SUSPENSION-BASED 3D CULTURE METHOD FOR ORGANOIDS

Abstract

Hybrid suspension cultures supplementing soluble extracellular matrix (ECM) for growth of organoids is disclosed. Viable lung organoid from epithelial, endothelial, and fibroblast human stable cell lines in suspension culture are also disclosed.

Description

TECHNICAL FIELD

The present disclosure relates to organotypic structures from stable cell lines that form in hybrid suspension cultures via supplementation of soluble extracellular matrix.

BACKGROUND

The extracellular matrix (ECM) is classically known for its roles in cell anchorage and mechanical signaling in organs. The role of ECM as an anchor is important in modulating organogenesis, cell differentiation, cell survival, and metabolism. These ECM characteristics have been exploited by tissue engineers to recreate tissue- and organ-like 3-dimensional (3D) biological materials essential for disease modeling and regenerative medicine. The tunability of ECM stiffness affects stem cell differentiation. The roles of ECM as a soluble supplement, however, are rarely studied and not well defined.

The majority of 3D culture techniques can be broken down into two categories: solid scaffold using some type of ECM or ECM-like synthetic materials and scaffold free, no ECM-like scaffolds. Both culture techniques have advantages and disadvantages.

In tissue engineering, the use of gelled ECM or other solid ECM-like polymers are prevalent in the construction of organotypic structures. Scaffold-based cultures mimic the presence of a solid ECM akin to that of native organ tissue. By this, the cells are provided with a substrate for organotypic attachment leading to biochemical signaling. The ECM has both constructive and instructive roles in tissues and organs. In several stem cell-based approaches, cell clusters are embedded in solid ECM scaffolds to encourage organotypic formation. Some obstacles in solid scaffold-based cultures include slow formation of tissues, inconsistent growth of aggregates, difficult recovery, and high contamination for downstream analyses.

Scaffold-free techniques, on the other hand, often use forced aggregation of cells on ultra-low attachment surfaces and rely on self-patterning of tissue to create consistently sized, reproducible multicellular aggregates. Due to high initial local cell concentration, self-assembly into tissue-like structures is relatively faster than scaffold-based methods. This characteristic gives scaffold-free technique an edge for being used in downstream high-throughput experiments. The use of scaffold-free force aggregated cultures, however, is limited to creating tissue-like structures. The lack of organotypic structures is attributed to lack of organ-like ECM during self-patterning.

Researchers have struggled to produce organotypic models from stable cell lines. There are several definitions given for organoids in the literature. The prevailing definition focuses on stem cell differentiation and self-patterning of stem-derived cells while embedded in ECM with the idea that stable and mature cells lines do not self-pattern as well into organ-like structures nor give rise to other cell types.

There remains, therefore, a need in the art to provide alternative media and growth factors for organictypic structures and organoids in cell cultures. Moreover, there is an unmet need to understand the pathogenesis of PF in human lung cells and tissue via 3D modeling.

BRIEF SUMMARY

In one aspect, a cell culture for obtaining an organoid is disclosed. The cell culture includes epithelial cells or tissue fragments comprising the epithelial cells, endothelial cells or tissue fragments comprising the endothelial cells, fibroblast cells or tissue fragments comprising the fibroblast cells, and soluble, non-gelling concentration of extracellular matrix proteins.

In another aspect, an in vitro method for obtaining an organoid is disclosed. The method includes culturing a mixture of (a) epithelial cells or tissue fragments comprising the epithelial cells, (b) endothelial cells or tissue fragments comprising the endothelial cells, (c) fibroblast cells or tissue fragments comprising the fibroblast cells, and (d) soluble extracellular matrix proteins.

In one embodiment, an organoid obtained by the methods disclosed is obtained. In one embodiment, the epithelial cells are A549. In one embodiment, the endothelial cells are EAhy. In one embodiment, the fibroblast cells are HFL1. In one embodiment, the culture further includes basement membrane proteins.

DESCRIPTION OF THE DRAWINGS

A detailed description of the invention is hereafter provided with specific reference being made to the drawings in which:

FIGS. 1A-1F depict Alveolar-like lumen structure formation of an embodiment.

(FIG. 1A) Representative bright-field images of 3D cell aggregates after 14 days of culture. Scale bars, 300 μm

(FIG. 1B) Effect of soluble ECM in aggregate density. Line profile analysis at the major axis of the aggregates expressed as normalized grey value. Lines indicate the grey value range at the specific normalized distance from the center.

(FIG. 1C) Live 3D fluorescence confocal image (single z-section) showing the self-organized localization of the three cell lines—A549 (green), EAHy (blue), and HFL1 (magenta). In aggregates grown using 300 μg mL⁻¹ Matrigel, organotypic structures such as the lumina (*) and endothelial networks (arrow) are indicated. Scale bars, 200 μm

(FIG. 1D) Hematoxylin and Eosin staining of the aggregates showing that the lumen formation in 300 μg mL⁻¹ Matrigel aggregates is comparable to the mammalian lung parenchyma. Scale bars, 300 μm for full image; 50 μm for inset. Lumen formation is quantified using number of lumen normalized to aggregate size and percent lumen area. Bar colors are indicated in the micrographs above. Mean, individual measurements, and standard deviation are shown. Three independent cell aggregates and lungs from two mice and one pig were used. **P<0.01, ns (P>0.05) determined by One-way ANOVA with Welch's correction.

(FIG. 1E) Fluorescence confocal images (maximum projection) showing localization of epithelial cells (EPCAM, green) and mesenchymal cells (Vimentin, magenta) relative to the lumen. Specific alveolar epithelial subtypes: Type I (Podoplanin, red) and Type II (prosurfactant protein C, blue). Scale bars, 50 μm

(FIG. 1F) Transmission electron microscopy of cell aggregates showing stratification and lumen formation in 300 μg mL⁻¹ Matrigel aggregates. Alveolar type II-like epithelial cells (AT2L) shown with their lamellar body-like inclusions (LBL) and microvilli (mv). Other features include: thin, alveolar type I-like cells (AT1L), a luminal structure, presence of a basement membrane (BM), and luminal endothelial cells (LEC). Scale bars, 3 μm for full images; 500 nm for zoomed images.

FIGS. 2A-2F depict 3D aggregate growth and cell survival of an embodiment.

(FIG. 2A) Bright-field images of 3D cell aggregates during the 14-day culture. Scale bar, 300 μm

(FIG. 2B) Line graph showing change in aggregate area. Areas were normalized to their respective day 1 area. Means and standard deviation are shown. Individual line indicates independent experiments performed by independent researchers. N=10 independently sampled aggregates on each measured day.

(FIG. 2C) Cell counts at day 14-fold change from day 0 seeding density. Means, individual values, and standard deviation are shown. 3 independent experiments were performed with >3 cell aggregates used; N=12 aggregates. ****P<0.0001 determined by two-tailed t-test with Welch's correction.

(FIG. 2D) Hematoxylin and Eosin staining of cell aggregates showing stability of lumen structure in hFLO (up to 70 days of culture) as quantified using lumen area and count. Mean, individual values, and standard deviation are shown. ****P<0.0001 determined using two-tailed t-test with Welch's correction using values from n=27 independent aggregates.

(FIG. 2E) Cell population composition at days 3, 7, and 14 of culture; n=7 independently sampled aggregates. **P<0.01, ***P<0.001 determined using One-way ANOVA with Welch's correction comparing day 14 to day 3 values.

(FIG. 2F) Expression of cleaved caspase 3 of day 14 cell aggregates using imaging flow cytometry. Three independent plates (around 200 cell aggregates) were used and an unstained control from pooled samples was used as a negative gating control. Left bar plot shows percent positive cells with mean, individual points, and standard deviation indicated. Right bar plot shows mean intensities found in each of the samples. ***P<0.001 determined using two-tailed t-test with Welch's correction.

FIGS. 3A-3F depict Vascular endothelial branching of an embodiment.

(FIG. 3A) Live fluorescence confocal images (maximum projection) of day 14 cell aggregates showing EAHy (endothelial, blue) and HFL1 (magenta). Scale bars, 100 μm

(FIG. 3B) AngioTool outputs characterizing the abundance and branching of the EAhy-HFL1 networks. We used 8 independent aggregates per condition. **P<0.01, ***P<0.001, ****P<0.0001 determined using two-tailed t-test with Welch's correction.

(FIG. 3C) Fluorescence confocal images (maximum projections) of day 14 hFLO showing the presence of vascular cells including endothelial-like (UEA1 lectin), smooth muscle-like (αSMA), and pericyte-like (PDGFRβ) cells.

(FIG. 3D) Another perivascular marker, desmin was detected in day 14 hFLO. DAPI was used as the nuclear stain. Scale bars, 100 μm

(FIG. 3E) Volumetric analyses of UEA1, αSMA, PDGFRβ, and desmin in FA and hFLO aggregates normalized to DAPI volume. We used n=15 independent cell aggregates for UEA1, αSMA, and PDGFRβ, and n=4 independent cell aggregates for desmin. **P<0.01, ***P<0.001, ****P<0.0001 determined using two-tailed t-test with Welch's correction.

(FIG. 3F) Flow cytometric analysis of whole cell aggregates for expression of αSMA, PDGFRβ, and desmin in FA and hFLO. Contour plots show percent gated cells, contours, and outliers were indicated as dots. Three independent plates were used for each. Bar plots show means, individual points, and standard deviation from positive gates. *P<0.05, **P<0.01, ***P<0.001 determined using two-tailed t-test with Welch's correction.

FIGS. 4A-4G depict Shotgun proteomics.

(FIG. 4A) Principal component analysis plot of the first and second components. Dots represent the whole proteome of three independent samples used for FA aggregates (grey) and hFLO (pink). Grouping is highlighted using an enclosing oval.

(FIG. 4B) Volcano plot showing fold changes (log 2FC) of hFLO versus FA aggregates. P values were calculated using two-tailed t-tests with Welch's correction. Red points indicate proteins with P<0.01.

(FIG. 4C) Distribution of the differentially expressed proteins (DEPs, P<0.01).

(FIG. 4D) Gene set enrichment analysis (GSEA) plot of all proteins ranked based on enrichment score (Signal2Noise).

(FIG. 4E) Scatter plot of the top 50 GO-Terms enriched in hFLO. Dot size corresponds to number of genes annotated per term and color corresponds to the normalized enrichment score (NES).

(FIG. 4F) Scatter plot of the top 50 GO-Terms enriched in FA (negative enrichment in hFLO).

(FIG. 4G) GSEA enrichment plot for selected GO-Terms. Barcodes show individual proteins annotated in each GO-Term and their respective ranks based on enrichment of hFLO versus FA.

FIGS. 5A-5F depict Pre-clinical hFLO-bleomycin fibrotic model and resolution of fibrotic features using fasudil in an embodiment.

(FIG. 5A) Schematic diagram of the workflow showing aggregate formation and self-patterning for 7 days, induction of fibrosis using bleomycin (20 μg mL⁻¹) for 3 days, and antifibrotic trial using fasudil (10 μM). Dimethyl sulfoxide (DMSO) is the vehicle used for the bleomycin and fasudil.

(FIG. 5B) Histochemical and immunohistochemical analyses for the extent of induced fibrosis in the hFLO aggregates. Insets show fibroblastic foci for bleomycin-treated aggregates. Scale bars, 300 μm for full image; 60 μm for inset. Masson staining shows the extent of collagen deposition (blue). We used 9 independent aggregates per condition. Hematoxylin and DAB immunostaining (H-DAB) of pro-fibrotic markers αSMA, fibronectin, and PDGFRα, respectively. We used n=11, n=9, and n=9 independent aggregates per condition for H-DAB probing for αSMA, fibronectin, and PDGFRα, respectively.

(FIG. 5C) Histochemical and immunohistochemical image analyses. Bar graphs show means, individual values, and standard deviations are shown. *P<0.05, **P<0.01, ***P<0.001, ****P<0.0001 determined using One-way ANOVA with Welch's correction. Color legends shown in b.

(FIGS. 5D-5F) Cytokine array profiling the secreted factors from the treatment groups. Raw immunoblot intensity were normalized to internal positive and negative controls.

(FIG. 5D) Differentially secreted factors (P<0.05) were determined using two-tailed Welch's t-test with Benjamini-Hochberg FDR correction. Statistical tests were done comparing each group to each other. Venn diagram shows overlap among differentially secreted factors.

(FIG. 5E) Principal component analysis of the differentially secreted factors. Dots show media samples collected from the organoids and axes represent principal components (PC) 1, 2, and 3. Clustering among fasudil-treated and control samples is emphasized by the grey ellipse.

(FIG. 5F) Cluster heatmap (Euclidean) of the differentially secreted factors showing clustering of fasudil-treated and control samples, separate from bleomycin-treated samples. Known cytokine/chemokine effectors of angiogenesis and fibrosis are annotated. Cell color is based on row average-normalized z-scores.

FIGS. 6A-6H depict hypoxic vascularization using hFLO in an embodiment.

(FIG. 6A) Schematic diagram of the workflow showing further vascular growth using hypoxia and pro-angiogenic factors (top left). Bright-field images of aggregates at day 14 of culture (bottom left). vhFLO is hFLO grown under hypoxia for 7 days with supplementation of FGF2 and VEGF. Line profile analysis at the major axis of the aggregates expressed as normalized grey value. Effects of the hypoxic culture in aggregate density is shown using line profile analysis (right). Lines indicate the grey value range at the specific normalized distance from the center. Scale bar, 300 μm

(FIG. 6B) Aggregate area at day 14 of culture. 9 independent aggregates were measured for each condition. *P<0.05, **P<0.01 determined using One-way ANOVA with Welch's t-test.

