Evaluation of variability in human kidney organoids

Phipson, Belinda; Er, Pei X.; Combes, Alexander N.; Forbes, Thomas A.; Howden, Sara E.; Zappia, Luke; Yen, Hsan Jan; Lawlor, Kynan T.; Hale, Lorna J; Sun, Jing; Wolvetang, Ernst J.; Takasato, Minoru; Oshlack, Alicia; Little, Melissa H.

doi:10.1038/s41592-018-0253-2

Cited by 190 publications

(175 citation statements)

References 45 publications

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“…1C, Supplementary Fig. 2), were found in D29 organoids, including melanoma-like cells (PMEL), SOX2-positive(+) neuronal precursors, STMN2+ neuron-like cells, and MYOG+ muscle-like cells, as reported previously (Phipson et al, 2019;Wu et al, 2018). A rare population of endothelial cells was also observed ( Fig.…”

Section: Mature Organoids From All Ipsc Lines Contain Predominant Nepsupporting

confidence: 84%

“…To harness the full potential of iPSC derived kidney organoid technology, we must address critical unsolved questions about their reproducibility, faithfulness, and quality. First, we must establish organoid reproducibility: the comparability and range of variability in cellular composition and state between different iPSC lines from normal individuals across replicates and protocols (building on previous efforts to draw comparisons between iPSC and embryonic stem cell (ESC) derived organoids (Wu et al, 2018) or bulk RNASeq data comparing iPSC derived organoids (Phipson et al, 2019)). This is critically important, because individual patient iPSCs offer significant advantages over ESCs for precision medicine and drug development projects (Boreström et al, 2018;Burrows et al, 2016;Takasato et al, 2016b).…”

Section: Introductionmentioning

confidence: 99%

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Kidney organoid reproducibility across multiple human iPSC lines and diminished off target cells after transplantation revealed by single cell transcriptomics

Subramanian

Sidhom

Emani

et al. 2019

Preprint

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Human iPSC-derived kidney organoids have the potential to revolutionize discovery, but assessing their consistency and reproducibility across iPSC lines, and reducing the generation of off-target cells remain an open challenge. Here, we used single cell RNA-Seq (scRNA-Seq) to profile 415,775 cells to show that organoid composition and development are comparable to human fetal and adult kidneys. Although cell classes were largely reproducible across iPSC lines, time points, protocols, and replicates, cell proportions were variable between different iPSC lines. Off-target cell proportions were the most variable. Prolonged in vitro culture did not alter cell types, but organoid transplantation under the mouse kidney capsule diminished offtarget cells. Our work shows how scRNA-seq can help score organoids for reproducibility, faithfulness and quality, that kidney organoids derived from different iPSC lines are comparable surrogates for human kidney, and that transplantation enhances their formation by diminishing off-target cells.

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Section: Mature Organoids From All Ipsc Lines Contain Predominant Nepsupporting

confidence: 84%

Section: Introductionmentioning

confidence: 99%

Kidney organoid reproducibility across multiple human iPSC lines and diminished off target cells after transplantation revealed by single cell transcriptomics

Subramanian

Sidhom

Emani

et al. 2019

Preprint

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“…Multiple stromal populations were also identified, which expressed collagens COL1A1 and COL3A1, as well as kidney stromal markers DCN and CXCL12. We note the apparent absence of an endothelial cluster in this dataset, despite clear evidence for this cell type in previous studies [19][20][21], including in bioprinted organoids [preprint: 15].…”

Section: Single-cell Rnaseq Of Kidney Organoids Reveals Widespread Sicontrasting

confidence: 62%

Reporter‐based fate mapping in human kidney organoids confirms nephron lineage relationships and reveals synchronous nephron formation

et al. 2019

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Nephron formation continues throughout kidney morphogenesis in both mice and humans. Lineage tracing studies in mice identified a self‐renewing Six2‐expressing nephron progenitor population able to give rise to the full complement of nephrons throughout kidney morphogenesis. To investigate the origin of nephrons within human pluripotent stem cell‐derived kidney organoids, we performed a similar fate‐mapping analysis of the SIX2‐expressing lineage in induced pluripotent stem cell (iPSC)‐derived kidney organoids to explore the feasibility of investigating lineage relationships in differentiating iPSCs in vitro. Using CRISPR/Cas9 gene‐edited lineage reporter lines, we show that SIX2‐expressing cells give rise to nephron epithelial cell types but not to presumptive ureteric epithelium. The use of an inducible (CreERT2) line revealed a declining capacity for SIX2+ cells to contribute to nephron formation over time, but retention of nephron‐forming capacity if provided an exogenous WNT signal. Hence, while human iPSC‐derived kidney tissue appears to maintain lineage relationships previously identified in developing mouse kidney, unlike the developing kidney in vivo, kidney organoids lack a nephron progenitor niche capable of both self‐renewal and ongoing nephrogenesis.

