, Cao, Can, Guo, Shijie, Wang, Chen, Chen, Xi, Wang, Xinnan, Song, Ping, Li, Ning, and Xu, Ruodan

Subjects

*MONOSODIUM glutamate, *DRUG absorption, *ETIOLOGY of diseases, *TOPICAL drug administration, *DRUG bioavailability, KERATINOCYTE differentiation

Abstract

Psoriasis is a chronic, relapsing, and refractory immune-mediated skin disease with the etiology and pharmaceutical targets remaining unsatisfactorily addressed. Topical herbal-derived compounds, such as tryptanthrin (Tryp), have been considered as an alternative therapy for psoriasis due to their lower costs and fewer side effects compared to other therapies. However, the effectiveness of topically administered drugs is substantially limited by the thickened pathological skin barrier and the low bioavailability of drugs in the deeper layers of the lesion. Ethosomes, being a novel phospholipid-based vesicle system with high content of ethanol, have been implicated in enhancing topical drug absorption and restoring psoriatic lesions. In this study, taking advantages of ethosomes as a soft and malleable drug carrier, we constructed the Tryp-loaded ethosome (Tryp-ES) through a one-step microfluidics-based technique. The optimal formulation of Tryp-ES was achieved by adding amino-acid-derived surfactant sodium lauroyl glutamate, and Tryp-ES exhibited homogeneous particle size and favorable stability at room temperature. In vitro evaluations showed that Tryp of Tryp-ES could be easily internalized into cells and accumulated in cell nuclei, hence inhibited the abnormally proliferated keratinocytes by inducing apoptosis. In vivo and in vitro assessment using psoritic skin of mice revealed that Tryp-ES had preferred skin retention and permeation of loaded drugs within the initial 1 h of topical administration, which could be attributed to transient disintegrations of cell membranes by ethosomes, thus improved cellular fluidity and permeability. Notably, a synergistic effect of ethosomes and Tryp was found in psoriatic mice. Tryp-ES-treated mice showed substantially ameliorated symptoms of psoriasis and reduced pathological alterations due to hyperplasia, inflammation and angiogenesis, without detectable local or systemic toxicities. Interestingly, lipidomics analysis confirmed that the supplementation of phospholipids, as in the form of ethosome vehicles, was an alterantive strategy to relieve psoriatic pathologies. Taken together, this study provides a novel impact for ethosomal topical delivery of Tryp and underlines their potential as an effective therapy for the management of psoriasis. [ABSTRACT FROM AUTHOR]

Published

2024

32. Protease-Activated Receptor 2 in inflammatory skin disease: current evidence and future perspectives.

Author

Mengjie Fan, Xiaoyao Fan, Yangfan Lai, Jin Chen, Yifan Peng, Yao Peng, Leihong Xiang, and Ying Ma

Subjects

G protein coupled receptors, PROTEASE-activated receptors, ACNE, KERATINOCYTE differentiation, SERINE proteinases

Abstract

Protease-activated receptor-2 (PAR2) is a class-A G protein-coupled receptor (GPCR) activated by serine proteases and is expressed by multiple tissues, including the skin. PAR2 is involved in the skin inflammatory response, promoting Th2 inflammation, delaying skin barrier repair, and affecting the differentiation of keratinocytes. It also participates in the transmission of itch and pain sensations in the skin. Increasing evidence indicates that PAR2 plays an important role in the pathogenesis of inflammatory skin diseases such as acne vulgaris, rosacea, psoriasis, and atopic dermatitis. Additional focus will be placed on potential targeted therapies based on PAR2. The Goal of this review is to outline the emerging effects of PAR2 activation in inflammatory skin disease and highlight the promise of PAR2 modulators. [ABSTRACT FROM AUTHOR]

Published

2024

33. The Importance of Biotinylation for the Suitability of Cationic and Neutral Fourth-Generation Polyamidoamine Dendrimers as Targeted Drug Carriers in the Therapy of Glioma and Liver Cancer.