(FIG. 6C) HFL1 (red), A549 (green), and EAhy (blue) cell population percent volume composition in hFLO and vhFLO. N=7 independent 3D live confocal images were used. **P<0.01 determined using two-tailed t-test with Welch's correction.

(FIG. 6D) Whole aggregate immunostaining of αSMA expression. Scale bar, 200 μm

(FIG. 6E) 3D fluorescence confocal image of vhFLO showing vascular-like formation and localization of endothelial-like (UEA1 lectin+, BLUE), pericyte-like (PDGFRβ+, yellow), and smooth muscle-like (αSMA+, red). 3D renderings highlight annular tube morphology typical of a vasculature. Scale bar, 50 μm

(FIG. 6F) Illustration of the vascular perfusion assay using dextran 70 kDa flown through a peristaltic pump system (top). The chip used for this assay is shown as a CAD render with fluidic flow indicated by arrows. Additional information can be found in Supplementary FIG. 10.

(FIG. 6G) Whole aggregate fluorescence confocal images (single z section) of A549 spheroid, FA, hFLO and vhFLO. Images show extent of dextran 70 kDa perfusion. Zoomed images showing dextran and azurite colocalization in vhFLO. Scale bars, 200 pm for full images; 50 μm for zoomed images.

(FIG. 6H) Volumetric analysis of extent of perfusion in the aggregates. A549 spheroid was used as a negative control. We used n=6 A549 spheroid, n=7 FA, n=15 hFLO, and n=11 vhFLO independent aggregates. ***p<0.001 determined using One-way ANOVA with Welch's t-test.

FIGS. 7A-7D deouct cell lines and depletion of NCad high population in A549 in an embodiment.

(FIG. 7A) 2D monocultures of EAhyAzurite, A549eGFP, and HFL1mCherry cells. Scale bars, 100 μm.

(FIG. 7B) 2D bicultures of A549 with EAhy (Left) or HFL1 (Middle); and 2D triculture of the cells (Right). Scale bar, 200 μm.

(FIG. 7C) FACS depletion of NCadherin+ cells in A549-eGFP to improve epithelial phenotype. Workflow for the purification (Left). NCad-AF647 intensity histogram (Middle) indicating NCadhigh population as gated. Delineating NCadherin high and low expressing populations (Right).

(FIG. 7D) These cells were then cultured and after 4 passages stained to confirm phenotypic stability from sorting. ECadherin+(CDH1) and NCadherin+ (CDH2) cells were counted from 15 fields of view and expressed as percent in a box plot.

FIGS. 8A-8C depict effects of ECM concentration in self patterning of an embodiment.

(FIG. 8A) Bright field images of tricultures grown embedded in gel ECM: 3 mg ml-1 collagen type I, 3 mg ml-1 Matrigel, and 4 mg ml-1 Matrigel. Scale bars, 300 μm

(FIG. 8B) Live 3D fluorescence confocal images (3D renders, tilted and top view) of the gel ECM cultures. Scale bars, 200 μm.

(FIG. 8C) Effect of collagen type I concentration in self-patterning. Vascular (endothelial-fibroblast) networks sprout from the compact core as shown in the bright field images (Top). Scale bars, 200 μm. Live 3D confocal images (maximum projection) of the cell aggregates. Scale bars, 100 μm.

FIGS. 9A-9B depict suspension culture for a lung organoid via triculture.

(FIG. 9A) Cell lines used in the 3D model: epithelial (A549-eGFP) and interstitial/vascular (HFL1-mCherry and EAhy-Azurite) in an embodiment. Timeline and culture workflow for culture with 300 μg mL-1 Matrigel and 0.024% methylcellulose (Bottom).

(FIG. 9B) A cartoon of the human fluorescent lung triculture organoid (hFLO) depicting suspension culture on ultra-low adherence (ULA) agarose U-bottom well (Left). Microscopic features of the hFLO showing epithelial cells forming septate airspace-like lumen, endothelial cells and fibroblasts interacting with each other in the interstitial spaces, and presence of ECM proteins in the organoids (Right).

FIGS. 10A-10C depict transmission electron microscopy of an embodiment.

(FIG. 10A) 7-day A549 spheroid cells showing the presence of lamellar body-like inclusions (LBL) typical of a type II-like alveolar cell (AT2L).

(FIG. 10B) 14-day FA aggregates also shown with the presence of LBL.

(FIG. 10C) Porcine lung alveolus showing AT2 cells and AT1 cytoplasmic extension and other features including lumina, basement membranes, EC, red blood cell (RBC), and lamellar bodies (LB). Scale bars as indicated in each pictograph.

FIGS. 11A-11E depict morphometric analysis of cell death using imaging flow cytometry in an embodiment.

(FIGS. 11A-11E) Brightfield images representing spheroids typical of high and low spectrums of respective morphological features. Histograms show distributions of respective features of a typical sample of FA and hFLO. Barplots display histogram statistics (left column) and means of feature values (right column). *p<0.05; **p<0.01; ****p<0.0001; Welch's t-test.

FIGS. 12A-12F depict Matrigel deposition in the aggregates of an embodiment.

(FIG. 12A) Immunoblot and ponceau staining using 3D media, hFLO media, and biotinylated Matrigel media (BTN-MAT).

(FIG. 12B) Representative fluorescence confocal images (maximum projection, Top; single z-section, Bottom) of hFLO at day 3 with normal matrigel media (Control) and biotinylated matrigel media (BTN-MAT). Scale bars, 100 μm.

(FIG. 12C) Volumetric quantification of biotinylated Matrigel localization in the aggregate normalized to nuclear volume (DAPI). 11 independently grown aggregates were used in the study. ****P<0.0001 determined using two-tailed Welch's t-test.

(FIG. 12D) Immunoblot using whole aggregate lysates probing for fibronectin ($). β-tubulin ($$) was used as loading control. Semi-quantitative analysis of the blot were normalized to β-tubulin. *P<0.05 determined using two-tailed Welch's t-test.

(FIG. 12E) Representative fluorescence confocal images (maximum projection) of FA and hFLO triculture aggregates at day 14 of culture immunostained for fibronectin. Scale bars, 20 μm.

(FIG. 12F) Quantification of fibronectin networks using AngioTool. 13 fields of view from 3 independently grown aggregates were used. Means, individual values, and standard deviations are shown. *P<0.05; ***P<0.001; ****P<0.0001 determined using two-tailed Welch's t-test.

FIGS. 13A-13G depict FA versus hFLO AngioTool in an embodiment.

(FIG. 13A) Fluorescence confocal microscopy images showing the effects of co-culture to EAhy network formation in suspension. Co-culture with HFL1 is required for EAhy network formation. Scale bars, 100 μm for Day 3; 200 μm for Day 14.

(FIG. 13B) Representative maximum projection images acquired using confocal microscopy of FA and hFLO aggregates, filtered to show only mCherry (HFL1) and Azurite (EAhy) fluorescence. Vascular networks identified by AngioTool shown to the right. Scale bar, 100 μm.

(FIGS. 13C-13G) AngioTool quantification of vascular networks. In d, higher levels indicate more heterogeneity in the distribution of vascular networks. n=8 aggregates for each treatment. Means, individual values, and standard deviations are shown. ns, not significant; *P<0.05; ***P<0.001; Welch's t-test.

FIGS. 14A-14G depict proteomic data processing in an embodiment.

(FIG. 14A) Workflow for the proteomic profiling of FA and hFLO aggregates. Three independent samples were used for FA and hFLO; total proteome was extracted and run using a liquid chromatography-mass spectrometry (LC-MS). Proteomic data were input with MetImp and were quantile normalized.

(FIG. 14B) Boxplot of protein abundance (area) from all protein identified per sample before quantile normalization.

(FIG. 14C) After quantile normalization.

(FIG. 14D) Proteins in FA ranked based on abundance.

(FIG. 14E) Proteins in hFLO ranked based on abundance. Some highly abundant proteins are basement membrane proteins such as LAMB1 and LAMC1.

(FIG. 14F) Cluster analysis across samples and proteins was performed using Euclidean distance based on the protein z-scores.

(FIG. 14G) Correlation map of all detected proteins indicating Euclidean distance between proteins. Pearson's correlation coefficient was used and hierarchical clustering was based on Euclidean distance. Black dashed line indicates major clusters found.

FIGS. 15A-15D depict lumen analysis in fibrotic hFLO in an embodiment.

(FIG. 15A) Representative bright-field images of day 14 hFLO fibrotic model. Scale bar, 300 μm. Bar graphs for aggregate size and circularity. Means, standard deviation, and individual points are shown. We used n=13 independent cell aggregates. **P<0.01 determined using One-way ANOVA with Welch's correction.

(FIG. 15B) Live 3D fluorescence confocal imaging of the aggregates (maximum projection). Scale bar, 200 μm. Cell line volumetric analysis among treatment groups. *P<0.05 determined using One-way ANOVA with Welch's correction.

(FIG. 15C) H-DAB stained aggregates, showing the raw images (Top) and the images after ImageJ processing (Bottom). Scale bar, 250 μm. Quantification of lumen characteristics using ImageJ show means, individual values, and standard deviations are shown. n=11 independent aggregates; *P<0.05, **P<0.01, ****P<0.0001 determined using One-way ANOVA with Welch's correction.

(FIG. 15D) Whole spectrum histogram of intensity of pro-fibrotic markers collagen deposition (Masson), α-SMA, fibronectin, and PDGFR-α (Top). Zoom in on intensities ≥50 AU (Bottom). We used n=9, n=11, n=9, and n=9 independent aggregates for each condition, respectively. Means and 95% confidence intervals are shown.

FIGS. 16A-16C depict vascular cells in vhFLO in an embodiment.

(FIG. 16A) Live fluorescence confocal images (maximum projection) of EAhy cells in day 14 hFLO and vhFLO and AngioTool masks. Scale bar, 300 μm.

(FIG. 16B) Quantification of endothelial networks using AngioTool. We used 5 independent cell aggregates. Graphs show means, individual values, and standard deviation. *P<0.05, **P<0.01 determined using Two-tailed Welch's t-test.

(FIG. 16C) Fluorescence confocal microscopy *maximum projection) using day 14 hFLO showing vascular and perivascular cells stained using UEA1, αSMA, and PDGFRβ. Single z-section image shows luminal morphology in hFLO vasculature. Scale bar, 100 μm; zoomed image scale bar, 50 μm.

FIGS. 17A-17E depict perfusion setup in an embodiment.

(FIG. 17A) CAD render of the 3D printed PEGDA resin perfusion chip; arrows indicate fluidic flow.

(FIG. 17B) Zoomed image showing a micro-grate and its dimensions.

(FIG. 17C) 2D layout of the chip and dimensions of notable features; micro-grates are represented by dotted lines.

(FIG. 17D) Setup of the perfusion chip-pump system.

(FIG. 17E) Time lapse showing even perfusion of dye through both channels over time; perfusion rate is set at 1 mL min⁻¹ well⁻¹.

DETAILED DESCRIPTION

Researchers have struggled to produce organotypic models from stable cell lines. There are several definitions given for organoids in the literature. The prevailing definition focuses on stem cell differentiation and self-patterning of stem-derived cells while embedded in ECM with the idea that stable and mature cells lines do not self-pattern as well into organ-like structures nor give rise to other cell types. We used A549 cells because earlier studies have proven that epithelial cells such as the A549 can form organotypic aggregate structures with a central lumen when embedded in ECM. In this disclosure, we define an organoid as an organotypic 3D cell aggregate composed of multiple specialized cell types, luminal self-patterning, and extracellular matrix which mimic organ structure and function.

Our hypothesis is that incorporating non-gelling concentrations of ECM proteins will improve the currently used scaffold-free, suspension culture resulting in a hybrid culture method. This research demonstrates the importance of the ECM in promoting organotypic patterning, growth, and survival as soluble supplements in suspension culture. Previous studies show that the composite properties of ECM are capable of determining stem cell fate. Additionally, soluble ECM enhances cell proliferation and survival in 2D mesenchymal cell cultures, and enhanced formation of tight junctions in hepatic spheroid cultures. The effects of low, soluble ECM concentrations in organotypic self-patterning and growth, however, have yet to be fully elucidated. We illustrate the use of soluble ECM in the development of an organotypic model from stable cells within a 14-day time period. We refer to it as human fluorescent lung organoid (hFLO). hFLO has airspace-like lumen-gas exchange units and a perfusable vasculature, not present in traditional scaffold-free spheroids.

Here, we provide two potential applications of the hFLO: modeling bleomycin-induced pulmonary fibrosis with a pre-clinical therapeutic and a hypoxic angiogenesis study. Pulmonary fibrosis (PF) in humans is a progressive manifestation of interstitial lung diseases of known and unknown cause and leads to distorted lung parenchyma, irreversible fibrosis, honeycomb lung, respiratory failure and death. Major advances in the pathogenesis of human PF have been made utilizing in vitro and in vivo models of experimentally induced lung injury and PF. There is an unmet need to understand the pathogenesis of PF in human lung cells and tissue via 3D modeling. The creation of such models will result in needed therapeutic development and validation in the targeting the cascades of inflammation and fibrosis.

