Figures and data
Culture of muscle layer-derived cells prepared from embryonic hindgut.
(A) Culture of muscle layer-derived cells prepared from embryonic hindgut with FBS free-media and substrates. (B) Long-term time-lapse imaging after seeding on Matrigel with Neurobasal media. The images show the ability of these cells to self-assemble at 0, 20, 40, 60, 80 and 100 hours taken from Movie 1. Scale bars: 100 µm in A, B.
Forming spheroids exhibited reiterated contractions.
(A) Clusters/spheroids on day 3, 5 and 7 exhibited periodic contractions. Graphs show contractions quantified by differences in the intensity of brightfield in sequential images. (B) Frequency of contractions of the cluster/spheroid on day 3-7 (N=day 3: 46, day 5: 35, day 7: 60). The number on each graph shows the average of contraction frequencies. Scale bars: 50 µm in A.
The cluster/spheroid is composed of ICCs internally and SMCs peripherally.
(A) Co-staining with anti-c-Kit- and αSMA antibodies. White arrowheads show co-expression of c-Kit and αSMA at Day 3. Yellow arrowheads indicate a cell expressing αSMA but not c-Kit at day 7. A diagram shows an image of cell arrangement (green: ICC, magenta: SMC) in the spheroid at day 7. (B) Cell morphology in the spheroid at day 6 revealed by RCAS-gapEGFP expression. (C) Staining of spheroids at day 5 with anti-N-cadherin antibody. A white arrowhead shows expression of N-cadherin. A yellow arrowhead shows a cell which does not express N-cadherin in the outer region of the spheroid. Scale bars: 30 µm in A-C, 10 µm in a.
Ca2+ imaging of the gut contractile organoid revealed intercellular synchronization.
(A) RCAS-GCaMP6s-P2A-mRuby3 plasmid. (B) Ca2+ imaging of gut contractile organoid during relaxation and contraction. Ca2+ dynamics (green) and contraction (grey) of gut contractile organoid. (C) Simultaneous measurement of intercellular Ca2+ dynamics between ICC-ICC, SMC-SMC or ICC-SMC. Three or two ROIs with Ca2+ signal-positive cells were set in a single organoid. Graphs show Ca2+ dynamics in the ROIs. Magnified view shows that a rise of Ca2+ signal in ICC (green) preceded that in SMC (magenta). Scale bar: 50 µm in B.
Gap junction inhibitor exerted limited effects on the synchronization of Ca2+ dynamics.
GCaMP6s-expressing organoids were cultured with CBX, and three or two ROIs were assessed for their Ca2+ synchronization. A single organoid was subjected to the assessment before (0 µM; control) and after administrations of 100 µM CBX. The synchronization was unaffected between (A) SMC-SMC and (B) ICC-ICC, but that in (C) ICC-SMC was partially affected. Magnified view shows that the preceding rise of Ca2+ in ICC (green) before CBX was abrogated after CBX. Scale bar: 50 µm in A.
The organoidal contraction is important for Ca2+ dynamics in ICCs.
GCaMP6s-expressing organoids were cultured with Blebbistatin. (A) Ca2+ oscillation was extinguished in the entire organoid by administration of Blebbistatin. (B-D) Ca2+ dynamics in (B) SMC-SMC, (C) ICC-ICC and (D) ICC-SMC. Three or two ROIs were assessed for their Ca2+ synchronization. A single organoid was subjected to the assessment before (0 µM; control) and after administrations of 10 µM Blebbistatin. (E) Ca2+ transients in a single ICC in 0 μM, 5 μM, and 10 μM. Scale bar: 50 µm in B.
Ca2+ dynamics in multiple gut contractile organoids undergo synchronization upon their fusion.
(A) Time-lapse imaging of organoidal fusion. (B) When two organoids that originally showed independent rhythm of Ca2+ fused to each other, their rhythm became synchronized after fusion (24 h). (C) Protrusions between two neighboring organoids. White arrowheads show three protrusions from the left organoid. Scale bars: 100 µm in A-C, 20 µm in a.
Smooth muscle cells mediate the Ca2+ synchronization between organoids.
(A) Diagram of 3-well hydrogel in which an organoid placed in each well. This gel mold does not allow organoidal bodies to fuse to each other, but allow them to extend/migrate protrusions/cells through a narrow channel connecting the wells (B). (C) After 3 days, three organoids displayed synchronization of Ca2+ dynamics. (D) Some organoid-derived cells crawled out from the wells and covered the top surface of the hydrogel, resulting in bridging the three unfused organoids. (E) Diagram of 3-well hydrogel without channels (F) Surface-covering cells were SMCs (αSMA positive and c-Kit-negative). (G) In the hydrogel without channels but with surface-covered SMCs, Ca2+ dynamics in the 3 organoids were synchronized. (H) The Ca2+ synchronization shown in (G) was not altered by 18β-GA. Scale bars: 50 µm in B, 100 µm in C-H.
(A) Chicken embryonic hindgut at E15. The hindgut was dissected from the bottom of the cecum to the front of the cloaca (white lines). (B) Three layers of E15 hindgut: serosa, muscle layer, intestinal epithelium. Remak’s ganglion was also removed. Scale bars: 1 mm in A, B
(A) Co-staining of Day 7 organoids with anti-c-Kit- and Tuj1 antibodies. White arrowhead shows a Tuj1+ cell. (B) Representation of Tuj1+ cells in an organoid at day 7. Scale bar: 30 µm in A.
(A) Day 7 organoid exhibited periodic contractions both before (0 µM; control) and after adding CBX. Graphs show contractions quantified by the difference in intensity of brightfield in sequential images. (B) Relative changes to the control in contraction frequency in day 7 organoid after CBX. The number is an average. Scale bar: 50 µm in A.
