Experimentally, lung inflammation in laboratory animals is usually detected by the presence of inflammatory markers, such as immune cells and cytokines, in the bronchoalveolar lavage fluid (BALF) of sacrificed animals. This method, although extensively used, is time, money and animal life consuming, especially when applied to genetically modified animals. Thus a new and more convenient approach, based on in vivo imaging analysis, has been set up to evaluate the inflammatory response in the lung of CFTR-deficient (CF) mice, a murine model of cystic fibrosis

A Bianchi

AC Thomas

AK Claes

Angela Sandri

AR Hauser

B Schmeck

Barouk M. Assael

Claudio Sorio

D Ansaldi

F Stellari

Fabio Stellari

Federico Boschi

FF Stellari

Francesca Ravanetti

Francesca Ruscitti

FX Blé

G Matute-Bello

Gabriella Bergamini

Gaetano Donofrio

Gino Villetti

GM Dam van

HA Enright

HF Håkansson

LM Crane

M Cohen-Cymberknoh

M Galluzzo

M Lederlin

M Mauffray

M Paroni

M Simone De

Maria M. Lleo

MR Starkey

Paola Melotti

V Balloy

X Ma

Y Belessis

Journal of Translational Medicine

PubMed

Crossref

In vivo monitoring of lung inflammation in CFTR-deficient mice

Springer - Publisher Connector

Stellari, Fabio

BERGAMINI, Gabriella

Ruscitti, Francesca

Sandri, Angela

Ravanetti, Francesca

Donofrio, Gaetano

BOSCHI, Federico

Villetti, Gino

SORIO, Claudio

Assael, Barouk M

MELOTTI, Paola Maria

LLEO' FERNANDEZ, Maria Del Mar

Catalogo dei prodotti della ricerca

English

Background: Experimentally, lung inflammation in laboratory animals is usually detected by the presence of inflammatory markers, such as immune cells and cytokines, in the bronchoalveolar lavage fluid (BALF) of sacrificed animals. This method, although extensively used, is time, money and animal life consuming, especially when applied to genetically modified animals. Thus a new and more convenient approach, based on in vivo imaging analysis, has been set up to evaluate the inflammatory response in the lung of CFTR-deficient (CF) mice, a murine model of cystic fibrosis. Methods: Wild type (WT) and CF mice were stimulated with P. aeruginosa LPS, TNF-alpha and culture supernatant derived from P. aeruginosa (strain VR1). Lung inflammation was detected by measuring bioluminescence in vivo in mice transiently transgenized with a luciferase reporter gene under the control of a bovine IL-8 gene promoter. Results: Differences in bioluminescence (BLI) signal were revealed by comparing the two types of mice after intratracheal challenge with pro-inflammatory stimuli. BLI increased at 4 h after stimulation with TNF-alpha and at 24 h after administration of LPS and VR1 supernatant in CF mice with respect to untreated animals. The BLI signal was significantly more intense and lasted for longer times in CF animals when compared to WT mice. Analysis of BALF markers: leukocytes, cytokines and histology revealed no significant differences between CF and WT mice. Conclusions: In vivo gene delivery technology and non-invasive bioluminescent imaging has been successfully adapted to CFTR-deficient mice. Activation of bIL-8 transgene promoter can be monitored by non-invasive BLI imaging in the lung of the same animal and compared longitudinally in both CF or WT mice, after challenge with pro-inflammatory stimuli. The combination of these technologies and the use of CF mice offer the unique opportunity of evaluating the impact of therapies aimed to control inflammation in a CF background

In vivo monitoring of lung inflammation in CFTR-deficient mice

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Springer - Publisher Connector

Catalogo dei prodotti della ricerca

Archivio istituzionale della Ricerca - Università degli Studi di Parma