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    Syngeneic implantation of mouse hepatic progenitor cell-derived three-dimensional liver tissue with dense collagen fibrils

    2022-06-11 07:37:44MihoTamaiEijiroAdachiMasayaKawaseYohichiTagawa
    World Journal of Gastroenterology 2022年14期

    Miho Tamai,Eijiro Adachi,Masaya Kawase,Yoh-ichi Tagawa

    Abstract

    Key Words: Liver; Three-dimensional tissue culture; Hepatic progenitor cells; Angiogenesis; Biomimetic extracellular matrix

    INTRODUCTION

    Liver transplantation is a therapy for irreversible liver failure; however, donor organs are currently in short supply[1 ,2 ]. Cell transplantation therapy for liver failure is still at the developmental stage and has a critical problem in terms of a shortage of human primary hepatocytes[3 ]. Human embryonic stem/induced pluripotent stem (ES/iPS) cell-derived hepatocytes are thought to be an alternative to human primary hepatocytes, but ES/iPS cells are difficult to differentiate into mature hepatocytes in culture[4 ,5 ]. ES/iPS cell-derived immature hepatocytes successfully developed into mature liver tissue in animals after implantation[6 ,7 ]. However, this process requires a great deal of time, effort, and expense in order to obtain a sufficient number of ES/iPS cell-derived hepatocytes in culture to achieve the amount needed for them to continue to proliferate. There have been several reports of rat HPCs,such as small hepatocytes[8 ] and Lgr5 + rat and mouse liver stem cells[9 ,10 ], becoming established in culture. These hepatic stem/progenitor cells have the ability to proliferate and differentiate into hepatocytes and cholangiocytes[11 ,12 ]. Recently, we also succeeded in establishing HPC lines prepared from the portal branch-ligated hepatic lobe in mice (PBL-HPCs)[13 ]. These cells could differentiate into mature hepatocytes in the presence of oncostatin M, or to cholangiocytes in EHS gel.

    Besides dissociated hepatocyte implantation, regenerative medicine is also expected to enable the implantation of extracellular matrices containing aggregate, or organoids consisting of hepatocytes and non-parenchymal cells[14 -16 ].In vitroliver organoid tissue has previously been generated by accumulating collagen fibrils, human fibroblast cell line (HFO cell), and human hepatocarcinoma cell line (Hep G2 ) on a mesh of polylactic acid (PLA) fabric using a bioreactor[14 ]. Also, instead of HFO and Hep G2 ,mouse embryonic fibroblasts and primary hepatocytes were used for thisin vitroliver organoid tissue.Thesein vitroliver organoid tissues generated transplantable liver organoid tissues in the right portal vein branch-ligatednu/numouse with a condensed collagen fibril matrix[14 ]. The fibroblasts are embedded in the network collagen fibrils of this artificial tissue, and it is therefore useful for reconstructing the hepatic interstitial structure.

    In this study, the PBL-HPCs were expanded and formed liver organoid tissue, which was comparable to liver lobules using an originally designed bioreactor system, and was also implanted into its syngeneic wild-type mouse.

    MATERIALS AND METHODS

    Animals

    Pregnant BALB/cA mice at 13 .5 d post-coitus (CLEA Japan, Tokyo, Japan) were used for embryonic fibroblast isolation. Six-week-old female and male BALB/cA Jcl and BALB/cA Jcl-nu/nu 3 mice (CLEA Japan, Tokyo, Japan) were used as transplant recipients. The animal protocol was approved by the Animal Experimentation Committee of the Tokyo Institute of Technology.

    Cells and cultures

    The PBL-HPCs were established in a previous study with portal vein ligated methods[13 ]. The cells were cultured in Williams’ E medium (GIBCO Laboratories, Grand Island, NY, United States) supplemented with 5 % fetal bovine serum, 10 mmol/L nicotinamide (Sigma-Aldrich, St. Louis, MO, United States), 0 .1 μmol/L dexamethasone (Sigma-Aldrich), 1 ×Insulin-Transferrin-Sodium Selenite Supplement(Roche Diagnostics, Mannheim, Germany), and 20 ng/mL Recombinant Mouse Epidermal Growth Factor (R&D Systems, Minneapolis, MN, United States) in 5 % CO2 at 37 °C. These cells were passaged by treatment with 0 .05 % trypsin (Invitrogen) and 20 μmol/L ethylenediaminetetraacetic acid (EDTA;NACALAI TESQUE, Kyoto, Japan).