Author

Uram, Łukasz, Twardowska, Magdalena, Szymaszek, Żaneta, Misiorek, Maria, Łyskowski, Andrzej, Setkowicz, Zuzanna, Rauk, Zuzanna, and Wołowiec, Stanisław

Subjects

*POLYAMIDOAMINE dendrimers, *LIVER cells, *CENTRAL nervous system, *CAENORHABDITIS elegans, *DRUG carriers, KERATINOCYTE differentiation

Abstract

In this study, we hypothesized that biotinylated and/or glycidol-flanked fourth-generation polyamidoamine (PAMAM G4) dendrimers could be a tool for efficient drug transport into glioma and liver cancer cells. For this purpose, native PAMAM (G4) dendrimers, biotinylated (G4B), glycidylated (G4gl), and biotinylated and glycidylated (G4Bgl), were synthesized, and their cytotoxicity, uptake, and accumulation in vitro and in vivo were studied in relation to the transport mediated by the sodium-dependent multivitamin transporter (SMVT). The studies showed that the human temozolomide-resistant glioma cell line (U-118 MG) and hepatocellular carcinoma cell line (HepG2) indicated a higher amount of SMVT than human HaCaT keratinocytes (HaCaTs) used as a model of normal cells. The G4gl and G4Bgl dendrimers were highly biocompatible in vitro (they did not affect proliferation and mitochondrial activity) against HaCaT and U-118 MG glioma cells and in vivo (against Caenorhabditis elegans and Wistar rats). The studied compounds penetrated efficiently into all studied cell lines, but inconsistently with the uptake pattern observed for biotin and disproportionately for the level of SMVT. G4Bgl was taken up and accumulated after 48 h to the highest degree in glioma U-118 MG cells, where it was distributed in the whole cell area, including the nuclei. It did not induce resistance symptoms in glioma cells, unlike HepG2 cells. Based on studies on Wistar rats, there are indications that it can also penetrate the blood–brain barrier and act in the central nervous system area. Therefore, it might be a promising candidate for a carrier of therapeutic agents in glioma therapy. In turn, visualization with a confocal microscope showed that biotinylated G4B penetrated efficiently into the body of C. elegans, and it may be a useful vehicle for drugs used in anthelmintic therapy. [ABSTRACT FROM AUTHOR]

Published

2024

34. Revealing the Therapeutic Potential of Muscle-Derived Mesenchymal Stem/Stromal Cells: An In Vitro Model for Equine Laminitis Based on Activated Neutrophils, Anoxia–Reoxygenation, and Myeloperoxidase.

Author

Serteyn, Didier, Storms, Nazaré, Mouithys-Mickalad, Ange, Sandersen, Charlotte, Niesten, Ariane, Duysens, Julien, Graide, Hélène, Ceusters, Justine, and Franck, Thierry

Subjects

*LAMENESS in horses, *CELL metabolism, *HORSE diseases, *MESENCHYMAL stem cells, *STEM cells, *NEUTROPHILS, KERATINOCYTE differentiation

Abstract

Simple Summary: Equine laminitis is a serious condition causing severe pain and lameness in horses, often leading to euthanasia. This study developed a lab model to better understand laminitis using keratinocytes which were exposed to conditions simulating the disease. This research showed that adding muscle-derived stem cells helped protect and restore the keratinocytes' metabolism. These results highlight the potential of stem cell therapy in treating laminitis, offering new hope for managing this debilitating disease in horses. Laminitis in horses is a crippling condition marked by the deterioration of the dermal–epidermal interface, leading to intense lameness and discomfort, often necessitating euthanasia. This study aimed to establish an in vitro model of laminitis using a continuous keratinocyte cell line exposed to anoxia–reoxygenation and an activated neutrophil supernatant. A significant decrease in the keratinocytes' metabolism was noted during the reoxygenation period, indicative of cellular stress. Adding muscle-derived mesenchymal stem/stromal cells during the reoxygenation demonstrated a protective effect, restoring the keratinocytes' metabolic activity. Moreover, the incubation of the keratinocytes with either an activated neutrophil supernatant or myeloperoxidase alone induced increased keratinocyte myeloperoxidase activity, which was modulated by stem cells. These findings underscore the potential of muscle-derived mesenchymal stem/stromal cells in mitigating inflammation and restoring keratinocyte metabolism, offering insights for future cell therapy research in laminitis treatment. [ABSTRACT FROM AUTHOR]

Published

2024

35. MicroRNA Signature in an In Vitro Keratinocyte Model of Diabetic Wound Healing.

Author

Tsai, Hsin-Chung, Chang, Gary Ro-Lin, Tung, Min-Che, Tu, Min-Yu, Chen, I-Chien, Liu, Yu-Hsien, Cidem, Abdulkadir, and Chen, Chuan-Mu

