Method Article

Establishment and Evaluation of an In Vitro Human-Based Advanced Model of Pulmonary Fibrosis

DOI:

10.3791/67845

July 22nd, 2025

In This Article

Summary

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An imaging method was developed to evaluate the activation of fibroblasts in human precision-cut lung slices based on fibroblast activation protein (FAP). This methodology establishes a robust and reproducible platform for staging fibrotic progression, advancing translational in vitro models for therapeutic development while maintaining the fidelity of the human tissue microenvironment.

Abstract

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Pulmonary fibrosis is characterized by irreversible destruction of alveolar structure and excessive deposition of extracellular matrix. Although animal models have been widely used in pulmonary fibrosis research, none of the currently available models fully recapitulate the progressive nature of IPF or its defining histological feature, such as fibroblastic foci. Advanced in vitro models, including precision-cut lung slices (PCLS), are often considered the most physiologically relevant pulmonary test system and have been successfully employed for drug screening. Nevertheless, the inability to differentiate the degree of fibrosis in the IPF lung has resulted in blinding and uncertainty in the PCLS obtained. Previous research demonstrated that fibroblast activation protein (FAP) could evaluate the pro-fibrotic activity of ILD, potentially contributing to early diagnosis and the selection of appropriate therapeutic windows. In this study, 600 µm PCLS will be obtained from healthy donors and IPF patients using a shock slicer and evaluated using molecular probes targeting FAP to determine the degree of fibroblast activity based on fluorescent signal intensity. This approach provides an advanced in vitro model and evaluation technique for pulmonary fibrosis research, enhancing the ability to study disease mechanisms and assess therapeutic interventions.

Introduction

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Pulmonary fibrosis (PF) is a common form with an unknown etiology and a particularly poor prognosis, with a median five-year survival rate of only 25%1. The intratracheal bleomycin administration model is currently the most widely used animal model for preclinical studies2. However, fibrosis induced by bleomycin is transient and resolves over time, which contrasts sharply with the irreversible nature of IPF3. Moreover, the intratracheal bleomycin model presents significant challenges due to the heterogeneous severity of fibrosis resulting from endotracheal administration, whether surgical or nonsu....

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Protocol

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The study was approved by the Ethics Committee of the First Hospital of Guangzhou Medical University (2021G-29). IPF was diagnosed based on physical examination and chest high-resolution computed tomography findings, following the diagnostic criteria established by ATS/ERS/JRS/ALAT (2022). All IPF patient specimens were obtained from lung transplantation or lung biopsy. Healthy lung tissue samples were obtained from organ donors diagnosed with brain death10. Written consent for tissue collection was obtained from each patient or the patient's family prior to collection. For details regarding all materials, solutions, and instruments used in this protocol, refer to....

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Results

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The preparation procedure for PCLS of human lung tissue is depicted in Figure 1. Human lung tissue was embedded in agarose and subsequently trimmed into tissue blocks approximately 1 cm3 in size using a razor blade. Trimmed and flattened tissues were affixed to a platform for sectioning at 600 µm thickness using a microtome (Figure 1A,B). PCLS were incubated in 12-well plates (Figure 1C).

Prepa.......

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Discussion

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Through the above research methods, PCLS from healthy donors and IPF patients were prepared. Simultaneously, mammalian cells were used to express single-chain variable fragments of FAP, and their purity and specificity were verified. A molecular probe targeting FAP and labeled with ICG was employed to detect FAP expression levels, reflecting the degree of fibroblast activation. This approach provides an advanced evaluation method for pulmonary fibrosis treatment.

PCLS preserves the natural cel.......

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Disclosures

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The authors have no conflicts of interest to disclose.

Acknowledgements

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We are grateful that this work was supported by grants from the National Natural Science Foundation of China (82470061), the Young Scientists Program of Guangzhou Laboratory (QNPG23-15), and the Independent Project of the State Key Laboratory of Respiratory Diseases (SKLRD-Z-202305).

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Materials

List of materials used in this article
NameCompanyCatalog NumberComments
0.25 % trypsin-EDTAGibco15050-057
2× Color SYBR Green qPCR Master Mix (ROX2)EZBioscienceA0012-R2
20 ml syringeWinnerV532159
293T cellBeyotimeC6008
502 glueZhuolideD-40
Agarose, low gelling temperatureSigma AldrichA9414-25G
Anti-Collagen I antibodyabcamab138492
Anti-Fibronectin antibodyabcamab2413
Anti-His-tag mAb-Alexa Fluor 488MBLD291-A48
BL21BeyotimeD1009S
BladeGillette7in83a7Q
Color Reverse Transcription Kit (with gDNA Remover)EZBioscienceA0010CGQ
Coomassie Blue Super Fast Staining SolutionBeyotimeP0017F
DMEMGibco12800017
Erlenmeyer flaskSichuan ShunboGG-17
FAP Rabbit mAbCST66562
FBSGibco10099-141
ForcepsRobozRS-5135
ICG-NHSRuixibioR-TE-157
IPTGMCE367-93-1
microbalanceSecuraSecura225D-1CN
microwaveMideoPM2002
Multi-Mode In Vivo Animal Imaging SystemBioLightAniView600
Ni-NTAGenscriptL00250
NovoCyte flow cytometerACEA BiosciencesNovocyte
PBSGibco10010023
Penicillin-StreptomycinGibco15140122
SDS-PAGEBeyotimeP00528
Universal RNA PurificationEZBioscienceEZB-RN4
VibratomeDOSAKADTK-1000N
β-actin Rabbit pAbYeasen30102ES
Primer
β-actin primer-FiGenebook BiotechCATGTACGTTGCTATCCAGGC
β-actin primer-RiGenebook BiotechCTCCTTAATGTCACGCACGAT
FAP primer-FiGenebook BiotechTTGAGTGGATGGGAGGGAT
FAP primer-RiGenebook BiotechGCTGTGCTCGTGGATTTGT
Collagen-I primer-FiGenebook BiotechGAGGGCCAAGACGAAGACATC
Collagen-I primer-RiGenebook BiotechCAGATCACGTCATCGCACAAC
Fibronectin primer-FiGenebook BiotechCGGTGGCTGTCAGTCAAAG
Fibronectin primer-RiGenebook BiotechAAACCTCGGCTTCCTCCATAA

References

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  1. Raghu, G., et al. An official ATS/ERS/JRS/ALAT statement: Idiopathic pulmonary fibrosis: Evidence-based guidelines for diagnosis and management. Am J Respir Crit Care Med. 183 (6), 788-824 (2011).
  2. Jenkins, R. G., et al.

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Tags

Pulmonary FibrosisIn Vitro ModelPrecision Cut Lung SlicesFibroblast Activation ProteinExtracellular MatrixFibroblastic FociDrug ScreeningMolecular ProbesFluorescent SignalFibroblast Activity
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