BaseSpace
Correlation Engine 2.0
Import Your Data
Literature

FAQ

More FAQs

Back to top
Clear Search sequence regions
(e.g. Prostate, Laser capture microdissection, Clofibrate, rs6983267, PRKCA, Ischemia)
Bookmark Forward

Analysis of multiple gene co-expression networks to discover interactions favoring CFTR biogenesis and ΔF508-CFTR rescue.

Matthew D Strub, Long Gao, Kai Tan, Paul B McCray

BMC medical genomics 2021 Oct 30


filter terms:
  • biogenesis (3)
  • cftr protein (1)
  • cftr protein, human (1)
  • CHURC1 (1)
  • cystic fibrosis (3)
  • endocytosis (1)
  • factor (1)
  • gene (9)
  • GZF1 (1)
  • h 40 (1)
  • help (1)
  • humans (1)
  • mrna (1)
  • mrna transcript (1)
  • NEDD8 (6)
  • nedd8 protein, human (1)
  • networks gene (1)
  • protein complex (1)
  • protein human (2)
  • protein levels (1)
  • protein processes (1)
  • protein transport (1)
  • RPL15 (1)
  • sin3 corepressor complex (2)
  • SIN3A (6)
  • SYVN1 (5)
  • ubiquitin protein ligases (2)
  • δf508 cftr (4)
    • Sizes of these terms reflect their relevance to your search.

    We previously reported that expression of a miR-138 mimic or knockdown of SIN3A in primary cultures of cystic fibrosis (CF) airway epithelia increased ΔF508-CFTR mRNA and protein levels, and partially restored CFTR-dependent chloride transport. Global mRNA transcript profiling in ΔF508-CFBE cells treated with miR-138 mimic or SIN3A siRNA identified two genes, SYVN1 and NEDD8, whose inhibition significantly increased ΔF508-CFTR trafficking, maturation, and function. Little is known regarding the dynamic changes in the CFTR gene network during such rescue events. We hypothesized that analysis of condition-specific gene networks from transcriptomic data characterizing ΔF508-CFTR rescue could help identify dynamic gene modules associated with CFTR biogenesis. We applied a computational method, termed M-module, to analyze multiple gene networks, each of which exhibited differential activity compared to a baseline condition. In doing so, we identified both unique and shared gene pathways across multiple differential networks. To construct differential networks, gene expression data from CFBE cells were divided into three groups: (1) siRNA inhibition of NEDD8 and SYVN1; (2) miR-138 mimic and SIN3A siRNA; and (3) temperature (27 °C for 24 h, 40 °C for 24 h, and 27 °C for 24 h followed by 40 °C for 24 h). Interrogation of individual networks (e.g., NEDD8/SYVN1 network), combinations of two networks (e.g., NEDD8/SYVN1 + temperature networks), and all three networks yielded sets of 1-modules, 2-modules, and 3-modules, respectively. Gene ontology analysis revealed significant enrichment of dynamic modules in pathways including translation, protein metabolic/catabolic processes, protein complex assembly, and endocytosis. Candidate CFTR effectors identified in the analysis included CHURC1, GZF1, and RPL15, and siRNA-mediated knockdown of these genes partially restored CFTR-dependent transepithelial chloride current to ΔF508-CFBE cells. The ability of the M-module to identify dynamic modules involved in ΔF508 rescue provides a novel approach for studying CFTR biogenesis and identifying candidate suppressors of ΔF508. © 2021. The Author(s).

    Citation

    Matthew D Strub, Long Gao, Kai Tan, Paul B McCray. Analysis of multiple gene co-expression networks to discover interactions favoring CFTR biogenesis and ΔF508-CFTR rescue. BMC medical genomics. 2021 Oct 30;14(1):258

    Expand section icon Mesh Tags

    Expand section icon Substances


    PMID: 34717611

    View Full Text
    • Copyright © 2024 Illumina Inc. All rights reserved.