    Preparation of murine embryonic fibroblasts

    A pregnant female BALB/c mouse at 13 .5 dpc (days post-coitus) was sacrificed by cervical dislocation,and embryos were removed. The limbs of the embryos were minced and treated with 0 .25 % trypsin(Invitrogen, Tokyo, Japan) + 1 mmol/L EDTA (about 2 mL per embryo) and incubated with gentle stirring at 37 °C for 10 -15 min. The cells were subsequently cultured in DMEM containing 10 % (v/v)FBS.

    Generation of three-dimensional liver tissue culture model

    As shown in Figure 1 , the three-dimensional (3 -D) liver tissue culture model was generated by accumulating collagen fibrils, primary murine embryonic fibroblasts, and PBL-HPCs using a closed-loop system with a bioreactor chamber (diameter 17 mm; thickness 20 mm) developed by our group as previously reported[14 ,17 ]. Briefly, primary embryonic fibroblasts (1 .0 × 105 cells/mL) in 10 % FBS and 7 .5 mg/mL type I collagen prepared from calfskin (Koken Collagen, Tokyo, Japan) in Williams’ E medium flowed through the closed-loop system at a predetermined flow rate (1 -5 mL/min) for 6 h. Subsequently, the same medium was circulated through the closed-loop system, and PBL-HPCs (5 .0 × 106 cells/mL) were injected using a syringe into the system upstream of the bioreactor chamber for 2 h. Finally, a suspension of fibroblasts (1 .0 × 105 cells/mL) was circulated for 6 h.

    Morphological analyses

    The 3 -D liver tissue culture models were fixed with Zamboni’s fixative for light microscopy. The samples were dehydrated with an ethanol series and embedded in paraffin. The sections were stained with hematoxylin and eosin or AZAN and examined with a light microscope.

    Hepatic function assay in liver tissue culture model

    Urea production in the medium was quantified using a urea assay kit (Bioassay Systems, Hayward, CA,United States) 24 h after the addition of 2 mmol/L NH4 Cl. Albumin production was quantified in the medium using an albumin EIA (Albuwell M) mouse kit (Exocell, Philadelphia, PA, United States).

    The metabolites of testosterone in the medium were quantified by HPLC analysis[18 ]. The 3 -D liver tissue culture models were incubated with fresh medium containing 0 .25 mmol/L testosterone and the medium was collected at 24 h. After sample treatment, HPLC analysis was performed using LC-10 ADVP (Shimadzu, Kyoto, Japan) with Cadenza columns (Cadenza CD-C18 ) (Imtakt, Kyoto, Japan)and SPD-10 A VP (Shimadzu, Kyoto, Japan).

    Transplantation of liver tissue culture model

    Under isoflurane anesthesia, mice were subjected to an upper-abdominal incision, followed by exposure and ligation of the left portal vein branch and subsequent hepatectomy of the left and middle lobes(70 %). The 3 -D liver tissue culture model was transplanted into the subcutaneous layer of a mouse. Two weeks later, the 3 -D liver tissue culture model was removed for histological analysis of the vascular network.

    Statistical analysis

    Results of multiple experiments were reported as the mean ± SE. Statistical comparisons were made using a Tukey-Kramer method and a Welcht-test using the IBM SPSS Statistic 27 .

    Figure 1 Reconstruction of the three-dimensional liver tissue culture model using hepatic progenitor cells. A and B: A schematic illustration showing reconstruction of the liver tissue culture model using a bioreactor; preparation steps (A), and culture steps (B); C: Micrographs of a reconstructed threedimensional (3 -D) liver tissue culture model with dense collagen fibrils; D and E: Histological analyses: hematoxylin-eosin staining of a section of the 3 -D liver tissue culture model on day 1 (D) and day 12 (E). Arrows indicate binuclear populations, like hepatocytes. Arrowheads indicate a bile duct-like structure; F: Histological analyses: AZAN staining of a section of the 3 -D liver tissue culture model on day 12 . Arrowheads indicate fibroblasts at condensed collagen fibril matrices. Bar corresponds to (C) 5 mm, (D) 50 μm, and (E) and (F) 100 μm. Col: Collagen; HPCs: Portal branch-ligated-hepatic progenitor cells; PLA-S: Polylactic acid sheet; C:Collagen layer; H: Hepatic layer.