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“…Our TLS already display remarkable reproducibility both at 166 the morphological and molecular level. Nevertheless, we realize the importance of further 167 integrated comparative analysis of single TLS at single-cell resolution, such as recently 168 published for brain and kidney organoids 37,38 . Finally, in vivo somites are formed in a rhythmic 169 process involving an oscillator -the segmentation clock 39 .…”

mentioning

confidence: 98%

Mouse embryonic stem cells self-organize into trunk-like structures with neural tube and somites

Veenvliet

Bolondi

Kretzmer

et al. 2020

Preprint

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One sentence summary: A platform for generating trunk-like-structures with precursors of spinal cord, bone and muscle from stem cells in a dish Abstract: Post-implantation embryogenesis is a highly dynamic process comprising multiple lineage decisions and morphogenetic changes inaccessible to deep analysis in vivo. Mouse embryonic stem cells (mESCs) can form aggregates reflecting the post-occipital embryo (gastruloids), but lacking proper morphogenesis. Here we show that embedding of aggregates derived from mESCs in an extracellular matrix compound results in Trunk-Like-Structures (TLS) with a high level of organization comprising a neural tube and somites. Comparative single-cell RNA-seq analysis demonstrates that TLS execute gene-regulatory programs in an embryo-like order, and generate primordial germ cell like cells (PGCLCs). TLS lacking Tbx6 form ectopic neural tubes, mirroring the embryonic mutant phenotype. ESC-derived trunk-like structures thus constitute a novel powerful in vitro platform for investigating lineage decisions and morphogenetic processes shaping the post-implantation embryo.2 Vertebrate post-implantation development comprises a multitude of complex morphogenetic 1 processes, which result from self-organization of stem cells and their descendants shaping the 2 embryonic body plan 1 . Recently developed stem cell models represent powerful platforms for 3 deconstructing the dynamics of these processes that are inaccessible in the embryo 1, 2 . The 4 most advanced models in terms of developmental stage accomplished so far are gastruloids 2,3 , 5 aggregates of mESCs able to self-organize into the three body axes 3 . However, gastruloids lack 6 proper morphogenesis, such as a failure of neural tube formation from neural cells or somite 7 condensation from presomitic cells 3 . In vivo, the extracellular matrix (ECM) has a critical role in 8 tissue morphogenesis 4 . In vitro, matrigel can serve as ECM surrogate, and culture media 9 supplemented with a low percentage of matrigel have been shown to induce complex 10 morphogenesis in organoids 5 . 11We therefore explored if embryo-like morphogenetic features could be induced by 12 embedding 96h post aggregation gastruloids in 5% matrigel for an additional 24h period ( Fig. 13 1a). We also tested a combination of matrigel together with the WNT signaling activator 14 CHIR99021 (CHIR) and the BMP signaling inhibitor LDN193189 (LDN), that have been reported 15 to induce a (pre-)somitic mesoderm ((P)SM) fate in 2D and 3D differentiation protocols 6-8 . To 16 facilitate high-throughput characterization and quantification of our conditions, we generated 17 mESCs with T::H2B-mCherry (hereafter T mCH ) and Sox2::H2B-Venus (hereafter Sox2 VE ) reporters, 18 marking the mesodermal (ME) or neural (NE) lineage respectively (Extended Data Fig. 1a). 19 Strikingly, embedding in 5% matrigel alone was sufficient for segmentation in the T mCH+ ME 20 domain and formation of a Sox2 VE+ neural tube like structure ( Fig. 1b,d; Extended Data Fig. 21 1b,c). The vast majorit...

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Evaluation of variability in human kidney organoids

Cited by 190 publications

References 45 publications

Kidney organoid reproducibility across multiple human iPSC lines and diminished off target cells after transplantation revealed by single cell transcriptomics

Kidney organoid reproducibility across multiple human iPSC lines and diminished off target cells after transplantation revealed by single cell transcriptomics

Reporter‐based fate mapping in human kidney organoids confirms nephron lineage relationships and reveals synchronous nephron formation

Mouse embryonic stem cells self-organize into trunk-like structures with neural tube and somites

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