While several agents are being investigated in the clinic to determine safety and efficacy of pharmacologic agents (clinicaltrials.gov), only two drugs have been approved for clinical use. These antifibrotic agents, nintedanib and pirfenidone are currently used in clinical practice but merely slow down disease process. A long-standing and well-accepted model used to understand pathogenesis and modulation of PF is the bleomycin induced injury model. Here, we show that with bleomycin induction, the hFLO is a viable model in mimicking PF features in vitro and could be applied in a preclinical drug trial of an antifibrotic drug.

The invention is a process in creating 3D cell aggregates (spheroids and organoids) using either stable or primary cell lines (FIGS. 1A-1F). The invention is a hybrid suspension 3D culture that uses non-gelling concentrations of extracellular matrix proteins (ECM) and scaffolds which allow rapid 3D cluster formation while supplementing structural materials for organlike growth. Such that, due to this hybrid culture method, the cells could form clusters within 24 hours. After cluster formation, the cells self-organize into their respective organotypic structures. Organotypic structures that can be formed include tissue stratification, basement membrane formation, and vascular tube formation among others. This method has application in diverse 3D cell culture scenarios including co-culture of cells and formation of primary-derived organoids. Moreover, this method ensures uniformity in quantity of cells used to form organoids, increases seeding survival rate of cells and long-term survival within a 3D structure.

Using this method, we derived a reproducible human fluorescent lung organoid (hFLO) that comprised of a triculture of mature stable cell lines representing the three cell lineages common to most organs especially the lung (FIGS. 2A-2F). hFLO has lung-like architecture with alveolar spaces and vasculature. hFLO has a wide range of usable application including: basic pulmonary lung biochemistry and biology, studying lung diseases, drug testing, and vascular modeling, among others.

This novel process merges two major fields of 3D culture namely scaffolded (gel) and nonscaffolded (suspension) cultures. As per writing, we have not seen any significantly similar prior art. This hybrid method allows for fast compaction and formation of cell clusters (typical to scaffold-free systems) while allowing organotypic growth and survival, especially of vascular components (typical to scaffold-based cultures). This method increases the survival of cells when compared to the traditional scaffold-free cultures. This allows the formation, growth, proliferation, and self-patterning of organoids and spheroids even from mature, differentiated cells in an expedited manner In addition, since the organoids grow in suspension, recovery is unimpeded by solid scaffolds which then makes downstream processing especially protein-based assays with low contaminating proteins.

On the other hand, the novel lung fluorescent triculture organoid (hFLO) is a self-organized organoid from three stable cell lines. The advantages of this organoid over stem cell derived organoids include reduced culture time, cost, and complexity of culture. Since this culture is based on stable cells, it is more accessible to small and low-funded laboratories who do not have access to primary cells and stem cells. Moreover, the production of hFLO is minimalistic, using only fetal bovine serum, methylcellulose, and soluble Matrigel concentrations as the supplements instead of using various differentiation factors.

EXAMPLES

Except in the examples, or where otherwise expressly indicated, all numerical quantities in this description indicating amounts of material or conditions of reaction or use are to be understood as modified by the word “about” in describing the broadest scope of the invention. Practice within the numerical limits stated is generally preferred. The first definition of an acronym or other abbreviation applies to all subsequent uses herein of the same abbreviation and applies mutatis mutandis to normal grammatical variations of the initially defined abbreviation; and, unless expressly stated to the contrary, measurement of a property is determined by the same technique as previously or later referenced for the same property.

Unless indicated otherwise, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention belongs.

Throughout this application, where publications are referenced, the disclosures of these publications in their entireties are hereby incorporated by reference into this application to more fully describe the state of the art to which this invention pertains.

It is also to be understood that this invention is not limited to the specific embodiments and methods described below, as specific components or conditions may, of course, vary. Furthermore, the terminology used herein is used only for the purpose of describing particular embodiments of the present invention and is not intended to be limiting in any way.

It must also be noted that, as used in the specification and the appended claims, the singular form “a,” “an,” and “the” comprise plural referents unless the context clearly indicates otherwise. For example, reference to a component in the singular is intended to comprise a plurality of components.

The term “or” is understood to mean “and/or”.

The term “comprising” is synonymous with “including,” “having,” “containing,” or “characterized by.” These terms are inclusive and open-ended and do not exclude additional, unrecited elements or method steps.

The phrase “consisting of” excludes any element, step, or ingredient not specified in the claim. When this phrase appears in a clause of the body of a claim, rather than immediately following the preamble, it limits only the element set forth in that clause; other elements are not excluded from the claim as a whole.

The phrase “consisting essentially of” limits the scope of a claim to the specified materials or steps, plus those that do not materially affect the basic and novel characteristic(s) of the claimed subject matter.

The terms “comprising”, “consisting of”, and “consisting essentially of” can be alternatively used. When one of these three terms is used, the presently disclosed and claimed subject matter can include the use of either of the other two terms.

Micropatterned suspension culture creates consistently sized and shaped cell aggregates but has not produced organotypic structures from stable cells, thus restricting its use in accurate disease modeling. Here, we show that organotypic structure is achieved in hybrid suspension culture via supplementation of soluble extracellular matrix (ECM). We created a viable lung organoid from epithelial, endothelial, and fibroblast human stable cell lines in suspension culture. We demonstrate the importance of soluble ECM in organotypic patterning with the emergence of lumen-like structures with airspace showing feasible gas exchange units, formation of branching, perfusable vasculature, and long-term 70-day maintenance of lumen structure. Our results show a dependent relationship between enhanced fibronectin fibril assembly and the incorporation of ECM in the organoid.

We successfully applied this technology in modeling lung fibrosis via bleomycin induction and test a potential antifibrotic drug in vitro while maintaining fundamental cell-cell interactions in lung tissue. Our human fluorescent lung organoid (hFLO) model represents features of pulmonary fibrosis that were ameliorated by fasudil treatment. We also demonstrate a 3D culture method with potential of creating organoids from mature cells, thus opening avenues for disease modeling and regenerative medicine, enhancing understanding of lung cell biology in health and lung disease.

2.1. Media Formulations

The media formulations used appear in Table S4.

TABLE S4
Media formulations
Media	Contents	Notes
2D growth	DMEM/F12	For 2D culture
media	+10% Fetal bovine serum (FBS)	of A549, HFL1,
	+Anti-biotic/anti-mycotic (anti-anti)	and LentiX
	(Carson)
	+Plasmocin prophylactic (Invivogen)
3D growth	DMEM/F12	For 3D culture
media	+10% Fetal bovine serum (FBS)	of monoculture
	+Anti-biotic/anti-mycotic (anti-anti)	and triculture
	(Carson)	cell aggregates.
	+Plasmocin	Metylcellulose
	+0.024% methylcellulose (Sigma)	enhances
		aggregate
		compaction.
hFLO	DMEM/F12	The minimum
media	+10% Fetal bovine serum (FBS)	gelling
	+Anti-biotic/anti-mycotic (anti-anti)	concentration of
	(Carson)	Matrigel is 3 mg
	+Plasmocin prophylactic (Invivogen)	mL−1 according
	+0.024% methylcellulose (Sigma)	to the
	+300 μg mL−1 Matrigel GFR	manufacturer*.
		Matrigel
		concentration in
		the hFLO
		media keeps
		the Matrigel
		proteins
		solubilized in
		media.
Vascularization	DMEM/F12	FGF2 and
media (vhFLO	+10% Fetal bovine serum (FBS)	VEGF are pro-
media)	+Anti-biotic/anti-mycotic (anti-anti)	vascular
	(Carson)	factors.
	+Plasmocin prophylactic (Invivogen)
	+0.024% methylcellulose (Sigma)
	+300 μg mL−1 Matrigel GFR.
	+60 ng mL−1 FGF2
	+60 ng mL−1 VEGF-165
*See Corning ® Matrigel ® Matrix Frequently Asked Questions (CLS-DL-CC-026)

2.2. 2D Cell Culture and Cell Line Development

The cell lines used in this disclosure are HFL1 (ATCC CCL-153), EA.hy926 (ATCCRL-2922), A549 (ATCC CCL-185), and Lenti-X™ 293T (632180, Takara Bio, CA, USA). These cells were maintained in 2D culture using the complete 2D growth media. 0.25% trypsin-EDTA (90057, Thermo Fisher Scientific, MA, USA) was used during subculture and split ratios were kept being within the suggested range by the manufacturer. Subculture was done every 2-3 days.

Fluorescent tags were introduced using transfer plasmids that were kindly gifted by Pantelis Tsoulfas via Addgene. Specifically, we used pLV-mCherry (36084, Addgene, MA, USA), pLV-Azurite (36086, Addgene, MA, USA), or pLV-eGFP (36083, Addgene, MA, USA) with second-generation lentiviral vectors pMD2.G (12259, Addgene, MA, USA) and psPax2 (12260, Addgene, MA, USA) which were gifted by Didier Trono through Addgene. Viral gene vectors were transfected using PEI 25 K (23966, Polysciences, PA, USA) into Lenti-XTM 293T cells. Lentiviral particles for eGFP, Azurite, and mCherry gene insertions were collected with the media and were transduced into A549, EAhy or HFL1, respectively using polybrene (TR-1003-G, Sigma-Aldrich, MO, USA) for 72 hours. Cell purification was then done using fluorescence-activated cell sorting (FACS).

2.3. Fluorescence-Activated Cell Sorting (FACS)

Cells and cell aggregates were dissociated using Accumax (AM105.500, Innovative Cell Technologies, CA, USA) for 10 min and 30 min, respectively and strained using a 100 μm cell strainer (15-1100-1, Biologix Research Company, MO, USA) twice. The cells were then resuspended in 1% Bovine serum albumin (BSA, ab41899, Abcam, Cambridge, UK)-PBS buffer. All the FACS experiments were performed using BDAria Fusion Special Order System (BD Biosciences, CA, USA) equipped with 355 nm, 488 nm, 568 nm, and 640 nm lasers. Single cells were gated using forward scatter area (FSC-A) versus forward scatter width (FSC-W) and then with side scatter area (SSC-A) versus side scatter width (SSC-W). Positive expressing cells were gated from a negative control. Cells were sorted into 2D growth media using an 85 μm nozzle and a 0.32.16 purity mask. In depleting NCadherinhigh A549 cells, dissociated cells were stained for an hour on ice with NCadherin antibody (1:200) conjugated in-house using an Alexa Fluor 647 conjugation kit (A32733, Thermo Fisher Scientific, MA, USA). The bottom 30% and top 10% of cells based on AF647 signal were then sorted to deplete or enrich for N-cadherin markers, respectively. Sorted cells were grown in 2D culture as described above. Sorting efficiency during purification of fluorescent cells was verified using an Amnis imaging cytometer and confocal microscopy.

2.4. Ultra-Low Attachment (ULA) Plate

Agarose (BP160-100, Thermo Fisher Scientific, MA, USA) was dissolved in DMEM/F12 media to a concentration of 2% and slowly boiled using a microwave until all particles are dissolved. 50 μL of the agarose solution was then transferred over to each well of the 96 well U bottom plate (10062-900, VWR, PA, USA) then let solidify at room temperature (RT). These plates were then UV irradiated for at least 30 minutes and kept in a 4° C. refrigerator for storage for a maximum of 1 month. For a high-output culture, we used our novel 217-well 3D agarose silicone cast as described previously.

2.5. 3D Cell Culture

To calculate the seeding ratios for each cell line, literature search led us to lung alveolar cell ratios to be around 24% epithelial, 30% endothelial, and 37% interstitial. By this, we simplified the seeding ratio to be roughly 1:2:2 (A549 epithelial: EAhy endothelial: HFL1 fibroblast). For suspension-based cultures, a seeding ratio of 1.0×104 to 1.0×105 total cells per aggregate was used and was divided to each of the cell line using the ratio above. 100-200 μL of mixed cell suspension in 3D media or ECM supplemented 3D media were seeded into each well of the 96-well ULA plate. The triculture suspensions were permitted to self-aggregate and self-organize with the help of gravity and centrifugation for 5 minutes at a maximum of 250×g fFor the first 2-3 days of culture, 10 μM Y-27632 ROCK inhibitor (10005583, Cayman Chemical Company, MI, USA) was supplemented to prevent dissociation-dependent cell death. The cultures were then kept in a 37° C. humidified incubator at 5% CO₂. Media was refreshed every 2-3 days and cultures were kept for 14 days unless otherwise mentioned in-text.

For the gel scaffolded cultures, 8.0×10⁴ cells mL⁻¹ in the same ratio were suspended in pre-gelled solutions of 3 mg mL⁻¹ collagen I, 3 mg mL⁻¹ Matrigel or 4 mg mL⁻¹ Matrigel. Rat tail collagen I (C3867-1VL, Sigma-Aldrich, MO, USA) was diluted in DMEM/F12 media with phenol red and 1 N NaOH was added dropwise until pH was around 7.4. Matrigel (354263, Corning, NY, USA) was simply diluted in DMEM/F12. The solutions were kept on ice to prevent gelling. Cells were resuspended in the pre-gelled solutions and 300 μL of the cell solutions were dropped into glass-bottom plates (P35G-1.5-14-C, MatTek, MA, USA). These were then gelled for 30 minutes in a 37° C. humidified incubator, after which complete growth media was added to each plate and incubated. Media was refreshed every 2-3 days of culture.

