A novel method for a high enrichment of human corneal epithelial stem cells for genomic analysis

Kasinathan, Jhansi Rani; Namperumalsamy, Venkatesh Prajna; Muthukkaruppan, Veerappan; Chidambaranathan, Gowri Priya

doi:10.1002/jemt.22771

Cited by 6 publications

(4 citation statements)

References 25 publications

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“…Priya et al successfully identified and quantified LSCs based on ABCG2 and N/C ≥ 0.7 [ 69 ]. Additionally, Kasinathan et al established a two-step protocol by combining basal cell isolation and laser capture microdissection (LCM) of small cells with N/C ≥ 0.7 for LSC enrichment, which achieved 76–78% enrichment of LSC from 2% LSCs in total LECs [ 104 ]; Label-retaining cell: bromodeoxyuridine (BrdU) can take the place of thymidine to be incorporated into the replicated DNA during the S-phase of the cell cycle. The BrdU-based “pulse-chase” experiment has been widely applied for the identification of stem cell.…”

Section: Identification Of Lscsmentioning

confidence: 99%

Section: Identification Of Lscsmentioning

confidence: 99%

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An Insight into the Difficulties in the Discovery of Specific Biomarkers of Limbal Stem Cells

Guo

Zhang

Jia

et al. 2018

IJMS

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Keeping the integrity and transparency of the cornea is the most important issue to ensure normal vision. There are more than 10 million patients going blind due to the cornea diseases worldwide. One of the effective ways to cure corneal diseases is corneal transplantation. Currently, donations are the main source of corneas for transplantation, but immune rejection and a shortage of donor corneas are still serious problems. Graft rejection could cause transplanted cornea opacity to fail. Therefore, bioengineer-based corneas become a new source for corneal transplantation. Limbal stem cells (LSCs) are located at the basal layer in the epithelial palisades of Vogt, which serve a homeostatic function for the cornea epithelium and repair the damaged cornea. LSC-based transplantation is one of the hot topics currently. Clinical data showed that the ratio of LSCs to total candidate cells for a transplantation has a significant impact on the effectiveness of the transplantation. It indicates that it is very important to accurately identify the LSCs. To date, several putative biomarkers of LSCs have been widely reported, whereas their specificity is controversial. As reported, the identification of LSCs is based on the characteristics of stem cells, such as a nuclear-to-cytoplasm ratio (N/C) ≥ 0.7, label-retaining, and side population (SP) phenotype. Here, we review recently published data to provide an insight into the circumstances in the study of LSC biomarkers. The particularities of limbus anatomy and histochemistry, the limits of the current technology level for LSC isolation, the heterogeneity of LSCs and the influence of enzyme digestion are discussed. Practical approaches are proposed in order to overcome the difficulties in basic and applied research for LSC-specific biomarkers.

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Section: Identification Of Lscsmentioning

confidence: 99%

Section: Identification Of Lscsmentioning

confidence: 99%

An Insight into the Difficulties in the Discovery of Specific Biomarkers of Limbal Stem Cells

Guo

Zhang

Jia

et al. 2018

IJMS

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“…There have therefore been a number of recent marker-discovery models demonstrating ways in which a more representative LESC pool may be enriched and isolated for study. One such strategy is laser capture microdissection (LCM), in which cells can be selectively removed from tissue section based on features like size and position, providing an enriched pool which can be far more informative for downstream analysis (Bath et al, 2013;Kasinathan et al, 2016;Menzel-Severing et al, 2018;Polisetti et al, 2016). Another approach has been to purify a slow-cycling population of limbal epithelial cells using an inducible transgenic "pulse-chase" murine model, wherein the retention of a GFP label identifies quiescent cells within the tissue for co-expression studies and fluorescenceactivated cell sorting (FACS) for transcriptomic analysis (Sartaj et al, 2017).…”

Section: Targeting the Right Populationmentioning

confidence: 99%

The limbus: Structure and function

Seyed-Safi

Daniels²

2020

Experimental Eye Research

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Limbal function is a key determinant of corneal epithelial integrity. Lineage tracing studies in mice have highlighted that the centripetal movement of epithelial progenitors from the limbus drives both the steady-state maintenance of the corneal epithelium and its regeneration following injury. It is well established that this is facilitated by a population of limbal epithelial stem cells within the limbus. It is becoming increasingly apparent that the behaviour of these stem cells and their ability to respond to the needs of the tissue are closely linked to their immediate microenvironment -the stem cell niche. Increasing understanding of the structural features of this niche and the signalling networks that they coordinate is required to enhance the therapeutic application of these cells in the treatment of limbal stem cell deficiency. Importantly, an improved characterisation of the hierarchy of limbal epithelial progenitors using both new and old putative markers will enable a greater appreciation for the effects of many of these limbal niche factors on stem cell fate.

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“…In our previous study, CESCs have been enriched to 80% using a two-step protocol 8 and compared to differentiated central corneal epithelial cells by small RNA sequencing. Six miRNAs- hsa-miR-3168, hsa-miR-21-5p, hsa-miR-143-3p, hsa-miR-150-5p, hsa-miR-10a-5p and hsa-miR-1910-5p were identified to be highly expressed in the enriched CESCs and validated through qPCR.…”

Section: Introductionmentioning

confidence: 99%

Hsa-miR-143-3p inhibits Wnt-β-catenin and MAPK signaling in human corneal epithelial stem cells

Kalaimani

Devarajan²,

Namperumalsamy

et al. 2022

Sci Rep

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Our previous study demonstrated hsa-miR-143-3p as one of the highly expressed miRNAs in enriched corneal epithelial stem cells (CESCs). Hence this study aims to elucidate the regulatory role of hsa-miR-143-3p in the maintenance of stemness in CESCs. The target genes of hsa-miR-143-3p were predicted and subjected to pathway analysis to select the targets for functional studies. Primary cultured limbal epithelial cells were transfected with hsa-miR-143-3p mimic, inhibitor or scrambled sequence using Lipofectamine 3000. The transfected cells were analysed for (i) colony forming potential, (ii) expression of stem cell (SC) markers/ transcription factors (ABCG2, NANOG, OCT4, KLF4, ΔNp63), (iii) differentiation marker (Cx43), (iv) predicted five targets of hsa-miR-143-3p (DVL3, MAPK1, MAPK14, KRAS and KAT6A), (v) MAPK signaling regulators and (vi) Wnt-β-catenin signaling regulators by qPCR, immunofluorescence staining and/or Western blotting. High expression of hsa-miR-143-3p increased the colony forming potential (10.04 ± 1.35%, p < 0.001) with the ability to form holoclone-like colonies in comparison to control (3.33 ± 0.71%). The mimic treated cells had increased expression of SC markers but reduced expression of Cx43 and hsa-miR-143-3p targets involved in Wnt-β-catenin and MAPK signaling pathways. The expression of β-catenin, active β-catenin and ERK2 in hsa-miR-143-3p inhibitor transfected cells were higher than the control cells and the localized nuclear expression indicated the activation of Wnt and MAPK signaling. Thus, the probable association of hsa-miR-143-3p in the maintenance of CESCs through inhibition of Wnt and MAPK signaling pathways was thus indicated.

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A novel method for a high enrichment of human corneal epithelial stem cells for genomic analysis

Cited by 6 publications

References 25 publications

An Insight into the Difficulties in the Discovery of Specific Biomarkers of Limbal Stem Cells

An Insight into the Difficulties in the Discovery of Specific Biomarkers of Limbal Stem Cells

The limbus: Structure and function

Hsa-miR-143-3p inhibits Wnt-β-catenin and MAPK signaling in human corneal epithelial stem cells

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