Subjects

*GENE expression, *WOUND healing, *GENE ontology, *GENE targeting, *GENE transfection, KERATINOCYTE differentiation

Abstract

Treating diabetic wounds effectively remains a significant clinical challenge. Emerging studies suggest that microRNAs (miRNAs) play crucial roles in various physiological and pathological processes and hold promise as therapeutic tools. This study investigates the miRNA expression profile in keratinocytes using a cell model of diabetic wounds. Microarray analysis revealed that 43 miRNAs from wounded keratinocytes incubated under diabetic conditions (high glucose/hypoxia) exhibited a two-fold change in expression compared to those incubated under normal conditions (low glucose/normoxia). Quantitative RT-PCR confirmed significant differences in the expression of eight miRNAs, with miR-3138 and miR-3679-5p being further analyzed for their roles in keratinocyte migration. Transfection with a miR-3138 mimic and a miR-3679-5p inhibitor indicated that upregulation of miR-3138 and downregulation of miR-3679-5p enhance keratinocyte migration in both normal and diabetic wounds. Pathway and gene ontology (GO) analyses identified potential pathways and functional annotations associated with miR-3138 and miR-3679-5p in diabetic wound healing. Potential human gene targets of miR-3138 and miR-3679-5p were predicted using a three-way comparison of the TargetScan, miRDB, and DIANA databases. This study elucidates the miRNA expression signature of human keratinocytes in a diabetes-like environment, providing deeper insights into the pathogenesis of diabetic wounds. [ABSTRACT FROM AUTHOR]

Published

2024

36. Neutral evolution of snoRNA Host Gene long non-coding RNA affects cell fate control.

Author

Vietri Rudan, Matteo, Sipilä, Kalle H, Philippeos, Christina, Ganier, Clarisse, Bhosale, Priyanka G, Negri, Victor A, and Watt, Fiona M

Subjects

*GENETIC drift, *LINCRNA, *MOLECULAR biology, *NON-coding RNA, *GENOMES, KERATINOCYTE differentiation

Abstract

A fundamental challenge in molecular biology is to understand how evolving genomes can acquire new functions. Actively transcribed, non-coding parts of the genome provide a potential platform for the development of new functional sequences, but their biological and evolutionary roles remain largely unexplored. Here, we show that a set of neutrally evolving long non-coding RNAs (lncRNAs) whose introns encode small nucleolar RNAs (snoRNA Host Genes, SNHGs) are highly expressed in skin and dysregulated in inflammatory conditions. Using SNHG7 and human epidermal keratinocytes as a model, we describe a mechanism by which these lncRNAs can increase self-renewal and inhibit differentiation. The activity of SNHG7 lncRNA has been recently acquired in the primate lineage and depends on a short sequence required for microRNA binding. Taken together, our results highlight the importance of understanding the role of fast-evolving transcripts in normal and diseased epithelia, and show how poorly conserved, actively transcribed non-coding sequences can participate in the evolution of genomic functionality. Synopsis: Small nucleolar RNA host genes (SNHGs) are poorly conserved but highly expressed long non-coding RNAs (lncRNA). Using primary cells from multiple species, this comparative study shows that SNHGs can affect epidermal keratinocyte self-renewal and are able to acquire new functionality over short evolutionary times. Expression of SNHGs changes during human epidermal differentiation and is dysregulated in skin inflammatory conditions. SNHG7 lncRNA promotes self-renewal and prevents differentiation of keratinocytes. SNHG7 has acquired its biological activity recently in the primate linage. miR-34-5p response elements are necessary for SNHG7-mediated regulation of self-renewal in primate keratinocytes. Highly expressed, neutrally evolving long non-coding RNAs arising from host genes that contain intronic small nucleolar RNAs can rapidly acquire new biological activity and influence cell fate in primate keratinocytes. [ABSTRACT FROM AUTHOR]

Published

2024

37. CASIN exerts anti‐aging effects through RPL4 on the skin of naturally aging mice.

Author

Zhang, Yijia, Wang, Xueer, Huang, Jianyuan, Zhang, Xinyue, Bu, Lingwei, Zhang, Yarui, Liang, Fengting, Wu, Shenhua, Zhang, Min, Zhang, Lu, and Zhang, Lin

Subjects

*TOPICAL drug administration, *RIBOSOMAL proteins, *SUBCUTANEOUS injections, *CELL cycle proteins, *LABORATORY mice, *SKIN aging, KERATINOCYTE differentiation

