Bladder tissue formation from cultured bladder urothelium

Oottamasathien, Siam; Williams, Karin; Franco, Omar E.; Thomas, John C.; Saba, Katrina; Bhowmick, Neil A.; Staack, Andrea; DeMarco, Romano T.; Brock, John W.; Hayward, Simon W.; Pope, John C.

doi:10.1002/dvdy.20886

Cited by 22 publications

(15 citation statements)

References 30 publications

(49 reference statements)

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“…Under the influence of preputial gland mesenchyme, bladder epithelia retained its urothelial phenotype and expressed Foxa1 (previously reported in adult bladder [30]), compared to adjacent foci of sebaceous epithelial cells that did not express Foxa1, confirming the transformation of epithelia in those select regions (Fig. 6C, 6D).…”

Section: Resultssupporting

confidence: 82%

Lineage Enforcement by Inductive Mesenchyme on Adult Epithelial Stem Cells across Developmental Germ Layers

et al. 2009

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During development, cell differentiation is accompanied by the progressive loss of pluripotent gene expression and developmental potential, although de‐differentiation in specialized cells can be induced by reprogramming strategies, indicating that transdifferentiation potential is retained in adult cells. The stromal niche provides differentiating cues to epithelial stem cells (SCs), but current evidence is restricted to tissue types within the same developmental germ layer lineage. Anticipating the use of adult SCs for tissue regeneration, we examined if stroma can enforce lineage commitment across germ layer boundaries and promote transdifferentiation of adult epithelial SCs. Here, we report tissue‐specific mesenchyme instructing epithelial cells from a different germ layer origin to express dual phenotypes. Prostatic stroma induced mammary epithelia (or enriched Lin−CD29HICD24+/MOD mammary SCs) to generate glandular epithelia expressing both prostatic and mammary markers such as steroid hormone receptors and transcription factors including Foxa1, Nkx3.1, and GATA‐3. Array data implicated Hh and Wnt pathways in mediating stromal‐epithelial interactions (validated by increased Cyclin D1 expression). Other recombinants of prostatic mesenchyme and skin epithelia, or preputial gland mesenchyme and bladder or esophageal epithelia, showed foci expressing new markers adjacent to the original epithelial differentiation (e.g., sebaceous cells within bladder urothelium), confirming altered lineage specification induced by stroma and evidence of cross‐germ layer transdifferentiation. Thus, stromal cell niche is critical in maintaining (or redirecting) differentiation in adult epithelia. In order to use adult epithelial SCs in regenerative medicine, we must additionally regulate their intrinsic properties to prevent (or enable) transdifferentiation in specified SC niches. STEM CELLS 2009;27:3032–3042

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Section: Resultssupporting

confidence: 82%

Lineage Enforcement by Inductive Mesenchyme on Adult Epithelial Stem Cells across Developmental Germ Layers

et al. 2009

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“…Ultrastructural morphology showed microvilli in stratified urothelium and immunolabeled for cytokeratin 17, which confirmed successful urothelial cell culture. 30 Moreover, human J82 cells were used for examining whether activated NF-kB translocated to nucleus and affected COX-2 mRNA expression. Human J82 cells were cultured in Dulbecco's modified Eagle's medium Q16 (InvitroGen Corp., Carlsbad, CA) with 10% fetal bovine serum.…”

Section: Primary Urothelial Cell and Human J82 Cell Culturesmentioning

confidence: 99%

“…After the rat bladder was excised, a modified Roszell's procedure was performed. 29,30 The bladder mucosa was gently scraped from the muscle tissue. The bladder was immersed in 4 mL of 1% collagenase IV (Sigma-Aldrich) at 37 C on a shaker for 40 minutes.…”

Section: Primary Urothelial Cell and Human J82 Cell Culturesmentioning

confidence: 99%

“…The urothelial cells were plated at a cell density of 5 Â 10 6 cells/mL in Gibco keratinocyte serum-free medium Q15 (Life Technologies, Grand Island, NY). The culture was supplemented with 5 ng/mL epidermal growth factor, 100 U/mL penicillin, and 1 mg/mL streptomycin (Gibco) 30 for 48 hours. Ultrastructural morphology showed microvilli in stratified urothelium and immunolabeled for cytokeratin 17, which confirmed successful urothelial cell culture.…”

Section: Primary Urothelial Cell and Human J82 Cell Culturesmentioning

confidence: 99%

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Translocation of NF-κB and Expression of Cyclooxygenase-2 Are Enhanced by Ketamine-Induced Ulcerative Cystitis in Rat Bladder

Juan

Lee

Long

et al. 2015

The American Journal of Pathology

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“…We may postulate that the induction of the pseudostratified disposition of urothelial cells results from the achievement of the first step of horizontal development, which is promoted by the paracrine signals from BMCs. This hypothesis does not exclude the possibility of a sequential differentiation-specific growth factor release by the BMCs (DiSandro et al 1998, Oottamasathien et al 2006.…”

Section: Discussionmentioning

confidence: 86%

Maintenance of bladder urothelia integrity and successful urothelialization of various tissue-engineered mesenchymes in vitro

Bouhout

Tremblay²,

Bolduc

2015

In Vitro Cell.Dev.Biol.-Animal

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Tissue-engineering offers the opportunity to produce hybrid tissues in vitro. The induction of bladder urothelial cells (BUCs) differentiation in vitro has been assessed by several research groups to build bladder models for fundamental studies and clinical applications. However, BUC induction of advanced differentiation in culture remains a challenging task. To reach this goal, optimal culture conditions are required, notably the use of specific additives as well as proper mesenchymal support. The best positive control for BUCs functional state monitoring is native urothelium collected from healthy bladder samples. In order to establish the best culture conditions to maintain and promote BUC differentiated state, native urothelia were cultured on various mesenchymes. Native bladder mesenchymes were used as controls for the maintenance of native urothelia. Histological and ultrastructural analyses showed the necessity to have a cellularized mesenchyme for rapid formation of a pseudostratified urothelium, allowing apical membrane rearrangement of the superficial cells in culture. Taken together, the results strongly suggest that it is possible to conserve the integrity of urothelia in vitro and, thus, potentially use them for eventual clinical applications and pharmacological investigations.

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Bladder tissue formation from cultured bladder urothelium

Cited by 22 publications

References 30 publications

Lineage Enforcement by Inductive Mesenchyme on Adult Epithelial Stem Cells across Developmental Germ Layers

Lineage Enforcement by Inductive Mesenchyme on Adult Epithelial Stem Cells across Developmental Germ Layers

Translocation of NF-κB and Expression of Cyclooxygenase-2 Are Enhanced by Ketamine-Induced Ulcerative Cystitis in Rat Bladder

Maintenance of bladder urothelia integrity and successful urothelialization of various tissue-engineered mesenchymes in vitro

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