    RESULTS

    Preparation of 3 -D hepatic progenitor cell-derived 3 -D liver tissue culture model

    Type I collagen solution was circulated through a sheet of PLA into a reverse radial flow-type bioreactor, followed by the suspension of 5 .0 × 106 cells of mouse embryonic fibroblasts (MEFs). In the next step, the suspension of 1 .0 × 107 PBL-HPCs was circulated without oncostatin M. After these steps,the type I collagen solution was circulated again followed by the suspension of 5 .0 × 106 MEFs. Finally a 3 -D aggregate was prepared (Figure 1 A). The surface of this 3 -D aggregate which included PBL-HPCs,primary fibroblasts, and type I collagen was glossy and measured 17 mm in diameter and 1 .5 mm in height. This glossy aggregate consisted of a layer of PBL-HPCs, sandwiched between two layers of collagen fibrils with MEFs, and was constructed on a sheet of PLA as shown in Figure 1 G. Crosssectional profiles of the 3 -D liver tissue culture models were stained with hematoxylin-eosin and AZAN as shown in Figure 1 D-F. The collagen layers were composed of densely packed collagen fibrils running parallel to the plane of the PLA sheet. A layer of PBL-HPCs 200 -300 μm thick (Figure 1 D), and two layers of collagen fibrils populated with embryonic fibroblasts, approximately 400 μm thick, were observed in the 3 -D liver tissue culture model. To culture the 3 -D liver tissue model, the cylinder inside the bioreactor was changed from construction to culture (Figure 1 B). The 3 -D liver tissue culture model was cultured using a differentiation medium containing 20 ng/mL oncostatin M in the bioreactor for 12 d. After this, PBL-HPCs differentiated into mature hepatocyte-like cells, in binuclear populations, and with a bile duct-like structure (Figure 1 E). Collagen layers were maintained by the collagen fibers and fibroblasts on day 12 .

    Expression of liver-related genes in hepatic progenitor cell-derived 3 -D liver tissue culture model

    The expression of liver-specific genes was determined in the 3 -D liver tissue culture model. To investigate whether the 3 -D liver tissue culture models were able to show hepatic lineage differentiation(i.e., to mature into hepatocytes and bile duct cells), the cells were cultured in the presence of oncostatin M. By day 12 of the culture in the hepatic lineage differentiation medium, quantitative real-time polymerase chain reaction analysis revealed that the cells expressed hepatocyte differentiation markers including: Afp (α-fetoprotein); Albumin; Tat (tyrosine aminotransferase); Tdo (tryptophan 2 ,3 -dioxygenase); Cps1 (carbamoyl-phosphate synthetase 1 ); Cyp1 a2 (Cytochrome P450 , family 1 , subfamily a2 ); Cyp2 e1 (Cytochrome P450 , family 2 , sub-family e1 ); and Abcc2 [ATP-binding cassette, subfamily C (CFTR/MRP), member 2 ] (Figure 2 A-H). On the other hand, the gene expression ofBsep(bile salt export pump) andABCB11 (ATP-binding cassette, sub-family B member 11 ) decreased in the 3 -D liver tissue culture model (Figure 2 I). The expression of CK19 , a representative marker for HPCs, was confirmed in the PBL-HPCs. The gene expression ofCK19 decreased in the 3 -D liver tissue culture models (Figure 2 J). In addition, PBL-HPCs expressed the CD44gene, a progenitor cell marker, which decreased in the 3 -D liver tissue culture models (Figure 2 K). After that, CD44expression increased in the 3 -D liver tissue culture models on day 12 of culture (Figure 2 K).