2.6. 3D Aggregate Growth Assays

Triculture cell aggregates were grown for 14 days using either traditional force aggregation (FA) or as supplemented with 300 μg mL⁻¹ Matrigel. ROCK inhibitor Y27632 was supplemented for the first 3 days of culture. The media was then refreshed every 2-3 days and the cell aggregates were photographed using either Amscope phase-contrast microscope (Amscope, CA, USA) or Thermo Evos XL phase-contrast microscope (Thermo Fisher Scientific, MA, USA). To measure their respective areas, images were imported into ImageJ as 8-bit format, after which a threshold was manually applied. The image was then processed five times iteratively with the dilate function to converge cells. Cell aggregate sections were then selected using the freeform selection tool and measured for area. The measurements were then normalized to the day 1 measurements. Line graphs were created using the seaborn library in Python.

2.7. Multispectral Imaging Flow Cytometry (MIFC)

Cells were dissociated using Accumax (AM105.500, Innovative Cell Technologies, CA, USA) for 10 minutes for 2D culture and 20 min for 3D cultures. These were then fixed using 1% paraformaldehyde (PFA) in PBS for 30 minutes at 4° C. Cells were then permeabilized using 0.1%Triton X-100 for 10 min and blocked using Seablock blocking buffer (37527, Thermo Fisher Scientific, MA, USA) for 30 minutes at 4° C. Primary antibodies were then diluted with 10% Seablock in 0.1% Tween20 and PBS (PBST) and incubated overnight at 4° C. Secondary antibodies were then added for 1 hour at 4° C. The samples were run in 1% BSA-PBS solution. Positive controls were run first to optimize laser power for each experiment. Using the raw max pixel data for each channel, laser power was adjusted to prevent signal saturation. Data was collected after gating out cells using phase contrast area vs aspect ratio. Both FCS and RIF files were collected for most of the experiments. Color compensation was done during analysis in IDEAS software (Amnis, WA, USA, version 6.2) using the compensation wizard tool, after which in-focus cells were gated using gradient RMS data. For the cell death-related morphometric features, we used bright-field circularity, aspect ratio, shape ratio, contrast, and modulation. Then, the expression values were exported into either FCS or TXT files. FCS files were plotted using python. Representative images were exported as TIFF and colorized either in IDEAS or in Adobe Photoshop 2020 (Adobe, CA, USA, version 21.0.2).

2.8. Localization of Matrigel

A 10 mg mL⁻¹ solution of Matrigel was conjugated with 20× molar excess concentration NHS-dPEG-biotin (QBD10200-50 MG, Sigma-Aldrich, MO, USA) by mixing overnight at 4° C. Excess biotin was removed with a 5 K MWCO concentrator (CLS431487-12 EA, Millipore Sigma, MA, USA) at 4000×g for 100 minutes at 4° C. Matrigel concentration was then assayed with a BCA array (23225, Thermo Fisher Scientific, MA, USA) and diluted to 300 μg mL⁻¹ in 3D media. To confirm biotinylation, 50 μL of 3D growth media, hFLO media, and biotinylated hFLO media were loaded into 16% SDS-PAGE gel and transferred onto 0.2 μm nitrocellulose membranes (1620150, Bio-Rad, CA, USA) through electro blotting. The blot was then probed using Streptavidin Dy-Light 800 (21851, Invitrogen, 1:10,000, MA, USA) for an hour at RT. The blots were imaged using the Odyssey CLx (9140, Li-Cor, NE, USA).

To determine if the Matrigel localizes in the aggregate, 1.0×104 cells per aggregate were cultured in a multi-well agarose dish as described above. For the first 24 hours, normal hFLO media was used and this was changed into the biotinylated hFLO media after 24 hours. Control aggregates were kept in hFLO media. These were then kept in culture for 48 more hours. After 3D culture, the cell aggregates were processed and imaged as described in the whole-mount immunofluorescence methods using Streptavidin (29072, Biotium, 1:500, CA, USA) and a DAPI (1:500) counter-stain.

2.9. Flow Cytometry

Cells were dissociated using Accumax for 10 minutes for 2D culture and 20 minutes for 3D cultures. These were then fixed using 4% PFA in PBS for 15 minutes at 25° C. Cells were then permeabilized-blocked using 0.1%Triton X-100 in Seablock buffer for 15 minutes at 25° C. Primary antibodies were then diluted with 10% Seablock in 0.1% Tween20 and PBS (PBST) and incubated for 1 hour at 25° C. Secondary antibodies (1:500 dilution) were then added for 30 minutes at 25° C. The samples were run in 1% BSA-PBS solution. Detector voltages were determined using single-color controls. All files were exported as FCS and analyzed using FlowJo (BD, CA, USA, v9.9.4). Compensation was done using the Compensation Wizard and single-color controls. Doublets were then excluded using FSC-A vs FSC-H and SSC-A vs SSC-W gates. Single cells were then analyzed and any applicable gates are included in supplementary information.

2.10. Murine and Porcine Lungs

All experiments were performed per the NIH Guide for the Care and Use of Laboratory Animals and were approved by Institutional Animal Care and Use Committees at Brigham Young University-Provo. Wild type C57BL/6 mice were sacrificed and were perfused ventricularly with sodium heparin solution in PBS (H3393-100KU, Sigma-Aldrich, MO, USA). The lungs were then excised and fixed in 4% PFA overnight at 4° C. The porcine lungs were gifted by Circle V Meats Co. (UT, USA). The lungs were received and processed within the hour of sacrifice. Lung sections were washed thrice with heparinized PBS for 10 minutes each and visible blood clots were removed. The lungs were then sectioned into 1-inch cubes and fixed overnight with 4% PFA at 4° C.

2.11. Live Confocal Imaging

Suspension-based cell aggregates were collected and transferred to a MatTek glass bottom plate (P35G-1.5-14-C, MatTek, MA, USA) with minimal volume of complete cell media to prevent dehydration. The plates were then mounted into the live cell imaging chamber (Okolab, Ottaviano, Italy) attached to a Leica TCS SP8 confocal microscope (Leica, Wetzlar, Germany). The chamber was set to 5% CO₂ at 37° C. throughout the experiment. Either the 20× or 40× objectives were used during imaging. Argon laser was consistently set to 25% and individual laser powers were kept being less than 5% to prevent excessive phototoxicity while imaging. Images were acquired with at least 512×512 voxel density with optical zoom from 0.7 to 1.0×.

2.12. Section and 3D Whole-Mount Immunofluorescence

Samples were fixed in 1% PFA overnight at 4° C. 800 rpm shaking incubator, embedded in Tissue Tek OCT (4583, Sakura, Tokyo, Japan), and then sectioned into 7-10 μm sections using a TN50 cryostat (TNR TN50, Tanner Scientific, FL, USA). The slides were dried for 15 minutes at room temperature prior to storage in −80° C. or processing for immunohistochemistry or histology. The sections were then permeabilized using 0.1% Triton X-100 for 10 minutes and then blocked using Seablock buffer for 1 hour at room temperature. Primary antibodies (Table S4) were diluted in 10% Seablock in PBST and incubated overnight at 4° C. After intensive washing, secondary antibodies were then diluted to 1:500 in 10% Seablock PBST and incubated for an hour at RT. Counterstaining for the nucleus, if necessary, was done either by DAPI (14285, Cayman, MI, USA; 1:500), Hoecsht (62249, Thermo Fisher Scientific, MA, USA; 1:1000), or Toto-3 iodide (T3604, Invitrogen, MA, USA; 1:500) diluted in PBST. The slides were mounted using diamond antifade (P36961, Thermo Fisher Scientific, MA, USA) and cure at RT for at least 24 hours prior to imaging.

For whole mount imaging, each step was done in an 800-rpm temperature-controlled shaker. Permeabilization was achieved using 0.3% TritonX-100 for 15 minutes then blocked for 2 hours at RT using Seablock blocking buffer with 0.3%TritonX-100. Primary antibodies were diluted in 10% Seablock in 0.3% Triton X-100 and incubated for 24-48 hours at 4° C. Secondary antibodies and nuclear counterstain were added to the whole aggregates for 2 hours at RT. After the samples were immunostained, refractive index matching was achieved using an in-house Ce3D clearing buffer overnight at RT as previously shown.

Confocal imaging was done using a Leica TCS SP8 Hyvolution confocal microscope with LASX software (Leica, Wetzlar, Germany, version 3.1.1.15751). Argon laser power was consistently set to 25%. Use of the HyD detectors were preferred over the PMT detectors and gains for the detectors are set to less than 100%. If needed, samples were stitched using the built-in Auto Stitch function in the LASX software. The images were deconvolved Huygens Essential (SVI, Hilversum, The Netherlands, version 19.04) using the Deconvolution Wizard function. The final images were exported as TIFF files and gamma was not adjusted for any images. Volumetric image analysis was perfomed using the 3D analysis package in LASX software. Volumes were then normalized to nuclear volume.

2.13. Histological Staining

2.13.1. Hematoxylin and Eosin (H&E) Staining

H&E staining was performed on cell aggregate frozen sections as indicated by the manufacturer (Richard-Allen Scientific, MI, USA), using hematoxylin (7211, Richard-Allen Scientific, MI, USA) and eosin staining (7111, Richard-Allen Scientific, MI, USA). The slides were then cleared 3 times in 100% ethanol. Slides were then washed 3 times using Histo-Clear (HS-200, National Diagnostics, NC, USA) for 5 min, after which the slides were mounted using Clarion mounting medium (CO487, Sigma-Aldrich, MO, USA). Slides were then cured overnight at 37° C. before imaging.

2.13.2. Masson Staining

Cell aggregate sections were processed following the protocol of Trichrome Stain (Masson) as indicated by the manufacturer (HT15-1 KT, Sigma-Aldrich, MO, USA), after which the slides were allowed to air dry. Slides were then washed using Histo-Clear (HS-200, National Diagnostics, NC, USA) for 5 minutes before being mounted using Clarion mounting medium (CO487, Sigma-Aldrich, MO, USA). Slides were then cured overnight at 37° C. before imaging.

2.13.3. Hematoxylin-DAB

Cell aggregate sections were permeabilized using 0.1% Triton X-100 for 10 minutes and then blocked using Seablock buffer for 1 hr at room temperature. Primary antibodies (Table S4) were diluted in 10% Seablock in PBST and incubated overnight at 4° C. After intensive washing, HRP-conjugated secondary antibodies were then diluted to 1:500 in 10% Seablock PBST and incubated for an hour at room temperature (RT). The chromogen was developed using a DAB kit (34002, Thermo Scientific, MO, USA) for 15 minutes at RT. Counterstaining for the nucleus was done using hematoxylin staining and bluing reagent. The slides were then cleared 3 times in 100% ethanol. Slides were then washed 3 times using Histo-Clear (HS-200, National Diagnostics, NC, USA) for 5 minutes, after which the slides were mounted using Clarion mounting medium (CO487, Sigma Aldrich, MO, USA). Slides were then cured overnight at 37° C. before imaging.

2.14. Transmission Electron Microscopy (TEM)

Samples were collected directly into 2% Glutaraldehyde in 0.06 M sodium cacodylate buffer and remained in the fixative for at least 2 hours. The samples were washed 6 times in PBS for 10 minutes each. Secondary fixation continued using 1% Osmium tetroxide (19152, Electron Microscopy Sciences, PA, USA) for 1.5 hours. Samples were then washed 6 times with distilled water for 10 min each. The samples were then stained with 0.5% uranyl acetate overnight with gyration. In preparation for resin embedding the samples were dehydrated serially with ethanol (30%-50%-75%-90%-100%-100%-100%) with 10-minutes incubation per stage. Samples then were washed 3 times in acetone for 10 min each. Resin embedding was done using in house Spurr low viscosity resin with serial preparation steps in acetone (2:1-1:2-0:1, acetone:resin) for 90 minutes each with gyration. The samples were then resin-embedded in Beem capsules (130, Ted Pella, CA, USA) and cured overnight in a 70° C. oven. The embedded samples were then sectioned to 80 nm thick using an RMC MTX microtome using an in-house glass knife. Sections were collected on a Formvar/Carbon 200 mesh support grids (01800, Ted Pella, CA, USA) and counterstained with lead. Images were taken using a Helios NanoLab 600 Dual Beam FIB/SEM using the TEM feature.

2.15. Shotgun Proteomics

Fourteen-day old FA and hFLO cell aggregates were collected and washed twice with PBS for 10 minutes each with gyration. To lyse the samples, RIPA buffer with Halt's inhibitor cocktail (89900, Thermo Fisher Scientific, MA, USA) was added and then the samples were vortexed thrice for 5 min each time and then boiled for 5 minutes at 95° C. The samples were then further sheared using a bead beater and then passed through a 25G needle. The whole aggregate lysates were collected by centrifugation at 16,000×g for 5 minutes. Protein concentration was then quantified using Peirce™ BCA Protein assay kit (23225, Thermo Fisher Scientific, MA, USA). Processing the samples for proteomics was then continued using a 10 kDa filter aided sample preparation protocol previously published with minor modifications. The proteins were digested using Lys-C enzyme (P8109S, New England Biolabs, MA, USA; 1:50) and then with trypsin (V5111, Promega, WI, USA; 1:100). The samples were then dried in a vacuum centrifuge for 1.5 h at RT and then resuspended in running buffer. The samples were then analyzed using Thermo Fisher™ Q-Exactive Obitrap (Thermo Fisher Scientific, MA, USA). The mass spectrometry proteomics data have been deposited to the ProteomeXchange Consortium via the PRIDE partner repository with the dataset identifier PXD027296.