Abstract

Skin aging has been associated with the onset of various skin issues, and recent studies have identified an increase in Cdc42 activity in naturally aging mice. While previous literature has suggested that CASIN, a specific inhibitor of Cdc42 activity, may possess anti‐aging properties, its specific effects on the epidermis and dermis, as well as the underlying mechanisms in naturally aging mice, remain unclear. Our study revealed that CASIN demonstrated the ability to increase epidermal and dermal thickness, enhance dermal‐epidermal junction, and stimulate collagen and elastic fiber synthesis in 9‐, 15‐, and 24‐month‐old C57BL/6 mice in vivo. Moreover, CASIN was found to enhance the proliferation, differentiation, and colony formation and restore the cytoskeletal morphology of primary keratinocytes in naturally aging skin in vitro. Furthermore, the anti‐aging properties of CASIN on primary fibroblasts in aging mice were mediated by the ribosomal protein RPL4 using proteomic sequencing, influencing collagen synthesis and cytoskeletal morphology both in vitro and in vivo. Meanwhile, both subcutaneous injection and topical application exhibited anti‐aging effects for a duration of 21 days. Additionally, CASIN exhibited anti‐inflammatory properties, while reduced expression of RPL4 was associated with increased inflammation in the skin of naturally aging mice. Taken together, our results unveil a novel function of RPL4 in skin aging, providing a foundational basis for future investigations into ribosomal proteins. And CASIN shows promise as a potential anti‐aging agent for naturally aging mouse skin, suggesting potential applications in the field. [ABSTRACT FROM AUTHOR]

Published

2024

38. Salidroside alleviates imiquimod‐induced psoriasis by inhibiting GSDMD‐driven keratinocyte pyroptosis.

Author

Wang, Mengjie, Tu, Tuyagaer, Wang, Yangxingyun, Tian, Limin, and Yang, Yuenan

Subjects

*HEMATOXYLIN & eosin staining, *POLYMERASE chain reaction, *SKIN diseases, *KERATINOCYTES, *PYROPTOSIS, KERATINOCYTE differentiation

Abstract

Psoriasis is a common immune‐related polygenic inflammatory skin disease. Salidroside (SAL) exerts anti‐inflammatory and antioxidant effects and is used to treat skin diseases. However, the specific effects of SAL on psoriasis remain unclear. In this study, we aimed to investigate the efficacy of SAL for psoriasis treatment. Mice were treated with imiquimod (IMQ) to establish an in vivo psoriasis model. Histological analysis was conducted via hematoxylin and eosin staining. Cytokine release was determined via enzyme‐linked immunosorbent assay. Additionally, mRNA levels were determined via reverse transcription‐quantitative polymerase chain reaction. Protein expression was assessed via Western blotting. Gasdermin D (GSDMD) and Ki‐67 expression levels were determined via immunohistochemistry. Caspase 1 and GSDMD expression levels were determined via immunofluorescence assay. Furthermore, macrophage function and keratinocyte pyroptosis were also analyzed via flow cytometry. Cell proliferation was determined using 5‐ethynyl‐2ʹdeoxyuridine assay. SAL alleviated IMQ‐induced psoriasis. IMQ‐mediated GSDMD‐driven pyroptosis and keratinocyte hyperproliferation promoted M1 macrophage polarization. However, SAL treatment suppressed GSDMD expression, thereby inhibiting keratinocyte proliferation and pyroptosis and promoting M2 macrophage polarization. GSDMD deficiency further promoted the effects of SAL and suppressed psoriasis progression. Overall, our findings suggest that SAL exerts protective effects against psoriasis. Specifically, it exerts anti‐inflammatory effects by regulating M2 macrophage polarization and inhibiting keratinocyte pyroptosis‐driven proliferation induced by the immune microenvironment in psoriasis. [ABSTRACT FROM AUTHOR]

Published

2024

39. The coculture of in vitro produced porcine embryos and oviductal epithelial cells improves blastocyst formation and modify embryo quality.