    The 3 -D liver tissue culture model exhibits expression of multiple liver-specific functions

    The expression of several liver-specific functions, such as the production of urea and albumin, and drug metabolism, were analyzed in the 3 -D liver tissue culture models. Urea production was examined in cultured 3 -D liver tissue culture models in a hepatic lineage differentiation medium containing 2 mmol/L NH4+. The level of urea production in the 3 -D liver tissue culture model gradually increased and was significantly higher on days 6 and 12 than in the 2 -D culture (Figure 3 A). The amount of albumin released from the 3 -D liver tissue culture model into the medium was measured in each medium on day 1 , day 6 , and day 12 by enzyme-linked immunosorbent assay. As seen in Figure 3 B, the albumin level increased gradually from day 1 to day 12 . These results suggest that the 3 -D liver tissue culture model with PBL-HPCs had differentiated.

    To quantify P450 activities, the hydroxylated pattern of testosterone by cultured 3 -D liver tissue culture models in a hepatic lineage differentiation medium, containing 250 μmol/L testosterone, was examined using high-performance liquid chromatography. The concentration of each hydroxylated testosterone (6 β-OHT, 7 α-OHT, 16 α-OHT, and 16 β-OHT, respectively, corresponding to oxidation by Cyp3 a, Cyp2 a4 /5 and 2 d9 , Cyp2 d9 and 2 b, and Cyp2 c29 and 2 e) was quantified. The concentrations of hydroxylated testosterones, such as 6 β-OHT, 7 α-OHT, 16 α-OHT, and 16 β-OHT, in the media of the 3 -D liver tissue culture models after 12 days culture were measured. As compared with the hydroxylation levels of 6 b-OHT, 7 a-OHT, and 16 a-OHT in the 2 -D culture, the hydroxylation levels were significantly increased in the 3 -D liver tissue models (Figure 3 C).

    The 3 -D liver tissue was engrafted in the partially hepatectomized mouse

    The 3 -D liver tissue culture model of PBL-HPCs was syngeneically transplanted into the subcutaneous layer of a BALB/cA mouse which had received a 70 % partial hepatectomy as shown in Figure 4 A. The graft could be observed in the subcutaneous layer two weeks after transplantation. Microvascular networks were seen throughout this engrafted tissue. As shown in Figure 4 B and C, the hematoxylineosin staining of this specimen in the graft area showed that collagen remained rich in the graft,fibroblasts existed in the collagen area, and vessel-like tube formation was observed. To investigate whether the cells in these areas were hepatocytes, an immunohistochemical examination using staining with anti-albumin antibodies was carried out (Figure 4 D). This confirmed that the PBL-HPCs were accepted as albumin-positive cells after transplantation. These results indicate that the 3 -D liver tissue culture model was successfully grafted with angiogenesis in the partially hepatectomized mouse.

    Figure 2 Relative gene expression levels in the three-dimensional liver tissue culture model cultured in a bioreactor on day 1 and day 12 .Relative gene expression levels were analyzed in the three-dimensional liver tissue culture model. A: Afp; B: Albumin; C: Tat; D: Tdo; E: Cps1 ; F: Cyp1 a2 ; G: Cyp2 e1 ; H: Abcc2 ; I: Bsep; J: CK19 ; K: CD44 . Hprt was used as an internal control. Statistical comparisons were made using the Tukey-Kramer method. Data are shown as means ± SE, n = 3 , aP < 0 .05 and bP < 0 .01 . Afp: Alpha-fetoprotein; Tat: Tyrosine aminotransferase; Tdo: Tryptophan 2 ,3 -dioxygenase; Cps1 : Carbamoyl-phosphate synthetase 1 ; Cyp1 a2 : Cytochrome P450 , family 1 , sub-family a2 ; Cyp2 e1 : Cytochrome P450 , family 2 , sub-family e1 ; Abcc2 : ATP-binding cassette, sub-family C(CFTR/MRP), member 2 ; Bsep: Bile salt export pump; ABCB11 : ATP-binding cassette, sub-family B member 11 ; CK19 : Cytokeratin 19 ; CD44 : Hyaluronic Acid Binding Protein.