2.16. Proteomic Bioinformatic Analysis

Mass spectrometric raw data files were processed using PEAKS (Bioinformatics Solutions, Waterloo, Canada, version X PRO 2020) and were searched against the human proteome database (Uniprot_SwissProt_Oct2020). The Label-free quantification (LFQ) values were quantile normalized between FA and hFLO proteome. LFQ values were compared between the FA and hFLO proteomes using pairwise statistical tests based on two-tailed Welch's t-test. Protein-protein correlation was calculated using R Studio corrplot function. Unbiased gene set interrogation was performed using GSEA native GO-term set (ftp.broadinstitute.org://pub/gsea/gene_sets/c5.all.v7.4.symbols.gmt). Graphs were then created using GraphPad Prism (GraphPad Software, CA, USA) or R Studio ggplot2.

2.17. Bleomycin-Induced Fibrosis

Cell aggregates were grown as described above for 7 days, after which the cell aggregates were treated with 20 μg mL⁻¹ bleomycin (13877, Cayman Chemical Company, MI, USA, stock solution diluted in either PBS or DMSO). Media was changed after 3 days of culture with bleomycin (i.e., at day 10). At day 10, the organoids were weaned off the bleomycin insult and then treated with either 10 μM fasudil (B3523, ApexBio, TX, USA) or with DMSO (control, vehicle used for fasudil). The cultures were kept in treatment media for 4 more days with media changing every two days. Cell aggregates and media were collected and fixed as described above.

2.18. Cytokine Array

The organoid media from the three treatment groups were collected at day 14. The levels of cytokines secreted to the media were immediately evaluated using the Human Cytokine Array C1000 (AAH-CYT-1000-8, Ray Biotech, GA, USA) with minor modifications. Briefly, the membranes were blocked at room temperature for 30 minutes using the blocking buffer. The media from the organoids were transferred onto the membranes and incubated with gentle rocking overnight at 4° C. After washing, the membranes were incubated with the biotinylated antibody cocktail overnight at 4° C. After further washes, the membranes were probed with Streptavidin-CF680R (29072, Biotium, CA, USA 1:1000) for 1 hour at RT. The membranes were imaged using an Odyssey CLx imager (LI-COR, Cambridge, UK) at high resolution and a wavelength of 700 nm. The exported images of the membranes were quantified using gel analysis plugin on FIJI distribution of ImageJ (open source) under the GNU General Public License.

2.19. Hypoxic Culture

At day 7, media was changed to angiogenic media comprised as described in Table S4, and the culture was purged with 5% O₂, 5% CO₂, 90% N₂ gas mixture. Cell media was changed every 2-3 days using the angiogenic media. The air inside the chamber was replaced every time media was changed. The culture was harvested 7 days post induction.

2.20. 3D Printing

The 3D printed high-flow organoid devices used in this paper were designed in OpenSCAD and fabricated using a custom stereolithographic 3D printer. The printer was a third-generation model of the printer that was previously published. The printer's custom Python software allows for precise control over all aspects of the printing process enabling intricate design capabilities, such as the grates used on the organoid devices. A custom photo-polymerizable resin was used consisting of poly(ethylene glycol) diacrylate (PEGDA, MW258, 475629, Sigma-Aldrich, MO, USA) as the monomer, 1% (w w⁻¹) phenylbis(2,4,6-trimethylbenzoyl) phosphine oxide (Irgacure 819, 415952, Sigma-Aldrich, MO, USA) as the photo-initiator, and 0.38% (w w⁻¹) avobenzone (16633, Sigma-Aldrich, MO, USA)—a UV absorber to control light penetration during 3D printing. This was an ideal surface for organoid analysis because it has been proven to be non-cytotoxic with extremely low adherence. The resulting device has the dimensions shown in Table S5.

TABLE S5
Dimensions of 3D printed millifluidic perfusion device
	Part	Dimension	Value
	Bulk	Length	18.00	mm
		Width	12.16	mm
		Height	2.50	mm
	Input/Output	Width	319	μm
	channels	Height	300	μm
	Wells	Diameter	4.56	mm
		Depth	0.50	mm

2.21. Millifluidic Dextran Perfusion

Cell aggregates including A549 spheroids, triculture aggregates grown in traditional FA, hFLO cell aggregates, and vhFLO cell aggregates were grown until 14 days post seeding. Capillary fluidic flow was modeled using PTFE tubing (AO-06417-21, Cole-Palmer, IL, USA), a peristaltic pump (61161-354, VWR, PA, USA), and a 3D-printed biocompatible 4-well chip based on our previously published methodology. Prior to the experiment, the fluidic system was flushed with DMEM/F12 media and the peristaltic pump was then calibrated manually to 1 mL min⁻¹well⁻¹. Afterwards, 20 μg mL⁻¹ Texas Red™ 70 kDa dextran (D1864, Invitrogen, MA, USA) was perfused through the system to replace the media. 14-day old cell aggregates were then transferred into the 3D-printed microwell devices. To seal high-flow devices, glass slides wrapped with parafilm were carefully clamped onto the 3D printed chips. Dextran solution was perfused cyclically for 1 hour, after which cell aggregates were collected and rinsed with PBS thrice for 5 minutes each to remove unbound dextran. They were then fixed in 1% PFA overnight at 4° C. The cell aggregates were then counterstained with DAPI and processed for whole-mount immunofluorescence as described above.

2.22. Image Analyses

2.22.1. Line Profile Grey Value Analysis

Day 14 cell aggregate images were uploaded to ImageJ version 1.53c. We used the line tool and the plot profile function to derive grey values (Y) versus the line distance (X). We then used Microsoft Excel for further data processing. We normalized the grey values (Y) to a common scale where denser regions of tissue have the higher values (100%) and spaces/lumina have lower values (0%). The distance value (X) is normalized such that the core of the cell aggregate is set at zero (range=−100, +100). For more information, see supplementary protocol.

2.22.2. Lumen Size Quantification

Histologically stained samples were imaged and processed with ImageJ software. First, images were converted to an 8-bit greyscale, after which a threshold was applied. The image was then processed five times iteratively with the dilate function to converging boundary cells. Afterwards, the section area was selected, the image outside the aggregate section was cleared, and the image was inverted such that the lumens only were displayed. The “count particles” function was used to measure lumen characteristics. Data was processed in Microsoft Excel, lumen under the size of 200 μm2 were excluded in all analysis except the calculations of total lumen area and lumen percent area.

2.22.3. Masson-Trichrome and H-DAB Color Analyses

The ratios of collagen to tissue in organoids were determined by analyzing images of Masson-Trichrome stained sections. These images were separated into red, blue, and green components using ImageJ using color deconvolution function. For the Masson staining, areas of the blue and red image channels were determined by thresholding and collagen deposition was determined as the ratio of blue area to red area (collagen to tissue). Intensity histograms were created using the ImageJ histogram function on the selected red area, and average pixel intensity was calculated from the histogram output in Microsoft Excel. For H-DAB, the target protein is the brown channel and the hematoxylin is the blue-purple channel.

2.23. Statistical Analyses

Independent samples were randomly selected for all studies. Statistics were determined using GraphPad Prism (GraphPad Software, CA, USA, version 9.1.1). Where appropriate, equal sampling was employed. Pairwise comparisons to determine statistical significance was carried out using two-tailed Welch's t-test. For multiple group comparisons, One-way ANOVA was employed with pairwise tests carried out with Welch's correction. Graphs were then generated using GraphPad Prism 9, Python, or R Studio 3.6.2.

2.24. Data Availability

The mass spectrometry proteomics data are publicly available. They have been deposited to ProteomeXchange Consortium via the PRIDE partner repository and can be accessed with the dataset identifier PXD027296. All supporting the main and supplementary conclusions of the paper were provided with the manuscript. All other data are available upon reasonable request from the corresponding author, P.M.V.R. (pvanry@chem.byu.edu).

3. Results

3.1. Soluble ECM Promotes Airspace-Like Lumen-Gas Exchange Unit Formation in Suspension Culture

Previous studies have used soluble matrix proteins as media additives to improve cell aggregation and as a potent pro-proliferative factor. Despite this, the relationship between soluble ECM and self-patterning towards 3D organotypic growth is yet to be discovered. To model the lung alveolus, we used traditional forced aggregation (FA) method and our hybrid method supplementing soluble concentration of ECM to promote organotypic self-patterning. In order to visualize topographical changes accompanying ECM changes, three fluorescently labeled stable cell lines were employed to represent the three major alveolar tissue types including endothelial EA.hy926 (EAhy, Azurite-tagged), lung epithelial type II-like A549 (eGFP-tagged), and normal lung fibroblast HFL1 (mCherry-tagged) (FIGS. 7a-c). Previous studies show that A549 cells form organotypic luminal structures once embedded in ECM, mimicking features of an organotypic culture observed using primary-derived alveolar type 2 cells. Moreover, A549 has previously been shown to exhibit stem-like properties of self-renewal, multipotency, differentiation, and clonogenic formation in its epithelial (EPCAM+) subpopulation. On the other hand, due to its nature as a cancer cell line, certain subpopulations express mesenchymal, pro-metastatic proteins. To mitigate these traits and improve its epithelial stem-like nature, we used fluorescence-activated cell sorting (FACS) to deplete mesenchymal N-Cadherinhigh population which selects for the more stable epithelial cell population.

We then engineered a 3D triculture to model the lung alveolus and the morphological changes accompanying soluble ECM concentration. In the native lung alveolus, the epithelium forms airspaces with interstitial and vascular cells between the epithelium. We incorporated labeled or unlabeled A549-eGFP, HFL1-mCherry, and EAhy-Azurite in 3D tricultures with varying ECM concentrations—high (gel scaffold, ≥3 mg mL⁻¹), low (soluble ECM-supplemented suspension, ≤300 μg mL⁻¹), and no ECM (traditional FA) (FIGS. 1A-1F and FIGS. 8A-8C). The 3 cells were mixed in suspension prior to seeding and spheroid organization was dependent on self-patterning aided by soluble ECM. Cell seeding ratios were followed based on endogenous human lung cell composition which we determined to be roughly 1:2:2 (epithelial: interstitial: vascular) (Table S1).

TABLE S1
Cell composition of lung and hFLO triculture
			Per 1.0 × 104 cell
Cell type	Whole lung	Triculture	aggregate
Epithelial	24% of cells	20% of cells	2.0 × 103
cells*
Endothelial	29% of cells	40% of cells	4.0 × 103
cells**
Interstitial	36% of cells	40% of cells	4.0 × 103
cells***
Other cells	10% of cells	—	—
*This includes both Type I and Type II alveolar cells for whole lung. In hFLO, only A549 cells are used.
**In hFLO, endothelial cells are modeled with the EAhy cell line.
***In hFLO, interstitial cells are modeled with the HFL1 cell line.

With this ratio, high ECM concentrations in gel scaffolds led to the formation of multiple A549 epithelial clusters without cohesion of all three cell lines (FIGS. 8ab). In gel scaffolds, fibroblast-endothelial (HFL1-EAhy) network formation were observed as reported by previous researchers (FIG. 8B). In comparison, all soluble ECM concentrations tested led to the formation of a singular cell cluster with all three cell lines incorporated (FIG. 1A). An important component of the human alveolus is alveolar sacs, which are small airspace-filled voids made from epithelial cell and separated by a common septum. Bright-field images of cultures with soluble ECM were analyzed for possible less dense airspace-like voids. Images and grey line profile analysis show several less dense regions with supplementation of 300 μg mL⁻¹ Matrigel, while traditional FA cultures appear as densely packed aggregates (FIG. 1B). Live confocal imaging reveals self-organized structures in the triculture aggregates similar to those observed in mammalian alveolus (FIG. 1C and FIGS. 8B-8C). Self-organized structures observed in both gel scaffold and soluble ECM-supplemented cultures include epithelial clustering and an endothelial-fibroblast network, neither of which were observed in the traditional FA culture (0 μg mL⁻¹) (FIGS. 1C, 8B-8C, and 3A-3B). In soluble 100 μg mL⁻¹ collagen suspension cultures, epithelial cells form a dense core aggregate; however, 300 μg mL⁻¹ Matrigel cultures form airspace-like lumina (FIGS. 1A-1C, 8C, and 3A-3B).

Aggregates were stained with hematoxylin and eosin (H&E) and compared to healthy murine and porcine lung sections to further confirm the relationship between the use of soluble ECM and the formation of voids inside the aggregates. Triculture aggregates grown with traditional FA (0 μg mL⁻¹ ECM), 100 μg mL⁻¹ collagen I, and 100 μg mL⁻¹ Matrigel were confirmed to be predominantly compact cell clusters. Yet with 300 μg mL⁻¹ Matrigel supplementation, we observed the presence of mammalian airspace-like lumina with septa (FIG. 1D). Upon quantification of the soluble ECM supplemented aggregates, we saw an increased number and percent area of voids inside the 300 μg mL⁻¹ Matrigel-grown aggregates relative to the traditional FA. Together this data confirms that supplementation of soluble Matrigel leads to topographical arrangement of cells similar to those found in native alveoli (FIGS. 9A-9B).

