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miRNA Profiling in Human Precision-cut Lung Slices (PCLS))
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Abstract
ObjectiveHuman precision cut lung slices (PCLS) are widely used as an ex vivo model system for drug discovery and development of new therapies. PCLS reflect the functional heterogeneity of lung tissue and possess relevant lung cell types. We thus determined the use of PCLS in studying non-coding RNAs notably miRNAs, which are important gene regulatory molecules. Since miRNAs play key role as mediators of respiratory diseases, they can serve as valuable prognostic or diagnostic biomarkers, and in therapeutic interventions, of lung diseases. A technical limitation though is the vast amount of agarose in PCLS which impedes (mi)RNA extraction by standard procedures. Here we modified our recently published protocol for RNA 29 isolation from PCLS to enable miRNA readouts. Results The modified method relies on the separation of lysis and precipitation steps, and a clean-up procedure with specific magnetic beads. We obtained successfully quality miRNA amenable for downstream applications such as RTqPCR and whole transcriptome miRNA analysis. Comparison of miRNA profiles in PCLS with published data from human lung, identified all important miRNAs regulated in IPF, COPD, asthma or lung cancer. Therefore, this shows suitability of the method for analyzing miRNA targets and biomarkers in the valuable human 38 PCLS model.
Springer Science and Business Media LLC
Title: miRNA Profiling in Human Precision-cut Lung Slices (PCLS))
Description:
Abstract
ObjectiveHuman precision cut lung slices (PCLS) are widely used as an ex vivo model system for drug discovery and development of new therapies.
PCLS reflect the functional heterogeneity of lung tissue and possess relevant lung cell types.
We thus determined the use of PCLS in studying non-coding RNAs notably miRNAs, which are important gene regulatory molecules.
Since miRNAs play key role as mediators of respiratory diseases, they can serve as valuable prognostic or diagnostic biomarkers, and in therapeutic interventions, of lung diseases.
A technical limitation though is the vast amount of agarose in PCLS which impedes (mi)RNA extraction by standard procedures.
Here we modified our recently published protocol for RNA 29 isolation from PCLS to enable miRNA readouts.
Results The modified method relies on the separation of lysis and precipitation steps, and a clean-up procedure with specific magnetic beads.
We obtained successfully quality miRNA amenable for downstream applications such as RTqPCR and whole transcriptome miRNA analysis.
Comparison of miRNA profiles in PCLS with published data from human lung, identified all important miRNAs regulated in IPF, COPD, asthma or lung cancer.
Therefore, this shows suitability of the method for analyzing miRNA targets and biomarkers in the valuable human 38 PCLS model.
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