Intracameral Microimaging of Maturation of Human iPSC Derivatives into Islet Endocrine Cells

Zhao, Kaixuan; Shi, Yue; Yu, Jia; Yu, Lina; Mael, Amber A.; Li, Yuxin; Kolton, Anthony; Joyce, Thomas; Odorico, Jon S.; Berggren, Per Olof; Yang, Shao‐Nian

doi:10.1177/09636897211066508

Cited by 5 publications

(9 citation statements)

References 49 publications

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“…The procedure has been described elsewhere [ 5 , 19 ]. In brief, the undifferentiated hiPSC line NCRM-1 (Lonza/NIH, Walkersville, MD, USA) was cultured in mTeSR1 medium (Stem Cell Technologies, Vancouver, BC, Canada) on Growth Factor Reduced Matrigel (Corning, Corning, NY, USA) for 3–4 days at 37 °C in a humidified 5% CO 2 incubator.…”

Section: Methodsmentioning

confidence: 99%

“…At the end of the six-stage induction, cells were removed from the Transwell culture plates, resized and placed into Ultra Low Attachment flasks (Corning) in suspension as stage seven for eight days. Upon completion of stage seven, the resulting hiPSC-islets were obtained for in vitro quality testing and intraocular transplantation [ 5 , 19 ]. All reagents were purchased from R&D Systems (Minneapolis, MN, USA) unless otherwise stated.…”

Section: Methodsmentioning

confidence: 99%

“…Human-induced pluripotent stem cells (hiPSCs) have successfully been used to produce spherical aggregates of islet hormone-producing cells, referred to here as hiPSC-islets, through in vitro cultivation [ 1 , 2 , 3 , 4 , 5 , 6 ]. However, clinical hiPSC-islet transplantation as a curative treatment for diabetes still remains challenging because hiPSC-islets cannot fully mature in vitro into glucose-responsive insulin-secreting islets and may reliably achieve functional maturation post-transplantation [ 1 , 3 , 6 , 7 , 8 , 9 , 10 , 11 ].…”

Section: Introductionmentioning

confidence: 99%

“…However, it has not been possible to retrieve single, intact hiPSC-islet grafts, and thus, [Ca 2+ ] i dynamics could not be directly measured in these grafts without losing their in vivo gained phenotypes. This inspired us to exploit the anterior chamber of the eye (ACE) of immunodeficient mice, which has been used as a reliable transplantation site for hiPSCs and their derivative [ 5 , 19 , 20 , 21 , 22 ]. The ACE is filled with aqueous humor endowed with high oxygen and less stress and may serve as a unique niche for the in vivo maturation of single, non-aggregated hiPSC-islet grafts.…”

Section: Introductionmentioning

confidence: 99%

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In Vivo CaV3 Channel Inhibition Promotes Maturation of Glucose-Dependent Ca2+ Signaling in Human iPSC-Islets

Zhao

Shi

et al. 2023

Biomedicines

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CaV3 channels are ontogenetically downregulated with the maturation of certain electrically excitable cells, including pancreatic β cells. Abnormally exaggerated CaV3 channels drive the dedifferentiation of mature β cells. This led us to question whether excessive CaV3 channels, retained mistakenly in engineered human-induced pluripotent stem cell-derived islet (hiPSC-islet) cells, act as an obstacle to hiPSC-islet maturation. We addressed this question by using the anterior chamber of the eye (ACE) of immunodeficient mice as a site for recapitulation of in vivo hiPSC-islet maturation in combination with intravitreal drug infusion, intravital microimaging, measurements of cytoplasmic-free Ca2+ concentration ([Ca2+]i) and patch clamp analysis. We observed that the ACE is well suited for recapitulation, observation and intervention of hiPSC-islet maturation. Intriguingly, intraocular hiPSC-islet grafts, retrieved intact following intravitreal infusion of the CaV3 channel blocker NNC55-0396, exhibited decreased basal [Ca2+]i levels and increased glucose-stimulated [Ca2+]i responses. Insulin-expressing cells of these islet grafts indeed expressed the NNC55-0396 target CaV3 channels. Intraocular hiPSC-islets underwent satisfactory engraftment, vascularization and light scattering without being influenced by the intravitreally infused NNC55-0396. These data demonstrate that inhibiting CaV3 channels facilitates the maturation of glucose-activated Ca2+ signaling in hiPSC-islets, supporting the notion that excessive CaV3 channels as a developmental error impede the maturation of engineer ed hiPSC-islet insulin-expressing cells.