    DISCUSSION

    Figure 3 Validation of hepatic functions in the three-dimensional liver tissue culture model. A and B: Urea (A) and albumin (B) production levels in the culture medium in each culture condition; C: Hydroxylation activity of testosterone in the three-dimensional (3 -D) liver tissue culture model. The amount of each hydroxylated testosterone in culture medium. Culture medium was changed every 2 d over the course of the measurement period. 2 -D culture (open columns) and 3 -D culture (closed columns) system. Statistical comparisons were made using the Welch t-test. Data are shown as means ± SE, n = 3 , aP < 0 .01 .

    It is crucial to develop a technology that enables transplantable engineered tissues to be functionally engrafted and long-lasting, in order to maximize the therapeutic effects of this procedure[19 -21 ]. There are reports of transplanted hepatocytes at several different extrahepatic sites such as the small intestine[22 ,23 ]. Tissue engineering has been a promising procedure for providing transplantable tissues mimicking liverex vivo[24 ,25 ]. The attachment of hepatocytes to extracellular matrix scaffolds can help in their engraftment in extrahepatic sites[26 ,27 ]. It is important to provide scaffold materials for hepatocytes to enable significantly greater hepatocyte survival in heterotypic transplantation[28 ]. The liver is encased mainly with collagen fibrils. By fabricating graded structures specific for target tissues and organs, one can obtain suitable scaffolds for tissue regeneration[29 ]. Taking into account the architecture of the liver, we have generated a 3 -D liver tissue culture model of HPCs with a collagen fibril matrix using a bioreactor. Furthermore, defining and validating new sources is mandatory for ensuring functional hepatic cell supply[30 ]. Hepatic stem/progenitor cells have many advantages compared to adult hepatocytes as they are bipotent cells, so they can differentiate into hepatocytes and cholangiocytes[20 ]. Moreover, they have high proliferation ability.

    In this study, HPCs — PBL-HPCs — were used in an original procedure to generate a 3 -D liver tissue culture model. The histological structure of this model resembled that of the liver, with respect to its capillary network and surrounding cell clusters. As PBL-HPCs have the potential to reproduce themselves, it is easy to prepare the necessary numbers of cells (1 × 107 cells order). The PBL-HPCderived 3 -D liver tissue culture model reconstructed in a bioreactor produced cells that differentiated into hepatic-like cells, binuclear populations, and bile duct-like structures (Figure 1 F). These cells expressed hepatocyte differentiation markers (Figure 2 ) after 12 days of culture. The PBL-HPCs differentiated not only into hepatic cells but also bile duct-like cells in a reconstituted collagen fibril matrix. In the 3 -D liver tissue culture model derived from PBL-HPCs, the levels of urea and albumin production were gradually enhanced and were significantly higher than those cultured in dishes on days 6 and 12 (Figure 3 A and B). Cyp3 a, 2 a4 /5 , 2 d9 , and 2 b activities were significantly increased in the 3 -D liver tissue culture models (Figure 3 C). These results suggest that the PBL-HPCs differentiated to mature hepatocytes in the 3 -D liver tissue culture model.

    Figure 4 Transplanted three-dimensional liver tissue culture models in partially hepatectomized model mice. A: A schematic illustration showing the transplantation of the three-dimensional (3 -D) liver tissue culture model; B: Histological analyses and hematoxylin-eosin staining of the section for the 3 -D liver tissue culture model after transplantation; C: Higher magnification of the inscribed area in (B). The vascularization was observable at condensed collagen fibril matrices. Arrowheads indicate new blood vessels; D: Immunohistochemical analysis of the 3 -D liver tissue culture model of albumin-positive hepatic cells after being transplanted using anti-albumin (green) antibodies. Bar corresponds to 100 μm.

    Since PBL-HPCs differentiated into cells expressing hepatic functions in a 3 -D liver tissue culture model, further investigation was carried out to determine whether PBL-HPCs also maintained their acquired functions after transplantation. Following implantation of the PBL-HPC-derived 3 -D liver tissue culture model into mice, the 3 -D liver tissue culture model was grafted, and vessel-like tube formation was observed (Figure 4 B and C).