Author

Lorenzo, Maria Soledad, Teplitz, Gabriela Maia, Luchetti, Carolina Griselda, Cruzans, Paula Romina, Bertonazzi, Analia, and Lombardo, Daniel Marcelo

Subjects

*EPITHELIAL cells, *EMBRYOS, *EMBRYOLOGY, *BLASTOCYST, *HORMONE receptors, KERATINOCYTE differentiation

Abstract

The efficiency of in vitro embryo production in mammals is influenced by variables associated with culture conditions during maturation, fertilization, and embryonic development. The embryos obtained often exhibit low quality due to suboptimal in vitro culture conditions compared to the in vivo environment. Co-culturing gametes and embryos with somatic cells has been developed to enhance in vitro culture conditions. This study aimed to assess the impact of coculturing in vitro-produced porcine embryos with porcine oviductal epithelial cells (POEC) on embryo development and quality. Firstly, a pure culture of POEC suitable for coculture systems was established. The epithelial origin of the cells was confirmed by the expression of E-cadherin and cytokeratin. The expression pattern of hormone receptors aligned with the diestrous oviduct, and POEC also secreted oviductal glycoprotein type 1 (OVGP-1). Secondly, POEC from passage 1 (POEC-1) were used to coculture with in vitro-produced porcine embryos. A successful coculture system was established without the addition of fetal bovine serum as a supplement. Coculturing POEC-1 in monolayers with in vitro-produced porcine embryos during the initial two days of culture enhanced the percentage of blastocysts and their hatching. Although the coculture did not alter the number of cells in the blastocysts or apoptosis assessed by TUNEL, it significantly reduced reactive oxygen species (ROS) levels in cleaved porcine embryos. This study represents the first report evaluating the quality of porcine embryos produced by IVF in coculture systems and assessing ROS levels in cleaved porcine embryos obtained by IVF. • The presence of oviductal epithelial cells during embryo in vitro culture enhanced porcine blastocyst formation. • The oviductal epithelial cells during embryo culture decrease ROS levels in porcine in vitro produced cleaved embryos. • The porcine oviductal epithelial cells expressed OVGP-1 during in vitro culture. [ABSTRACT FROM AUTHOR]

Published

2024

40. 25th Annual meeting of the European Society for Pigment Cell Research, Marseille, France.

Subjects

*BIOPRINTING, *MEDICAL sciences, *MOLECULAR biology, *CYTOLOGY, *CUTANEOUS malignant melanoma, *CILIA & ciliary motion, *WOUND healing, *MELANOGENESIS, KERATINOCYTE differentiation

Published

2024

41. IPCC2023: Looking for translational opportunities by persevering in basic pigment cell research.

Author

Boyano, María D., Asumendi, Aintzane, Garcia‐Borrón, José Carlos, Montoliu, Lluís, and Alonso, Santos

Subjects

*MOLECULAR biology, *CYTOLOGY, *SECRETED frizzled-related proteins, *DEUBIQUITINATING enzymes, *MORPHOLOGY, *MICROPHTHALMIA-associated transcription factor, *MELANOGENESIS, KERATINOCYTE differentiation

Published

2024

42. 25th International Pigment Cell Conference, Bilbao, Spain IPCC 2023.

Subjects

*LIFE sciences, *SKIN aging, *MICROPHTHALMIA-associated transcription factor, *MEDICAL sciences, *MOLECULAR biology, *SECRETED frizzled-related proteins, *MACROPHAGE colony-stimulating factor, *PHENOMENOLOGICAL biology, KERATINOCYTE differentiation

Published

2024

43. Anti-Inflammatory and Wound Healing Properties of Different Honey Varieties from Romania and Correlations to Their Composition.

Author

Iosageanu, Andreea, Stefan, Laura Mihaela, Craciunescu, Oana, and Cimpean, Anisoara

Subjects

*HONEY composition, *SKIN regeneration, *WOUND healing, *VITAMIN C, *HONEY, *CELL migration, KERATINOCYTE differentiation

Abstract

The complex composition of honey plays a crucial role in wound healing, exhibiting varying effects at different stages of the healing process. This study investigated seven honey varieties sourced from different regions of Romania using in vitro experimental models developed in macrophage-like, fibroblast, and keratinocyte cell lines to explore the mechanisms by which honey promoted the healing process. This study assessed the impact of honey on inflammatory cytokine production in macrophage-like cells, cell proliferation and collagen synthesis in fibroblasts, and cell proliferation and migration in keratinocytes. Additionally, correlation analysis was conducted to examine the relationship between honey composition and its biological properties. Honey varieties presented both anti- and pro-inflammatory effects. Moreover, they displayed dose-dependent pro-proliferative effects, stimulating collagen synthesis and cell migration, thereby enhancing the re-epithelialization process. The Pearson coefficient analysis indicated a strong positive correlation between biological activities and phenolic content. Additionally, there was a medium positive correlation with the ascorbic acid content and a medium negative correlation with the glucose content in the different honey varieties. Romanian honey varieties rich in phenolics showed potential in modulating inflammation, proliferation, collagen synthesis, and cell migration, suggesting their suitability for further evaluation and development of innovative dressings for skin tissue regeneration. [ABSTRACT FROM AUTHOR]