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Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

In Vivo CaV3 Channel Inhibition Promotes Maturation of Glucose-Dependent Ca2+ Signaling in Human iPSC-Islets

Zhao

Shi

et al. 2023

Biomedicines

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“…For example, an adenoviral calcium biosensor, GCaMP6m, has been used to infect human islets transplanted into the ACE of immunocompromised mice, demonstrating that islet calcium dynamics were functionally conserved ( 20 ). Also, once the animal is being imaged, injection of various treatments and probes may be employed to study beta cell biology during imaging, such as injection of a vasculature dye or cell death marker ( 21 ). Aside from using islets isolated from cadaveric donors, human induced pluripotent stem cells (hiPSCs) can be differentiated in vitro into islet-like structures for transplantation purposes, potentially reducing the burden to obtain human tissue for future studies ( 21 ), making exciting future discoveries using these cells possible.…”

Section: Transplantation Sites For Fluorescent Imaging Purposesmentioning

confidence: 99%

Mouse models and human islet transplantation sites for intravital imaging

et al. 2022

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Human islet transplantations into rodent models are an essential tool to aid in the development and testing of islet and cellular-based therapies for diabetes prevention and treatment. Through the ability to evaluate human islets in an in vivo setting, these studies allow for experimental approaches to answer questions surrounding normal and disease pathophysiology that cannot be answered using other in vitro and in vivo techniques alone. Intravital microscopy enables imaging of tissues in living organisms with dynamic temporal resolution and can be employed to measure biological processes in transplanted human islets revealing how experimental variables can influence engraftment, and transplant survival and function. A key consideration in experimental design for transplant imaging is the surgical placement site, which is guided by the presence of vasculature to aid in functional engraftment of the islets and promote their survival. Here, we review transplantation sites and mouse models used to study beta cell biology in vivo using intravital microscopy and we highlight fundamental observations made possible using this methodology.

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Generation and application of novel hES cell reporter lines for the differentiation and maturation of hPS cell-derived islet-like clusters

Zanfrini,

Bandral,

Jarc

et al. 2024

Sci Rep

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The significant advances in the differentiation of human pluripotent stem (hPS) cells into pancreatic endocrine cells, including functional β-cells, have been based on a detailed understanding of the underlying developmental mechanisms. However, the final differentiation steps, leading from endocrine progenitors to mono-hormonal and mature pancreatic endocrine cells, remain to be fully understood and this is reflected in the remaining shortcomings of the hPS cell-derived islet cells (SC-islet cells), which include a lack of β-cell maturation and variability among different cell lines. Additional signals and modifications of the final differentiation steps will have to be assessed in a combinatorial manner to address the remaining issues and appropriate reporter lines would be useful in this undertaking. Here we report the generation and functional validation of hPS cell reporter lines that can monitor the generation of INS+ and GCG+ cells and their resolution into mono-hormonal cells (INSeGFP, INSeGFP/GCGmCHERRY) as well as β-cell maturation (INSeGFP/MAFAmCHERRY) and function (INSGCaMP6). The reporter hPS cell lines maintained strong and widespread expression of pluripotency markers and differentiated efficiently into definitive endoderm and pancreatic progenitor (PP) cells. PP cells from all lines differentiated efficiently into islet cell clusters that robustly expressed the corresponding reporters and contained glucose-responsive, insulin-producing cells. To demonstrate the applicability of these hPS cell reporter lines in a high-content live imaging approach for the identification of optimal differentiation conditions, we adapted our differentiation procedure to generate SC-islet clusters in microwells. This allowed the live confocal imaging of multiple SC-islets for a single condition and, using this approach, we found that the use of the N21 supplement in the last stage of the differentiation increased the number of monohormonal β-cells without affecting the number of α-cells in the SC-islets. The hPS cell reporter lines and the high-content live imaging approach described here will enable the efficient assessment of multiple conditions for the optimal differentiation and maturation of SC-islets.

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Intracameral Microimaging of Maturation of Human iPSC Derivatives into Islet Endocrine Cells

Cited by 5 publications

References 49 publications

In Vivo CaV3 Channel Inhibition Promotes Maturation of Glucose-Dependent Ca2+ Signaling in Human iPSC-Islets

In Vivo CaV3 Channel Inhibition Promotes Maturation of Glucose-Dependent Ca2+ Signaling in Human iPSC-Islets

Mouse models and human islet transplantation sites for intravital imaging

Generation and application of novel hES cell reporter lines for the differentiation and maturation of hPS cell-derived islet-like clusters

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