    Also, the 3 -D liver tissue culture model was grafted in the healthy mouse which did not undergo partial hepatectomy, and vascularization was observed (Supplementary Figure 1 A and B). On the other hand, the Matrigel-embedded PBL-HPCs were transplanted into male healthy mice or nu/nu mice, and vascularization was not observed (Supplementary Figure 1 C-F). PBL-HPCs differentiated into albumin positive cells (Figure 4 D). This haptic tissue consisted of fibroblasts and HPCs which can be differentiated into only hepatocytes and bile duct cells, not immune cells. As some blood vessels were observed after implantation, lymphocytes and monocytes may have been circulating. However, we did not detect Kupffer cells in the grafts. The 3 -D liver tissue culture model was investigated for efficiency of transplantation in extrahepatic sites. These findings demonstrated that a reconstituted collagen fibril matrix can provide an extracellular microenvironment to promote the maturation of progenitor cells into hepatic cells. A local vascular network would allow nutrient and gas transport to the graft. These findings could make a significant contribution to the problem of liver graft shortage.

    CONCLUSION

    In conclusion, a 3 -D liver tissue culture model was developed using HPCs. The advantage of our system is that it consists of proliferative HPCs. The 3 -D liver tissue culture models can be generated in an originally designed bioreactor within 24 h. By mimicking the structure of the natural liver, our system was effective in constructing a functional liver tissue model.

    ARTICLE HIGHLIGHTS

    ACKNOWLEDGEMENTS

    The authors would like to acknowledge Sakai H and Miyagawa S (Department of Surgery, Shinshu University School of Medicine) for skillful technical assistance.

    FOOTNOTES

    Author contributions:Tagawa YI designed the study; Tamai M conducted all experiments; Kawase M performed statistical processing; Adachi E and Tagawa YI supervised the project; Tamai M and Tagawa YI wrote the manuscript; all authors read and approved the manuscript.

    Supported byGrants-in-Aid for Scientific Research (A), No. 25242040 (to Tagawa YI); Grants-in-Aid for Challenging Exploratory Research, No. 20 K21520 (to Tagawa YI); Grants-in-Aid for Early Career Scientists from the Japan Society for the Promotion of Science (JSPS), No. 19 K20655 (to Tamai M); Grant-in-Aid for Scientific Research on Innovative Areas from the Ministry of Education, Culture, Sports, Science and Technology of Japan (MEXT), No. 231190003 (to Tagawa YI); Japan Agency for Medical Research and Development (AMED), No. 20 fk0310102 (to Tagawa YI); and Building of Consortia for the Development of Human Resources in Science and Technology, Ministry of Education,Culture, Sports, Science and Technology, Japan (to Tamai M).

    Institutional animal care and use committee statement:All animal experiments conformed to the internationally accepted principles for the care and use of laboratory animals. All animal experiments were conducted in accordance with policies of the Animal Experimentation Committee of the Tokyo Institute of Technology Guide for the Care and Use of Laboratory Animals. Specific protocols used in this study were approved by the Animal Experimentation Committee of the Tokyo Institute of Technology (approved protocols are D2015009 , D2012019 and 2009024 -5 ).

    Conflict-of-interest statement:The authors declare no conflict of interest relevant to this manuscript.

    Data sharing statement:No additional data are available.

    ARRIVE guidelines statement:The authors have read the ARRIVE Guidelines, and the manuscript was prepared and revised according to the ARRIVE Guidelines.

    Open-Access:This article is an open-access article that was selected by an in-house editor and fully peer-reviewed by external reviewers. It is distributed in accordance with the Creative Commons Attribution NonCommercial (CC BYNC 4 .0 ) license, which permits others to distribute, remix, adapt, build upon this work non-commercially, and license their derivative works on different terms, provided the original work is properly cited and the use is noncommercial. See: http://creativecommons.org/Licenses/by-nc/4 .0 /

    Country/Territory of origin:Japan

    ORCID number:Miho Tamai 0000 -0001 -8016 -9663 ; Eijiro Adachi 0000 -0002 -0520 -5211 ; Masaya Kawase 0000 -0003 -4003 -4013 ; Yoh-ichi Tagawa 0000 -0002 -7673 -6781 .

    S-Editor:Gao CC

    L-Editor:Webster JR

    P-Editor:Guo X

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