Published

2024

44. Adipose-Derived Stem-Cell-Membrane-Coated PLGA-PEI Nanoparticles Promote Wound Healing via Efficient Delivery of miR-21.

Author

Peng, Huiyu, Du, Fangzhou, Wang, Jingwen, Wu, Yue, Wei, Qian, Chen, Aoying, Duan, Yuhan, Shi, Shuaiguang, Zhang, Jingzhong, and Yu, Shuang

Subjects

*VASCULAR endothelial cells, *GENE expression, *CELL anatomy, *STEM cells, *WOUND healing, *SKIN regeneration, KERATINOCYTE differentiation

Abstract

miRNAs have been shown to be involved in the regulation of a variety of physiological and pathological processes, but their use in the treatment of diseases is still limited due to their instability. Biomimetic nanomaterials combine nanomaterials with cellular components that are readily modifiable and biocompatible, making them an emerging miRNA delivery vehicle. In this study, adipose-derived MSC membranes were wrapped around PLGA-PEI loaded with miR-21 through co-extrusion and later transplanted into C57BL/6 mice wounds. The wound-healing rate, epithelialization, angiogenesis, and collagen deposition were assessed after treatment and corroborated in vitro. Our study demonstrated that m/NP/miR-21 can promote wound healing in terms of epithelialization, dermal reconstruction, and neovascularization, and it can regulate the corresponding functions of keratinocytes, fibroblasts, and vascular endothelial cells. m/NP/miR-21 can inhibit the expression of PTEN, a gene downstream of miR-21, and increase the phosphorylation activation of AKT, which can then regulate the functions of fibroblasts. In conclusion, this provides a new approach to therapy for skin wounds using microRNA transporters and biomimetic nanoparticles. [ABSTRACT FROM AUTHOR]

Published

2024

45. Photodynamic Therapy as a Novel Therapeutic Modality Applying Quinizarin-Loaded Nanocapsules and 3D Bioprinting Skin Permeation for Inflammation Treatment.

Author

do Amaral, Stéphanie R., Amantino, Camila F., Atanasov, Aleksandar, Sousa, Stefanie Oliveira, Moakes, Richard, Oliani, Sonia Maria, Grover, Liam M., and Primo, Fernando L.

Subjects

*BIOPRINTING, *SKIN inflammation, *THERAPEUTICS, *PHOTODYNAMIC therapy, *CYTOTOXINS, KERATINOCYTE differentiation

Abstract

Skin inflammation associated with chronic diseases involves a direct role of keratinocytes in its immunopathogenesis, triggering a cascade of immune responses. Despite this, highly targeted treatments remain elusive, highlighting the need for more specific therapeutic strategies. In this study, nanocapsules containing quinizarin (QZ/NC) were developed and evaluated in an in vitro model of keratinocyte-mediated inflammation, incorporating the action of photodynamic therapy (PDT) and analyzing permeation in a 3D skin model. Comprehensive physicochemical, stability, cytotoxicity, and permeation analyses of the nanomaterials were conducted. The nanocapsules demonstrated desirable physicochemical properties, remained stable throughout the analysis period, and exhibited no spectroscopic alterations. Cytotoxicity tests revealed no toxicity at the lowest concentrations of QZ/NC. Permeation and cellular uptake studies confirmed QZ/NC permeation in 3D skin models, along with intracellular incorporation and internalization of the drug, thereby enhancing its efficacy in drug delivery. The developed model for inducing the inflammatory process in vitro yielded promising results, particularly when the synthesized nanomaterial was combined with PDT, showing a reduction in cytokine levels. These findings suggest a potential new therapeutic approach for treating inflammatory skin diseases. [ABSTRACT FROM AUTHOR]

Published

2024

46. Pathological Mechanisms Involved in Epidermolysis Bullosa Simplex: Current Knowledge and Therapeutic Perspectives.

Author

Bchetnia, Mbarka, Powell, Julie, McCuaig, Catherine, Boucher-Lafleur, Anne-Marie, Morin, Charles, Dupéré, Audrey, and Laprise, Catherine