Keeping our overarching goal in mind to produce an organotypic structure for use in downstream processes, we used established mammalian alveolus markers that are cell type-specific and are known to localize to specific regions in the alveolus Immunohistochemistry of day 14 cell aggregates were compared to murine and porcine lung sections to verify the typical mammalian lung alveolus localization pattern. Epithelial cells as indicated by epithelial cell adhesion molecule (EPCAM+) are known to localize on the airspace-like lumen with mesenchymal cells labeled with (Vimentin+) in the alveolar-like septum (FIG. 1E). Epithelial subpopulation type II (pro-surfactant protein C, SPC+) and type I (Podoplanin, Pdpn+) cells should be found proximal to the lumina. Observational comparisons show that all four of these markers distributed in aggregates grown using 300 μg mL⁻¹ Matrigel in a similar fashion to both murine and porcine sections. (FIG. 1E).

Transmission electron microscopy (TEM) was used to visualize vital ultrastructures in the aggregates such as the presence of lamellar bodies and microvilli in type II cells, presence of basement membrane, and the localization of the epithelial cells bordering the airspaces. We observed the presence of lamellar body-like (LBL) inclusions A549 (type II-derived cell line) as previously shown. We also identified LBL inclusions in 0 μg mL⁻¹ ECM and 300 μg mL⁻¹ Matrigel cell aggregates and A549 spheroids which is attributed to A549 being a type II-derived cell (FIGS. 1F and 10A-10B). Using TEM, we verified that the use of 300 μg mL⁻¹ Matrigel led to the formation of luminal structures—both on the alveolar epithelial surface and within the luminal endothelial cells (FIG. 1F). Moreover, we observed the presence of a basement membrane between epithelial and endothelial tissue layers in 300 μg mL⁻¹ Matrigel cell aggregates further supporting observations of organotypic formation (FIG. 1F). Together, our data suggests that basic alveoli-like and vascular structure is achieved in a triculture suspension by supplementing with 300 μg mL⁻¹ Matrigel. Hereafter, we will refer to this triculture hybrid 3D method as the human fluorescent lung organoid (hFLO) (FIGS. 9A-9B).

3.2. Soluble ECM Promotes Aggregate Growth and Survival Compared to FA Cultures

Previous studies show pro-survival effects of a soluble ECM in mesenchymal stem cells. Thus, we examined pro-survival and pro-growth effects of soluble Matrigel in 3D suspension. We tracked aggregate size using bright-field microscopy during a 14-day culture of both FA and hFLO and found that hFLO aggregates increase 2-fold in size while FA aggregates remained nearly constant (FIGS. 2A-2B). Dissociated aggregate cell counts revealed a 3-fold increase in cell counts in hFLO, whereas FA aggregates only increased 1.5-fold from original seeding density (FIG. 2C). To determine if supplementation of soluble ECM supports the maintenance of the general aggregate structure, we cultured hFLO up to day 70 and examined general histological structure using H&E staining. Although we saw a slight increase in percent lumen area, no change was observed in average number of luminal voids, suggesting that the general organotypic structure can be maintained for at least 70 days (FIG. 2D).

One of the drawbacks of using FA culture is that within the dense aggregate core cell death occurs due to hypoxia and starvation. Previous research demonstrates that endothelial cells are susceptible to cell death when cultured in suspension. Moreover, in precision cut lung slice cultures, endothelial cells were observed to not survive beyond 7 days of culture. Cell type survival was measured through volumetric analysis of each fluorescently-labeled population to determine cell ratio changes throughout the 14-day culture in suspension. Without soluble ECM, we found that HFL1-fibroblast and EAHy-endothelial cell populations progressively decrease through the time of culture with A549-epithelial cells constituting greater than 80% of FA by day 14. (FIG. 2E). In contrast, cell population ratios based on volume were maintained in hFLO for the same time period (FIG. 2E).

To determine if cell death was activated in FA more than in hFLO, we performed imaging flow cytometry. We found that apoptotic marker, cleaved caspase 3 (CASP3) is significantly increased in FA (FIG. 2F). Moreover, cell death morphometric analyses for shape change (cell circularity, aspect ratio, and shape ratio) show increased apoptotic markers in FA (low circularity, low aspect ratio, and low shape ratio, FIGS. 11A-11E). Our data suggests that hFLO with 300 μg mL⁻¹ Matrigel supplementation resulted in enhanced aggregate growth with conserved cell populations and histological structure.

Our results imply that the supplementation of 300 μg mL⁻¹ Matrigel is responsible for improved organotypic structure over FA. Though it is unclear, if Matrigel is taken up by the organoid and then embedded as a component in the aggregate or if processes are initiated to increase fibronectin expression. To answer this, we conjugated Matrigel with biotin for visualization of potential incorporation in the organoid (FIG. 12A). Cross-sectional confocal images (z-sections) revealed biotinylated Matrigel is indeed embedded throughout the aggregates (FIGS. 12B-12C). Due to a recent report showing that immobilization of Matrigel promotes fibronectin fibrillar formation, we immunostained whole FA and hFLO cell aggregates to determine the extent of fibronectin expression and organization into fibrils. Through semi-quantitative Western blot analysis, we observed increased fibronectin expression (FIG. 12D). Since there is a known link between fibrillar formation and vascular morphogenesis, we used AngioTool (an image analysis software employed to measure network formation) to characterize fibronectin fibrillar morphology and found significantly improved fibrillar features such as branching and lacunarity (FIGS. 12E-12F). Together this data shows that there is both an increase in fibronectin expression and fibril assembly with the supplementation of Matrigel.

3.3. Soluble ECM Promotes Vascular Formation in Aggregates

Literature shows that endothelial and fibroblast interactions are essential for vascular-like branching. We used live confocal images to explore the effects of soluble ECM in formation of a vascular-like network. We found that co-culture of epithelial and endothelial cell did not form branching networks but co-culture of epithelial and fibroblast were sufficient for fibroblast network formation (FIG. 13A) Presence of all three cell lines with ECM supplementation resulted in the formation of vascular like networks composed of both fibroblast and endothelial cells around epithelial cells (FIGS. 1A-1F, 3A, and 8A-8C). Quantification using AngioTool verified significantly more vascular like characteristics such as, endothelial-fibroblast branching (FIGS. 3B and 13B). Thus, for the first time, we show that endothelial branching is activated in the presence of soluble ECM and is dependent on fibroblasts.

We used expression and patterning of known markers of vascular maturation (having both endothelial and perivascular cells) to verify formation of vascular like structures. Imaging of vascular cells in hFLO revealed the presence of endothelial cell marker Ulex europaeus lectin (UEA1+), in proximity to perivascular cell markers including smooth muscle actin (αSMA), platelet-derived growth factor receptor (PDGFRβ), and desmin (FIGS. 3C and 3D). Upon volumetric analysis, we found that these endothelial and perivascular-like expressing cells were barely present in FA (FIG. 3E). Flow cytometry analysis confirmed that although these perivascular-like cells were rare in hFLO, accounting for 2-3% of total cells, they were nearly absent in FA with 0.2-0.36% of the total cells (FIG. 3F). This provides additional evidence that growth of organotypic, vascular-like networks are promoted with the addition of soluble ECM.

3.4. Pro-Morphogenic Expression is Enriched with Soluble ECM

To determine if the histological and biochemical changes noted thus far are supported by proteomic changes, we analyzed the whole proteome of day 14 FA and hFLO. This data was used to identify upregulated or down-regulated protein groups with addition of soluble ECM (FIG. 14A). After imputation and quantile normalization, we confidently identified 967 proteins common to both FA and hFLO (FIGS. 14B-14E). Some of the most abundant proteins detected in hFLO are basement membrane proteins including laminins LAMB1 and LAMC1, which is expected based on the addition of Matrigel (FIG. 14E). Upon clustering and principal component analysis we observed statistical difference between FA and hFLO proteome (FIGS. 4A-4B and 14F). Hierarchical clustering of protein-protein correlation across all samples shows the general proteome landscape changes and implies co-regulation among proteins associated with hFLO (FIG. 14G). Among the proteins, 147 were determined as differentially expressed proteins but only 42 are highly differentially expressed having an absolute fold change greater than 2 (FIG. 4C). 19 proteins (2% of total) were upregulated in hFLO while 23 (2.4% of total) were downregulated. Some upregulated proteins include extracellular structural proteins such as COL18A1, LAMA1, and NID1 supporting the possible deposition of Matrigel in the aggregates as observed in our biotin experiment (FIG. 4B).

We used the built-in gene ontology term (GO-Term) biological process set in Gene Set Enrichment Analysis (GSEA) to perform an unbiased characterization of the whole proteome (FIG. 4D). Some of the top significantly enriched GO-terms in hFLO are pro-morphogenic, related to ECM organization, and markers of active metabolism (FIG. 4E and Table S2).

TABLE S2
GO_TERM	SIZE	NOM p-val	NES
GO_EXTRACELLULAR_MATRIX	46	0.0000	1.8681
GO_EXTRACELLULAR_MATRIX_STRUCTURAL_CONSTITUENT	15	0.0000	2.2185
GO_EXTRACELLULAR_STRUCTURE_ORGANIZATION	38	0.0000	1.8125
GO_OXIDOREDUCTASE_ACTIVITY	95	0.0000	1.6920
GO_CELLULAR_CARBOHYDRAT_METABOLIC_PROCESS	26	0.0024	1.8148
GO_OXIDATION_REDUCTION_PROCESS	125	0.0030	1.6308
GO_COLLAGEN_CONTAINING_EXTRACELLULAR_MATRIX	43	0.0048	1.8572
GO_LIPID_BINDING	64	0.0052	1.5987
GO_NEGATIVE_REGULATION_OF_MULTICELLULAR_ORGANISMAL_PROCESS	66	0.0079	1.5475
GO_ISOMERASE_ACTIVITY	27	0.0093	1.6299
GO_REGULATION_OF_PROTEIN_CONTAINING_COMPLEX_DISASSEMBLY	18	0.0118	1.7349
GO_ANATOMICAL_STRUCTURE_FORMATION_INVOLVED_IN_MORPHOGENESIS	61	0.0148	1.4774
GO_GENERATION_OF_PRECURSOR_METABOLITES_AND_ENERGY	84	0.0179	1.4288
GO_VESICLE_LUMEN	78	0.0236	1.4563
GO_FATTY_ACID_DERIVATIVE_METABOLIC_PROCESS	20	0.0245	1.6936
GO_REGULATION_OF_CELL_ADHESION	44	0.0246	1.4709
GO_TRANSITION_METAL_ION_BINDING	49	0.0260	1.4731
GO_ICOSANOID_METABOLIC_PROCESS	16	0.0276	1.6214
GO_PROTEIN_MATURATION	26	0.0291	1.5363
GO_ENERGY_DERIVATION_BY_OXIDATION_OF_ORGANIC_COMPOUNDS	42	0.0299	1.5700
GO_CELL_SUBSTRATE_ADHESION	35	0.0304	1.5099
GO_ALPHA_AMINO_ACID_METABOLIC_PROCESS	17	0.0305	1.5692
GO_FICOLIN_1_RICH_GRANULE	51	0.0306	1.5090
GO_NEGATIVE_REGULATION_OF_PROTEOLYSIS	33	0.0320	1.5045
GO_METHYLATION	21	0.0328	1.5146
GO_TUBE_MORPHOGENESIS	49	0.0357	1.4751
GO_ENDOPLASMIC_RETICULUM_LUMEN	48	0.0363	1.4231
GO_STRUCTURAL_CONSTITUENT_OF_CYTOSKELETON	21	0.0370	1.5081
GO_CARBOHYDRATE_METABOLIC_PROCESS	65	0.0374	1.3632
GO_FATTY_ACID_METABOLIC_PROCESS	32	0.0385	1.5376
GO_POSITIVE_REGULATION_OF_CELL_POPULATION_PROLIFERATION	51	0.0385	1.4107
GO_CARBOHYDRATE_BIOSYNTHETIC_PROCESS	26	0.0387	1.6355
GO_REGULATION_OF_CELLULAR_COMPONENT_MOVEMENT	68	0.0403	1.4010
GO_LIPID_METABOLIC_PROCESS	88	0.0476	1.2902
GO_NEGATIVE_REGULATION_OF_CELLULAR_COMPONENT_MOVEMENT	23	0.0478	1.5128
GO_NEGATIVE_REGULATION_OF_PROTEIN_CONTAINING_COMPLEX_ASSEMBLY	22	0.0486	1.4451
GO_PHOSPHOLIPID_BINDING	36	0.0528	1.4085
GO_BLOOD_MICROPARTICLE	28	0.0534	1.4643
GO_BIOLOGICAL_ADHESION	88	0.0580	1.3130
GO_EPITHELIAL_CELL_PROLIFERATION	22	0.0581	1.4577
GO_REGULATION_OF_CELL_SUBSTRATE_ADHESION	23	0.0602	1.4335
GO_PROTEIN_POLYMERIZATION	44	0.0613	1.4062
GO_PEPTIDE_SECRETION	37	0.0633	1.4016
GO_CELLULAR_LIPID_METABOLIC_PROCESS	65	0.0633	1.3097
GO_CELLULAR_RESPIRATION	32	0.0647	1.4218
GO_CELLULAR_OXIDANT_DETOXIFICATION	16	0.0662	1.4344
GO_MESENCHYMAL_CELL_DIFFERENTIATION	15	0.0684	1.4328
GO_ANTIOXIDANT_ACTIVITY	16	0.0684	1.4530
GO_REGULATION_OF_PROTEIN_POLYMERIZATION	40	0.0713	1.3524
GO_GLUCOSE_METABOLIC_PROCESS	23	0.0724	1.4297
GO TERM Gene ontology annotations unibiasedly found using GSEA 4.1.0
Size Number of genes (proteins) annotated per GO Term
NOM p-val P-value for GO Term enrichment
NES Normalized enrichment score for each GO term. Positive enrichment means enrichment in hFLO.

