Figure 1.
Immunofluorescence of mucins in CM and CVM.
CM (A) and CVM (B) were frozen, cryosetioned, and fixed for immunofluorescent staining. All sections were stained for WGA (blue), mucin5AC (green), and mucin5B (red). Upper panels are images acquired with a 20X (A) or 10X (B) lens. Lower panels were acquired with a 100X lens.
Figure 2.
(A) CM was stained for IgA (green) and IgG (red). Left column shows Ig expression with WGA (blue). White pixels highlight regions of A-hi/G-lo (middle column) and G-hi/A-lo (right column) staining. (B) Graph of total area of highlighted pixels for IgG and IgA dense regions.
Figure 3.
Immunofluorescence of IgG and IgA in CVM.
Frozen CVM was stained for IgG (red) and IgA (green) and imaged with a 100X lens. (A) CVM also stained with WGA (blue). (B) Same field of view in (A) with nuclei now shown in blue. (C) Zoom in of white boxes in (B) to show separated IgA (top) and IgG (bottom) stains.
Table 1.
Quantification of IgG and IgA dense regions in CM images.
Figure 4.
Detection of immunogloblulins in endocervical explants.
Sectioned explants of endocervix were stained with antibodies to detect IgA (green) and IgG (red). Cytokeratin 7 (blue) was also stained to identify the layer of columnar cells. Each row represents a different donor sample. Images were acquired with a 100X lens as a panel and then stitched together. Second and third columns have red or green color removed, respectively, from image in first column.
Figure 5.
(A) 100X image of fluorescently labeled IgG in CM. (B) Zoomed in ROI from (A) at select timepoints. Images were acquired every 0.50ms over the course of 1 minutes, with a rebleach after 30 seconds. Fluorescence intensities (FI) after normalization are shown. (C) Graph of normalized intensities of photobleached ROIs in IgG or IgA labeled CM. (D) Graph of normalized intensities of photobleached ROIs in IgG labeled CVM. CM average from (C) is included for comparison. (E) Average values from other graphs redisplayed.
Figure 6.
CM (A) and CVM (B) were dialyzed through a 700 kDa filter (Post) and loaded onto gels for western blotting with pre-dialyzed mucus (Pre). Blots were stained for IgA or IgG. Various proteins known to be components of mucus were identified pre-and post- dialysis, the intensities of bands quantified as described, and the percent reduction graphed. P-value <0.01 indicated by a *, <0.005 by a **, and <0.001 by a ***. Abbreviations: HSA: human serum albumin, SC: secretory component, LFN: lactoferrin, SLPI: secretory leukocyte protease inhibitor.