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SP-B Detection and Gene Expression in Chronic Rhinosinusitis

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Title: SP-B Detection and Gene Expression in Chronic Rhinosinusitis


1
SP-B Detection and Gene Expression in Chronic
Rhinosinusitis
  • Bradford A. Woodworth, MD
  • Noam A. Cohen, MD, PhD
  • Rachel Wood, BS
  • Geeta Bhargave, BS
  • John E. Baatz, PhD
  • Rodney J. Schlosser, MD
  • Department of Otorhinolaryngology HNS
  • University of Pennsylvania Health System
  • Medical University of South Carolina

2
Grant support
  • Cystic Fibrosis Foundation

3
Surfactant
  • Secreted in lungs by type II pneumocytes and
    Clara cells
  • Phospholipids (lamellar bodies) 80-90
  • Used for premature infants
  • Decrease surface tension
  • Decrease viscosity of mucus
  • Proteins 10-15
  • SP B and C hydrophobic, PL processing
    trafficking, anti-microbial properties
  • SP A and D hydrophilic, immune functions

4
Surfactant in Airway Mucus
  • Coats surface of gel layer to reduce surface
    tension
  • Decreases the viscosity of mucus
  • Increases mucociliary clearance
  • SP-B facilitates properties of surfactant and is
    also shown to have direct anti-microbial
    properties

5
SP-B
  • Extremely hydrophobic protein with multiple
    post-translational modifications
  • SP-A and D found at mucosal and epithelial
    surfaces throughout the body
  • SP-B originally thought to be limited to the
    lungs
  • Recent studies show expression in the Eustachian
    tube mucosa

6
SP-B in Pulmonary Surfactant
SP-B
LB
Tubular Myelin
What role does surfactant play in the sinuses?
7
Prior Studies
  • Phospholipid lamellar bodies in sinonasal
    epithelium

8
Prior Studies
  • Hydrophilic surfactant proteins A and D in sinus
    mucosa
  • Localize to epithelium and submucosal glandular
    elements
  • Upregulated in cystic fibrosis CRS mucosa

Is there a role for SP-B?
9
Hypothesis
  • SP-B is present in sinonasal mucosa and
    expression is altered in several types of CRS
    when compared to healthy controls.

10
Methods
  • Sinus mucosal biopsies
  • Allergic Fungal Rhinosinusitis (n7)
  • Cystic Fibrosis (n 4)
  • Non-atopic CRS with nasal polyps (n5)
  • Healthy controls (n5)
  • Quantitative RT-PCR, immunoblot,
    immunohistochemistry

11
Methods Cycle threshold (Ct)
12
Methods Cycle threshold (Ct)
  • Delta Ct (?Ct) - Ct for mRNA subtracted from Ct
    of internal control (18s rRNA).
  • Eliminates effect of differences in sample
    concentration on Ct.
  • Individual ?Ct values of each subtype of CRS are
    compared to the healthy control tissue

13
SP-B Quantitative RT-PCR

p 0.004
167-fold elevation in CF patients compared to
healthy controls
14
Detection of SP-B Proprotein
42 kDa
Detection of the proprotein and intermediate
forms confirms translated product
  • Where is the protein produced and secreted?

15
Immunofluorescence
Sinus Epithelium
Submucosal Glands
SP-B expression green, Nuclear stain in blue
SP-B localizes to the epithelium and submucosal
glands
16
Discussion
  • SP-B was significantly upregulated in CF CRS
    mucosa
  • Pseudomonas produces proteases known to degrade
    SPs (Malloy et al).
  • SP-B upregulated in response to degradation of
    SP-B and surfactant by Pseudomonas.
  • Alternatively, increased submucosal glands in CF
    mucosa contribute more mRNA transcripts to sample

17
Conclusion
  • SP-B is upregulated in cystic fibrosis CRS and is
    produced by the epithelium and submucosal glands
    of the sinonasal cavities.
  • Further studies indicated to investigate the role
    that SP-B and surfactant have in CRS.

18
Future directions
  • Anti-microbial properties of SP-B as a potential
    therapy for infectious CRS
  • In vivo and in vitro models
  • Further delineation of protein expression and
    specific localization with immunoelectron
    microscopy

19
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