In FA, however, the top significantly upregulated GO-Terms are negative regulation of signaling and metabolism (FIG. 4F and Table S3).

TABLE S3
GO_TERM	SIZE	NOM p-val	NES
GO_REGULATION_OF_PROTEIN_DEPHOSPHORYLATION	15	0.0018	−1.7795
GO_PROTEIN_CONTAINING_COMPLEX_LOCALIZATION	34	0.0034	−1.7046
GO_ION_CHANNEL_BINDING	21	0.0035	−1.9105
GO_RNA_BINDING	327	0.0056	−1.4074
GO_REGULATION_OF_DEVELOPMENTAL_GROWTH	24	0.0071	−1.6707
GO_REGULATION_OF_PHOSPHATASE_ACTIVITY	15	0.0073	−1.8296
GO_POSITIVE_REGULATION_OF_PROTEIN_METABOLIC_PROCESS	131	0.0092	−1.4571
GO_NEGATIVE_REGULATION_OF_BIOSYNTHETIC_PROCESS	110	0.0096	−1.4693
GO_NEGATIVE_REGULATION_OF_RNA_BIOSYNTHETIC_PROCESS	80	0.0113	−1.5377
GO_NEGATIVE_REGULATION_OF_TRANSCRIPTION_BY_RNA_POLYMERASE_II	45	0.0116	−1.5605
GO_POSITIVE_REGULATION_OF_DEVELOPMENTAL_GROWTH	17	0.0119	−1.6527
GO_REGULATION_OF_DEPHOSPHORYLATION	19	0.0120	−1.7613
GO_MICROTUBULE_CYTOSKELETON_ORGANIZATION_INVOLVED_IN_MITOSIS	22	0.0142	−1.6419
GO_MITOTIC_SPINDLE_ORGANIZATION	21	0.0145	−1.6805
GO_POSITIVE_REGULATION_OF_PROTEIN_KINASE_ACTIVITY	32	0.0152	−1.6073
GO_POSTTRANSCRIPTIONAL_REGULATION_OF_GENE_EXPRESSION	106	0.0203	−1.4663
GO_ESTABLISHMENT_OF_RNA_LOCALIZATION	37	0.0219	−1.5196
GO_TRANSCRIPTION_REGULATOR_ACTIVITY	68	0.0228	−1.4866
GO_REGULATION_OF_ORGANELLE_ASSEMBLY	21	0.0250	−1.5159
GO_MULTICELLULAR_ORGANISMAL_SIGNALING	18	0.0260	−1.5848
GO_NEGATIVE_REGULATION_OF_SIGNALING	104	0.0262	−1.4008
GO_REGULATION_OF_GROWTH	49	0.0274	−1.4870
GO_REGULATION_OF_MRNA_CATABOLIC_PROCESS	53	0.0276	−1.4930
GO_POSITIVE_REGULATION_OF_ION_TRANSMEMBRANE_TRANSPORT	19	0.0286	−1.6010
GO_POSITIVE_REGULATION_OF_PHOSPHORUS_METABOLIC_PROCESS	72	0.0288	−1.4360
GO_POSITIVE_REGULATION_OF_CELLULAR_BIOSYNTHETIC_PROCESS	145	0.0293	−1.3436
GO_NUCLEOBASE_CONTAINING_COMPOUND_TRANSPORT	37	0.0296	−1.4891
GO_POSITIVE_REGULATION_OF_TRANSMEMBRANE_TRANSPORT	20	0.0307	−1.5214
GO_REGULATORY_REGION_NUCLEIC_ACID_BINDING	38	0.0315	−1.4866
GO_POSITIVE_REGULATION_OF_NUCLEOBASE_CONTAINING_COMPOUND_METABOLIC_PROCESS	128	0.0320	−1.3373
GO_REGULATION_OF_MRNA_METABOLIC_PROCESS	81	0.0350	−1.4188
GO_AMIDE_BIOSYNTHETIC_PROCESS	137	0.0351	−1.3610
GO_PROTEIN_N_TERMINUS_BINDING	17	0.0361	−1.5657
GO_MUSCLE_CONTRACTION	35	0.0362	−1.4040
GO_RNA_3_END_PROCESSING	23	0.0366	−1.5343
GO_TRANSCRIPTION_COREPRESSOR_ACTIVITY	17	0.0376	−1.5174
GO_MRNA_METABOLIC_PROCESS	176	0.0377	−1.3201
GO_HEAD_DEVELOPMENT	50	0.0385	−1.4241
GO_NEGATIVE_REGULATION_OF_NUCLEOBASE_CONTAINING_COMPOUND_METABOLIC_PROCESS	109	0.0387	−1.3646
GO_CIS_REGULATORY_REGION_SEQUENCE_SPECIFIC_DNA_BINDING	22	0.0401	−1.5646
GO_CARDIAC_CONDUCTION	16	0.0406	−1.5525
GO_PEPTIDE_BIOSYNTHETIC_PROCESS	129	0.0410	−1.3464
GO_SINGLE_STRANDED_RNA_BINDING	17	0.0427	−1.4995
GO_REGULATION_OF_INTRINSIC_APOPTOTIC_SIGNALING_PATHWAY	30	0.0453	−1.4904
GO_REGULATION_OF_SMALL_MOLECULE_METABOLIC_PROCESS	47	0.0455	−1.4056
GO_REGULATION_OF_CATION_TRANSMEMBRANE_TRANSPORT	26	0.0467	−1.4652
GO_POSITIVE_REGULATION_OF_GROWTH	24	0.0468	−1.4482
GO_POSITIVE_REGULATION_OF_CATALYTIC_ACTIVITY	111	0.0477	−1.3554
GO_POSITIVE_REGULATION_OF_TRANSFERASE_ACTIVITY	44	0.0477	−1.4221
GO_PHOSPHATASE_BINDING	17	0.0492	−1.4578
GO TERM Gene ontology annotations unibiasedly found using GSEA 4.1.0
Size Number of genes (proteins) annotated per GO Term
NOM p-val P-value for GO Term enrichment
NES Normalized enrichment score for each GO term. Negative enrichment means enrichment in FA.

We selected a few relevant up-regulated GO-Terms including anatomical structure formation involved in morphogenesis (GO: GO:0048646, NES=1.477), cellular carbohydrate metabolism (GO: GO:0005975, NES=1.814), and tube morphogenesis (GO: GO:0035239, NES=1.475) for further interrogation of each gene set (FIG. 4G). Additionally, we included a downregulated process, intrinsic apoptotic signaling pathway (GO: GO:0097193, NES=−1.490) in this interrogation (FIG. 4G). These data support our previous observations that the supplementation of soluble ECM promotes cell survival and the formation of organotypic structures in hFLO triculture aggregates.

3.5. hFLO Accurately Models Pulmonary Fibrosis and Vascular Development

There is a critical need for viable organotypic models for the human lung to model diseases including pulmonary fibrosis (PF). In order to fill this need, we induced fibrosis using bleomycin in our hFLO model. Bleomycin-induced PF is an extensively used animal-based model for fibrosis, despite significant cellular and molecular differences between mouse and human lungs. Moreover, therapeutics against PF are limited due to lack of organotypic lung models adapted for drug testing and screening. Translation animal therapeutic research revealed the promise of rho-associated protein kinase (ROCK) inhibition in the reversal of bleomycin-induced lung fibrosis. This therapy, however, has not yet been validated in a human lung model. Here, we grew hFLO for 7 days and induced fibrosis using 20 μg mL−1 bleomycin for 3 days, after which aggregates were treated with 10 μM fasudil, a ROCK inhibitor for 4 days to observe possible changes in fibrosis (FIG. 5A). Since we did not include bleomycin from day 10-14 of culture, the effects observed in the bleomycin treatment are most likely the result of the irreversible effects within that timeframe. In PF, there is an observed alveolar and bronchiolar epithelial cell death and fibroblast abundance. We observed that with bleomycin induction, there was a decrease in the epithelial A549 with an increase in fibroblast HFL1 population (FIG. 15B). Moreover, we observed decreased lumen area in bleomycin-treated aggregates which is rescued by the fasudil treatment (FIG. 15C).

We used immunohistochemistry to ascertain whether fasudil treatment leads to decreased expression of common fibrotic markers, including collagen deposition, expression of stress fiber marker αSMA, ECM marker fibronectin, and fibroblast marker PDGFRα. We observed and quantified decreased intensity of collagen deposition using Masson staining in organoids treated with fasudil (FIGS. 5B and 15D). Moreover, the increased pro-fibrotic expression after bleomycin insult was lowered after fasudil treatment (FIGS. 5C-5E and 15D). Localization of these markers also led to the identification of fibroblastic-myofibroblastic foci in the aggregates, another histopathological feature of IPF (FIGS. 5C-5E).

To further confirm the fibrosis in hFLO-bleomycin fibrotic model and the anti-fibrotic effects of fasudil, we collected culture media from the aggregates and performed a cytokine array using 120 common inflammatory factors. Among these, we found that 68 factors were significantly increased by the bleomycin treatment (Control vs Bleomycin, FIG. 5D & Table S6).

TABLE S6
Primary antibodies and Stains
Antibody			Catalog	Dilution
(Anti-)	FIGS.*	Source	number	(Application**)
Fibronectin	F5, EF5,	ProteinTech	66042-1-Ig	1:200 (IF)
	EF8			1:200 (IHC-HRP)
Vimentin	F1	Cell Signaling Technology	D21H3	1:100 (IF)
PDGFRβ	F3, F6,	Cell Signaling Technology	3169	1:100 (IF)
	EF9			1:100(FC)
PDGFRα	F5, EF8	Cell Signaling Technology	3174	1:1000 (IHC-HRP)
αSMA	F3, F5,	Cell Signaling Technology	48938	1:200 (IF)
	F6, EF8,			1:200 (FC)
	EF9			1:200 (IHC-HRP)
ECadherin	EF1	Cell Signaling Technology	3195	1:200 (IF)
NCadherin	EF1	Thermo Fisher Scientific	33-3900	1:150 (IF)
				1:150 (FACS)
EPCAM	F1	Developmental Studies	G8.8	1:50 (IF)
		Hybridoma Bank
Pro-SPC	F1	Abcam	ab40879	1:250 (IF)
PDPN	F1	Thermo Fisher Scientific	14-5381-82	1:100 (IF)
Desmin	F3	Invitrogen	14-9647-82	1:100 (IF)
				1:100 (FC)
Rhodamine	F3, F6,	Vector Laboratories	RL-1062-2	1:100 (IF)
UEA1	EF9
Cleaved	F2,	Cell Signaling Technology	9661	1:800 (MIFC)
Caspase-3
(Asp175)
Streptavadin-	EF5	Biotium	29037	1:500 (IF)
CF ™633
*F = Figure; EF = Extended Figure
**IF = Immunofluorescence; FC = Flow Cytometry; FACS = Flow-Activated Cell Sorting; MIFC = Multispectral Imaging Flow Cytometry; IHC-HRP = Immunohistochemistry-Horseradish Peroxidase

While 56 factors were significantly changed associated with the fasudil treatment (Fasudil vs Bleomycin) and 36 factors between control and fasudil treatment (FIG. 5D). Among these significantly secreted factors, 51 are common between the factors enriched by bleomycin insult and the factors that are changed by fasudil treatment. Upon data reduction using principal component analysis, we observed a closer clustering of the fasudil-treated fibrotic aggregates with the control (vehicle, DMSO-treated) aggregates but not with the bleomycin-insulted aggregates (FIG. 5E). This is further supported by hierarchical clustering showing the association of the fasudil-treated aggregates with the normal, non-fibrotic aggregates in a single clade, while the bleomycin-treated hFLOs are grouped separately (FIG. 5F). This shows very similar patterns of cytokine secretion were observed in the control and fasudil-treated fibrotic aggregates. Upon close examination of these secreted factors, we observed that pro-inflammatory and pro-angiogenic factors increase in bleomycin treatment. Fasudil treatment significantly decreased these pro-inflammatory factors associated with tissue fibrosis including: CX3CL1, AREG, CCL3, IL4, IL2, AXL, EGF, and IL6 among others (FIG. 5F). Moreover, we observed increased secretion of pro-angiogenic factors including FGF2 and VEGFA in bleomycin-insulted aggregates which is then decreased with fasudil treatment. These results suggest that hFLO can accurately model certain fibrotic features in vitro and potentially evaluate pre-clinical anti-fibrotic drugs, as illustrated here with fasudil.

