The Rapid Development of Airway Organoids: A Direct Culture Strategy

Syahidatulamali Che Shaffi, Norashikin Zakaria, Nur Shuhaidatul Sarmiza Abdul Halim, Anan A. Ishtiah, Azim Ab Patar, Badrul Hisham Yahaya

Research output: Chapter in Book or Conference Publication/ProceedingChapterpeer-review

1 Citation (Scopus)

Abstract

Introduction: The lung is a complex organ composed of numerous cell types. Exposure to air pollutants, cigarette smoke, bacteria, viruses, and many others may cause injury to the epithelial cells that line the conducting airways and alveoli. Organoids are the 3D self-organising structures grown from stem cells and generated from adult stem and progenitor cells. Lung organoids are fascinating tools to investigate human lung development in vitro. The objective of this study was to establish a rapid method for generating lung organoids with a direct culture strategy. Methods: Trachea and lung organoids were derived from mixed cell populations of mice primary airway epithelial cells, fibroblasts, and lung microvascular endothelial cells and directly digested from the whole cell population in the distal lung. Results: The formation of spheres appeared as early as 3 days and continued to proliferate until day 5. The generation of trachea and lung organoids self-organised into discrete epithelial structures was formed within less than 10 days. Conclusion: We conclude that researchers will be able to examine cellular involvement during organ formation and molecular networks because organoids come in a variety of morphologies and stages of development, and this organoid protocol may be used for modelling lung diseases as a platform for therapeutic purposes and suitable for personalised medicine for respiratory diseases.

Original languageEnglish
Title of host publicationAdvances in Experimental Medicine and Biology
PublisherSpringer
Pages165-179
Number of pages15
DOIs
Publication statusPublished - 2023
Externally publishedYes

Publication series

NameAdvances in Experimental Medicine and Biology
VolumePart F1638
ISSN (Print)0065-2598
ISSN (Electronic)2214-8019

Keywords

  • 3D culture
  • Direct culture
  • Lung organoid
  • Trachea organoid

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