CD203c is expressed by human fetal hepatoblasts and distinguishes subsets of hepatoblastoma

Marcus O Muench; Marina E Fomin; Alan G Gutierrez; Dolores López-Terrada; Renata Gilfanova; Christopher Nosworthy; Ashley I Beyer; Gregory Ostolaza; Dina Kats; Kevin L Matlock; Stefano Cairo; Charles Keller

doi:10.3389/fonc.2023.927852

CD203c is expressed by human fetal hepatoblasts and distinguishes subsets of hepatoblastoma

Front Oncol. 2023 Feb 9:13:927852. doi: 10.3389/fonc.2023.927852. eCollection 2023.

Authors

Affiliations

¹ Vitalant Research Institute, San Francisco, CA, United States.
² Department of Laboratory Medicine, University of California, San Francisco, San Francisco, CA, United States.
³ Department of Pathology and Immunology, Baylor College of Medicine, Houston, TX, United States.
⁴ Texas Children's Cancer Center, Texas Children's Hospital, Houston, TX, United States.
⁵ Pediatric Cancer Biology, Children's Cancer Therapy Development Institute, Beaverton, OR, United States.
⁶ Omics Data Automation, Beaverton, OR, United States.
⁷ Research and Development Unit, XenTech, Evry, France.

Abstract

Background & aims: Hepatocytic cells found during prenatal development have unique features compared to their adult counterparts, and are believed to be the precursors of pediatric hepatoblastoma. The cell-surface phenotype of hepatoblasts and hepatoblastoma cell lines was evaluated to discover new markers of these cells and gain insight into the development of hepatocytic cells and the phenotypes and origins of hepatoblastoma.

Methods: Human midgestation livers and four pediatric hepatoblastoma cell lines were screened using flow cytometry. Expression of over 300 antigens was evaluated on hepatoblasts defined by their expression of CD326 (EpCAM) and CD14. Also analyzed were hematopoietic cells, expressing CD45, and liver sinusoidal-endothelial cells (LSECs), expressing CD14 but lacking CD45 expression. Select antigens were further examined by fluorescence immunomicroscopy of fetal liver sections. Antigen expression was also confirmed on cultured cells by both methods. Gene expression analysis by liver cells, 6 hepatoblastoma cell lines, and hepatoblastoma cells was performed. Immunohistochemistry was used to evaluate CD203c, CD326, and cytokeratin-19 expression on three hepatoblastoma tumors.

Results: Antibody screening identified many cell surface markers commonly or divergently expressed by hematopoietic cells, LSECs, and hepatoblasts. Thirteen novel markers expressed on fetal hepatoblasts were identified including ectonucleotide pyrophosphatase/phosphodiesterase family member 3 (ENPP-3/CD203c), which was found to be expressed by hepatoblasts with widespread expression in the parenchyma of the fetal liver. In culture CD203c⁺CD326⁺⁺ cells resembled hepatocytic cells with coexpression of albumin and cytokeratin-19 confirming a hepatoblast phenotype. CD203c expression declined rapidly in culture whereas the loss of CD326 was not as pronounced. CD203c and CD326 were co-expressed on a subset of hepatoblastoma cell lines and hepatoblastomas with an embryonal pattern.

Conclusions: CD203c is expressed on hepatoblasts and may play a role in purinergic signaling in the developing liver. Hepatoblastoma cell lines were found to consist of two broad phenotypes consisting of a cholangiocyte-like phenotype that expressed CD203c and CD326 and a hepatocyte-like phenotype with diminished expression of these markers. CD203c was expressed by some hepatoblastoma tumors and may represent a marker of a less differentiated embryonal component.

Keywords: CD203c; antigens; endothelial cells; fetal cells; hepatoblastoma; hepatoblasts; hepatology; leukocytes.

Grants and funding

This work was supported, in part, by Vitalant Inc. and the California Institute for Regenerative Medicine, grant number DISC1-08855 (MM). RG, CN and GO were supported by a Bridges to Stem Cell Research and Therapy Award EDUC2-08400 from the California Institute of Regenerative Medicine. CK was supported by the Macy Easom Cancer Research Foundation, The Foundation for Addie’s Research, Owls for Avery, and the family and community of Dawson Willcock. The content is solely the responsibility of the authors and does not necessarily represent the official views of the California Institute for Regenerative Medicine or any other agency of the State of California. This study received funding from Vitalant Inc. The funder was not involved in the study design, collection, analysis, interpretation of data, the writing of this article or the decision to submit it for publication.