We then looked into another application of hFLO, a model for hypoxia-induced angiogenesis that can mature to full perfusability. Blood vessel formation is an important process that affects several lung diseases including cancer and pulmonary hypertension. Previous vascular organoid methods use of hypoxia (5% O2) and supplementation of proangiogenic factors vascular endothelial growth factor (VEGF) and fibroblasts growth factor 2 (FGF2) to induce vascular endothelial branching, differentiation and maturation. Thus, at day 7, hFLO was treated with 60 ng mL−1 FGF2 and 60 ng mL−1 VEGF and cultured in 5% O2 (FIG. 6A). Hereafter, we will refer to the hFLO treated with FGF2 and VEGF under hypoxia as the vascular hFLO (vhFLO). In vhFLO, we observed hallmarks of lung development such as the increased prevalence of lumen and increased aggregate size with FGF2 and VEGF treatment under hypoxia when compared to hFLO (FIGS. 6A-6B). We also observed an increase in EAhy population volume and junction formation in vhFLO (FIGS. 6C and 16A-16C). We then tested whether this increase in EAhy resulted in improved vascular branching and maturation. Immunostaining revealed increased prevalence of αSMA+networks (FIG. 6D). 3D confocal imaging revealed luminal tube-like formation of UEA1+ endothelial cells with pericyte-like (PDGFRβ+) and smooth muscle-like (αSMA+) cells surrounding the abluminal side (FIG. 6E).

An important feature of a mature vasculature is perfusability. We created a PEGDA biocompatible 3D-printed chip to assess vascular perfusability using 70 kDa Dextran (FIGS. 6F and 17A-17E). Upon fluidic exposure to fluorescent 70 kDa Dextran, we observed that hFLO and vhFLO had perfusable regions while A549 and FA spheroids did not (FIGS. 6G-6H). Among these, vhFLO has the highest perfusable volume, with a 27-fold and 2.7-fold increase from FA and hFLO, respectively. In vhFLO and hFLO, the perfusion was localized with EAhy cells suggesting that perfusion is targeted to vascular-like regions (FIG. 6G). These data show that vasculature in hFLO is perfusable and exposure to hypoxia and pro-angiogenic growth factors increase the perfusability of the aggregates, as observed in vhFLO. These findings open additional avenues for the adaptation of hFLO in vascular modeling and angiogenic diseases such as pulmonary hypertension/vasculopathy and in lung cancer.

4. Discussion

The role of the ECM in organotypic structures has been extensively studied but research is limited when it comes to the roles and use of soluble ECM. Previous organ model research focused on the constructive (adhesion and architectural biomaterial) and instructive (cell signaling) roles of the ECM as effect of its solid hydrogel form. Regarding its instructive roles, the ECM is a known agonist to various receptors which activate mechanotransduction pathways responsible for organotypic growth, survival, and development. We questioned whether these known organotypic effects of the ECM are true even in its soluble form. To study this possibility, we developed a novel hybrid suspension culture that features organotypic growth instead of the typical compacted spheroid morphology with the help of soluble ECM. To show the efficacy of this novel 3D method, we introduced soluble ECM (growth factor reduced Matrigel) to a triculture of epithelial, endothelial, fibroblast cells. With this new methodology, an organotypic lung vascular alveolar model was derived using stable cell lines. After 14 days in our soluble ECM triculture, we observed various cell populations including type I-like (Pdpn+), type II-like (SPC+, lamellar body+) alveolar epithelial cells, mesenchymal cell populations including fibroblasts, endothelial cells, pericyte-like (PDGFRβ+), and smooth muscle-like cells (αSMA+, desmin+) cells. Moreover, the distribution of these cells was similar to that of the alveolus and the blood vessels. Early studies and recent advancements in single cell RNA sequencing show that these cell types populate the lung alveolus and the associated mesenchyme and vasculature.

Other novelties of this research include: 1) formation of organotypic luminal structures in a suspension culture where normally, cells form compact tissue-like spheroids; 2) effects of soluble ECM in 3D growth, cell survival, and long-term structure maintenance; 3) the first perfusable vasculature in an organotypic lung model; and 4) creation of a high-throughput bleomycin lung alveolus model along with human cell-based pre-clinical study of an anti-fibrotic drug.

Recently, a study illustrated the use of a soluble ECM, tropoelastin in promoting growth and survival of mesenchymal stem cells in 2D culture. Another study showed that soluble collagen VI is able to prevent apoptosis in serum-starved fibroblasts. These pro-survival effects of soluble ECM, however, have not been demonstrated in 3D culture. Within the field of 3D culture, overcoming cell death is vital to create viable cell aggregates capable of sustaining long term growth. Here, we present evidence that soluble ECM improves cell survival in 3D suspension culture. During the 14-day culture, proteomic data gives insights on the feasible pro-survival mechanism of the soluble ECM to be hinged on increased carbohydrate metabolism and the prevention of anoikis, two processes that are well-studied effects of solid ECM. Our growth assays suggest that culture in soluble ECM allows for long-term survival and structural maintenance of cell aggregates up to 70 days of culture. The ability of 3D models to be maintained for an extended period of time is essential in studying long-term processes such as organ maturation, disease resolution, and aging among others. We believe that our finding is the first account to show the pro-survival effects of non-solid ECM in 3D multicellular aggregates.

One of the major features that sets organoids apart from spheroids is the presence of central lumen that is essential in organs for their specialized functions. In the lung, the alveolar lumen is populated by type I and type II epithelial cells that facilitate gas exchange and pressure regulation, respectively. Moreover, lumen formation is not just confined to the epithelium but is also observed in the vasculature which allows for efficient material circulation. In the hFLO, we observed both types of lumina formed via immunochemistry, histology, and electron microscopy. In the epithelial lumen, we observed the presence of multilamellar body-presenting type II-like cells in close proximity to long, slender type I-like cells. Moreover, upon close examination, we also observed that adjacent to these epithelial cells and separated by a basement membrane are luminal endothelial cells (LECs). Further, immunostaining and flow cytometry revealed that at least three types of cells inhabit these lumina—endothelial cells, pericytes, and vascular smooth muscles.

Current stable cell suspension co-cultures lack the presence of perfusable and branching vasculature, thus, these cell culture methods are only capable of recapitulating compacted organization and are growth-limited due to poor material circulation. In the presence of solid ECM endothelial cells alone form networks and co-culture with fibroblast cells result in lumen formation of endothelial cells. In soluble ECM culture, we show that endothelial cells only form networks in the presence of fibroblasts. Additionally, these endothelial-fibroblastic branching networks express perivascular cell markers. This observed vascularization followed by maturation into functioning perfusable tubular networks is vital for material circulation and for epithelial-endothelial interaction to form. During endothelial tube formation, fibronectin (FN) is required, and its organization into fibrils initiates vascular tube formation. Matrigel promotes FN fibrillogenesis only when it is immobilized and not in its soluble form. In our model, we observed FN fibrillogenesis even with the use of soluble Matrigel due to the immobilization and incorporation of the soluble ECM into the aggregate. This immobilization magnifies the assembly of fibronectin into fibrillar structures, alluding to the instructive role that the immobilized ECM has in fibril assembly. These vascular interactions are the basis of the alveolar gas exchange unit, thus the importance of these results become clear.

Recent developments in tissue engineering led to the creation of induced pluripotent stem cell (iPSC)-derived lung organoids. These organoids show high-fidelity in mimicking organ development, and have a high potential for use in disease modeling and subsequent drug development. Moreover, these iPSC-derived lung organoids show high organotypic complexity with multiple types of cells from various lung regions including the bronchi and the alveolus. Though directed differentiation of iPSC-derived organoids is a laborious process which takes on average over 50 days, involves several culture transfers, and requires multiple growth factors. In contrast, hFLO features a minimalistic methodology and a 14-day culture time to produce aggregates with organotypic lung alveolar markers. This characteristic makes this model adaptable for automated downstream high throughput studies. These features also make hFLO a feasible and important tool for time-sensitive disease modeling like the COVID-19 pandemic or future respiratory pandemics. Moreover, the lack of a perfusable vasculature in iPSC derived organoids limit their expansion and their use in vascular lung disease research. We posit that the use of the basic vascular unit described in this paper is vital in the improvement of current epithelial organoids in expanding their growth and stability via co-culture.

To illustrate a disease modeling application of hFLO, we used bleomycin induction to model lung fibrosis. Bleomycin promotes inflammation and formation of fibrotic lesions with similar biochemical and morphological features in patients with IPF and other fibrotic lung disorders. Histopathological and biochemical patterns of usual interstitial pneumonia (UIP), the hallmark feature of IPF include: epithelial injury leading to disrupted basement membrane (ie. increased collagen deposition), loss of airspaces, presence of dominant fibroblastic foci, and increased mesenchymal markers. We found that bleomycin induction in hFLO resulted in increased collagen deposition implying disruption in the basement membrane. The bleomycin-treated hFLO organoids had decreased air space-like gas exchange units as shown through lumen analysis, presence of fibrotic foci and increased mesenchymal markers. Moreover, the aberrant cytokine secretion in the hFLO-bleomycin is enriched with pro-inflammatory cytokines implicated in fibrosis, especially in PF; these includes CX3CL1, AREG, CCL3, IL4, IL2, AXL, EGF, and IL6 among others. Our observations demonstrate that the hFLO-bleomycin fibrotic model not just recapitulates alveolar histopathological features of PF, but also the associated pro-fibrotic, inflammatory cytokine secretion. Together, these results suggest that the bleomycin induction in hFLO successfully achieved fibrosis and is irreversible during the timeframe but was ameliorated by fasudil treatment. The application of this innovative method closely replicates multiple features in patients with PF and since hFLO is a human in vitro model, it has the potential to replicate disease pathogenesis and drug interactions that current animal models are unable to show.

We chose to test our human lung fibrosis model with fasudil, a ROCK inhibitor clinically used to treat cerebral vasospasm in Japan and China, but not yet approved in the United States. Fasudil was found effective in resolving PF symptoms in traditional 2D in vitro and in vivo mouse studies. However, lack of data in a human model of the disease precludes further investigation and fasudil's potential adoption as a human PF treatment. Our results show that fasudil improved the above-mentioned PF pathologies present in the hFLO-bleomycin model. Moreover, the highly similar cytokine secretion of fasudil-treated fibrotic organoids to non-disease hFLO indicate the reversal of the inflammatory fibrotic effects of bleomycin. These results may also open the door to pre-clinical trials of existing ROCK inhibitors such as Y27632 and the development of other ROCK inhibitors. Further isoform-specific ROCK inhibition studies are needed for more fine-tuned targeting of the disease. We view the hFLO-bleomycin model to be an important tool that could be used in high-throughput drug screens for PF and related diseases.

To further improve upon the hFLO, we mimicked developmental lung angiogenesis through a combination of pro-vascular growth factors (VEGF, FGF2) and a hypoxic environment (5% O2), creating vhFLO, which has more perfusable volume than hFLO. This adds additional physiologically relevant characteristics for researchers to utilize in the study of alveoli-vascular interactions. Our research demonstrates that soluble ECM suspension promotes the formation of a viable vascular lung organoid; further research needs to be completed to further understand the capabilities and limitations of this method. We identify the following steps to better understand the capabilities of the system: (1) the utilization of a precise serum free, chemically defined media to develop the organoids; (2) the utilization of primary alveolar epithelial cells or adult lung progenitor and stem cells; (3) profiling of all the cell types in the hFLO via single cell RNA sequencing; and (4) formation of macroscopic tissue constructs using hFLO as the building block. We illustrated several novelties of our methodology leading to the creation of a human PF bleomycin model, which shows a closer approximation to distal lung than has been shown to date for PF in vitro modeling.

5. Conclusions

Our hybrid soluble ECM-based 3D culture method promotes organotypic growth using stable mature cells within 14 days of culture. We illustrate that soluble ECM can be used to enhancing 3D growth and survival in suspension cultures. We believe that this is the first account illustrating that soluble ECM can create an organotypic lung model from mature stable cells. Moreover, the lung model presented in this paper has a perfusable vasculature which current lung organoids lack. We demonstrate the utility of the novel hFLO model provide further insights in the pathogenesis of PF. The organotypic features of this model allowed us to mimic PF and demonstrate its resolution using a ROCK inhibitor, fasudil. The application of this method in the formation of patient- or primary-derived organoids is yet to be performed but will be necessary to create high-throughput screens for personalized medicine. Our findings open an avenue for novel tissue engineering using soluble ECM and the application of the hFLO in modeling lung diseases such as PF and COVID-19.

Various aspects are described above with reference to the drawings. The relationship and functioning of the various elements of the aspects may better be understood by reference to the following detailed description. However, aspects are not limited to those illustrated in the drawings or explicitly described below. It should be understood that the drawings are not necessarily to scale, and in certain instances, details may have been omitted that are not necessary for an understanding of aspects disclosed herein, such as conventional fabrication and assembly. Headings are provided for the convenience of the reader and to assist organization of the disclosure and should not be construed to limit or otherwise define the scope of the invention.

Claims

1. A cell culture for obtaining an organoid, the cell culture comprising: epithelial cells or tissue fragments comprising the epithelial cells,endothelial cells or tissue fragments comprising the endothelial cells,fibroblast cells or tissue fragments comprising the fibroblast cells, andsoluble extracellular matrix proteins.

2. An in vitro method for obtaining an organoid, the comprising: culturing a mixture of (a) epithelial cells or tissue fragments comprising the epithelial cells, (b) endothelial cells or tissue fragments comprising the endothelial cells, (c) fibroblast cells or tissue fragments comprising the fibroblast cells, and (d) soluble, non-gelling concentration of extracellular matrix proteins.

3. An organoid obtained by the method according to claim 2.

4. The cell culture of claim 1, wherein the epithelial cells are A549.

5. The cell culture of claim 1, wherein the endothelial cells are EAhy.

6. The cell culture of claim 1, wherein the fibroblast cells are HFL1.

7. The cell culture of claim 1, further comprising basement membrane proteins.