Subjects

*GENE expression, *EPIDERMOLYSIS bullosa, *MUCOUS membranes, *CELL junctions, *DOMINANCE (Genetics), KERATINOCYTE differentiation

Abstract

Epidermolysis bullosa (EB) is a clinically and genetically heterogeneous group of mechanobullous diseases characterized by non-scarring blisters and erosions on the skin and mucous membranes upon mechanical trauma. The simplex form (EBS) is characterized by recurrent blister formation within the basal layer of the epidermis. It most often results from dominant mutations in the genes coding for keratin (K) 5 or 14 proteins (KRT5 and KRT14). A disruptive mutation in KRT5 or KRT14 will not only structurally impair the cytoskeleton, but it will also activate a cascade of biochemical mechanisms contributing to EBS. Skin lesions are painful and disfiguring and have a significant impact on life quality. Several gene expression studies were accomplished on mouse model and human keratinocytes to define the gene expression signature of EBS. Several key genes associated with EBS were identified as specific immunological mediators, keratins, and cell junction components. These data deepened the understanding of the EBS pathophysiology and revealed important functional biological processes, particularly inflammation. This review emphasizes the three EBS subtypes caused by dominant mutations on either KRT5 or KRT14 (localized, intermediate, and severe). It aims to summarize current knowledge about the EBS expression profiling pattern and predicted molecular mechanisms involved and to outline progress in therapy. [ABSTRACT FROM AUTHOR]

Published

2024

47. EpidermaQuant: Unsupervised Detection and Quantification of Epidermal Differentiation Markers on H-DAB-Stained Images of Reconstructed Human Epidermis.

Author

Zamojski, Dawid, Gogler, Agnieszka, Scieglinska, Dorota, and Marczyk, Michal

Subjects

*IMMUNOSTAINING, *K-means clustering, *FILAGGRIN, *PROTEIN analysis, KERATINOCYTE differentiation

Abstract

The integrity of the reconstructed human epidermis generated in vitro can be assessed using histological analyses combined with immunohistochemical staining of keratinocyte differentiation markers. Technical differences during the preparation and capture of stained images may influence the outcome of computational methods. Due to the specific nature of the analyzed material, no annotated datasets or dedicated methods are publicly available. Using a dataset with 598 unannotated images showing cross-sections of in vitro reconstructed human epidermis stained with DAB-based immunohistochemistry reaction to visualize four different keratinocyte differentiation marker proteins (filaggrin, keratin 10, Ki67, HSPA2) and counterstained with hematoxylin, we developed an unsupervised method for the detection and quantification of immunohistochemical staining. The pipeline consists of the following steps: (i) color normalization; (ii) color deconvolution; (iii) morphological operations; (iv) automatic image rotation; and (v) clustering. The most effective combination of methods includes (i) Reinhard's normalization; (ii) Ruifrok and Johnston color-deconvolution method; (iii) proposed image-rotation method based on boundary distribution of image intensity; and (iv) k-means clustering. The results of the work should enhance the performance of quantitative analyses of protein markers in reconstructed human epidermis samples and enable the comparison of their spatial distribution between different experimental conditions. [ABSTRACT FROM AUTHOR]

Published

2024

48. PI3K/AKT/mTOR Signaling Network in Human Health and Diseases.

Author

Omolekan, Tolulope O., Chamcheu, Jean Christopher, Buerger, Claudia, and Huang, Shile

Subjects

*SCIENTIFIC literature, *PLATELET-derived growth factor receptors, *GENE expression, *TRANSCRIPTION factors, *PROTEIN kinase B, *DNA repair, *EXTRACELLULAR signal-regulated kinases, KERATINOCYTE differentiation

Abstract

The article discusses the PI3K/AKT/mTOR signaling network and its role in human health and diseases. Dysregulation of this pathway is associated with various diseases, including cancer, infections, inflammation, and neurological, metabolic, and cardiovascular disorders. The article emphasizes the importance of understanding this signaling network to develop targeted therapies for conditions like cancer, neurodegenerative disorders, inflammation, autoimmune diseases, obesity, and diabetes. Specific studies are mentioned that investigate the role of this pathway in diseases such as colorectal cancer, psoriasis, breast cancer, progressive multifocal leukoencephalopathy, and osteonecrosis of the femoral head. The article concludes that a comprehensive understanding of this pathway is crucial for managing human health and diseases effectively. [Extracted from the article]

