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RNA Sequencing Analysis of Monocytes Exposed to Airway Fluid From Children With Pediatric Acute Respiratory Distress Syndrome.

Authors :
Grunwell JR
Huang M
Stephenson ST
Tidwell M
Ripple MJ
Fitzpatrick AM
Kamaleswaran R
Source :
Critical care explorations [Crit Care Explor] 2024 Oct 04; Vol. 6 (10), pp. e1125. Date of Electronic Publication: 2024 Oct 04 (Print Publication: 2024).
Publication Year :
2024

Abstract

Objectives: Monocytes are plastic cells that assume different polarization states that can either promote inflammation or tissue repair and inflammation resolution. Polarized monocytes are partially defined by their transcriptional profiles that are influenced by environmental stimuli. The airway monocyte response in pediatric acute respiratory distress syndrome (PARDS) is undefined. To identify differentially expressed genes and networks using a novel transcriptomic reporter assay with donor monocytes exposed to the airway fluid of intubated children with and at-risk for PARDS. To determine differences in gene expression at two time points using the donor monocyte assay exposed to airway fluid from intubated children with PARDS obtained 48-96 hours following initial tracheal aspirate sampling.<br />Design: In vitro pilot study carried out using airway fluid supernatant.<br />Setting: Academic 40-bed PICU.<br />Participants: Fifty-seven children: 44 children with PARDS and 13 children at-risk for PARDS.<br />Interventions: None.<br />Measurements and Main Results: We performed bulk RNA sequencing using a transcriptomic reporter assay of monocytes exposed to airway fluid from intubated children to discover gene networks differentiating PARDS from at-risk for PARDS and those differentiating mild/moderate from severe PARDS. We also report differences in gene expression in children with PARDS 48-96 hours following initial tracheal aspirate sampling. We found that interleukin (IL)-10, IL-4, and IL-13, cytokine/chemokine signaling, and the senescence-associated secretory phenotype are upregulated in monocytes exposed to airway fluid from intubated children with PARDS compared with those at-risk for PARDS. Signaling by NOTCH, histone deacetylation/acetylation, DNA methylation, chromatin modifications (B-WICH complex), and RNA polymerase I transcription and its associated regulatory apparatus were upregulated in children with PARDS 48-96 hours following initial tracheal aspirate sampling.<br />Conclusions: We identified gene networks important to the PARDS airway immune response using bulk RNA sequencing from a monocyte reporter assay that exposed monocytes to airway fluid from intubated children with and at-risk for PARDS. Mechanistic investigations are needed to validate our findings.<br />Competing Interests: The authors have disclosed that they do not have any potential conflicts of interest.<br /> (Copyright © 2024 The Authors. Published by Wolters Kluwer Health, Inc. on behalf of the Society of Critical Care Medicine.)

Details

Language :
English
ISSN :
2639-8028
Volume :
6
Issue :
10
Database :
MEDLINE
Journal :
Critical care explorations
Publication Type :
Academic Journal
Accession number :
39365167
Full Text :
https://doi.org/10.1097/CCE.0000000000001125