Published

2024

49. Low Immunogenicity of Keratinocytes Derived from Human Embryonic Stem Cells.

Author

Shen, Jiayi, Zeng, Xuanhao, Lv, Haozhen, Jin, Yiting, Liu, Yating, Lian, Weiling, Huang, Shiyi, Zang, Qing, Zhang, Qi, and Xu, Jinhua

Subjects

*HUMAN embryonic stem cells, *EMBRYONIC stem cells, *GRAFT rejection, *CLINICAL medicine, *IMMUNE response, KERATINOCYTE differentiation

Abstract

Epidermal transplantation is a common and widely used surgical technique in clinical medicine. Derivatives of embryonic stem cells have the potential to serve as a source of transplantable cells. However, allograft rejection is one of the main challenges. To investigate the immunogenicity of keratinocytes derived from human embryonic stem cells (ESKCs), we conducted a series of in vivo and in vitro experiments. The results showed that ESKCs have low HLA molecule expression, limited antigen presentation capabilities, and a weak ability to stimulate the proliferation and secretion of inflammatory factors in allogeneic PBMCs in vitro. In humanized immune mouse models, ESKCs elicited weak transplant rejection responses in the host. Overall, we found that ESKCs have low immunogenicity and may have potential applications in the field of regenerative medicine. [ABSTRACT FROM AUTHOR]

Published

2024

50. Molecular evidence of sterile tissue damage during pathogenesis of the pododermatitis aseptica hemorrhagica circumscripta is associated with disturbed epidermal-dermal homeostasis

Author

T.L. Reeder, D.S. Zarlenga, and R.M. Dyer

Subjects

sterile inflammation, sole ulcer, pododermatitis aseptica hemorrhagica circumscripta, cell cycle, keratinocyte differentiation, Dairy processing. Dairy products, SF250.5-275, Dairying, SF221-250

Abstract

ABSTRACT: Pododermatitis aseptica hemorrhagica circumscripta is associated with metalloproteinase 2 weakening of distal phalangeal suspensory structures and sinkage of the distal phalanx in the claw capsule. Pressure from the tuberculum flexorium on the sole epidermis and dermis produces hemorrhagic tissue injury and defective horn production appearing as yellow-red, softened claw horn in region 4 of the sole. A model of the MAPK/ERK signal cascade orchestrating epidermal-dermal homeostasis was employed to determine if sterile inflammatory responses are linked to disturbed signal transduction for epidermal homeostasis in sole epidermis and dermis. The objective was to assess shifts in target genes of inflammation, up- and downstream MAPK/ERK signal elements, and targeted genes supporting epidermal proliferation and differentiation. Sole epidermis and dermis were removed from lateral claws bearing lesions of PAHC, medial claws from the same limb and lateral claws from completely normal limbs of multiparous, lactating Holstein cows. The abundance levels of targeted transcripts were evaluated by real-time PCR. Lesion effects were assessed by ANOVA, and mean comparisons were performed with t-tests to assess variations between mean expression in ulcer-bearing or medial claw dermis and epidermis and completely normal lateral claw dermis and epidermis or between ulcer-bearing dermis and epidermis and medial claw dermis and epidermis. The lesions were sterile and showed losses across multiple growth factors, their receptors, several downstream AP1 transcription components, CMYC, multiple cell-cycle and terminal differentiation elements conducted by MAPK/ERK signals and β 4, α 6, and collagen 17A hemidesmosome components. These losses coincided with increased cytokeratin 6, β 1 integrin, proinflammatory metalloproteinases 2 and 9, IL1B and physiologic inhibitors of IL1B, the decoy receptor, and receptor antagonist. Medial claw epidermis and dermis from limbs with lateral claws bearing PAHC showed reductions in upstream MAPK/ERK signal elements and downstream targets that paralleled those in hemorrhagic lesions. Inhibitors of IL1B increased in the absence of real increases in inflammatory targets in the medial claw dermis and epidermis. Losses across multiple signal path elements and downstream targets were associated with negative effects on targeted transcripts supporting claw horn production and wound repair across lesion-bearing lateral claws and lesion-free medial claw dermis and epidermis. It was unclear if the sterile inflammation was causative or a consequence of these perturbations.

Published

2024