Super-Resolution Microscopy Reveals a Nanoscale Organization of Acetylcholine Receptors for Trans-Synaptic Alignment at Neuromuscular Synapses

AChRs are distributed in stripes that are not correlated with the crest of NMJ junctional folds. A, A representative 3D-SIM image showing the AChR-rich stripes separated by dark bands. Scale bar, 5 µm. The areas enclosed by yellow rectangles (A’, A”) are shown in a high magnification on the right. Scale bar, 1 µm. B, A small region of the AChR stripes (left panel) are used to generate the intensity profile shown on the right. The width of the AChR stripes (W) and the distance between two adjacent stripes (D) are measured and presented in the bar graph in D. C, A representative transmission electron micrograph of an NMJ from the TVA muscle. The junctional folds are clearly visible at the postsynaptic compartment (highlighted by red color). Numerous synaptic vesicles and mitochondria are present within the opposing presynaptic terminal. The average width of junctional fold openings and fold crests (yellow brackets) were manually quantified and presented in the bar graph in D. Scale bar, 0.2 µm. D, The bar graph summarizing the measurement results from the SIM data (blue bars, n = 4, >180 stripes) and EM data (red bars; n = 7, >40 folds). Error bars represent the SD.

Correlation of AChR distribution with specific pre- and postsynaptic markers at NMJs. A, B, Colocalization of AChRs (white) with various synaptic markers (magenta, threshold). Representative fluorescent images are shown on the right and the schematics on the right depict the known localization of each synaptic marker (magenta line) with respect to the junctional folds. Scale bars, 5 µm. The representative intensity profiles of AChRs (gray) and each of the synaptic markers (magenta) are shown in B. Four markers were examined: Rapsyn, an intracellular AChR scaffolding protein; piccolo, an active zone component; integrin α7, an integrin subunit involved in adhesion in NMJs. C, Quantification of the colocalization of each marker with AChRs. One-way ANOVA analysis: p = 2.22 × 10⁻⁵ (n = 4). Error bars represent the SD. Bonferroni analysis: *p = 0.012, ***p < 0.004.

Super-resolution imaging reveals AChRs are concentrated around the opening of junctional folds. A, 3D-STORM imaging of AChRs highlights the 3D nature of the postsynaptic membrane. The widths of AChR stripes (∼130 nm) and the distance between stripes (∼210 nm) is consistent with quantifications from our previous SIM data. A small region outlined by dashed rectangle (A’) is shown in a higher magnification on the right. Color scale bar indicates Z-depth. Scale bars, 2 µm. B, Representative STORM images of AChRs at a NMJ. Scale bar, 5 µm. Inset image shows the same NMJ imaged using widefield microscopy. Close-up regions (B’, B”) reveals a thin slit at the center of each AChR stripe (arrow). Scale bar, 1 µm. Bottom, close-up view of individual AChR stripes. C, Representative profile linescan further highlighting the slit at the center of each AChR stripe. D, Quantification of the width of the AChR stripe gap (measured from STORM data, n = 23) and the width of the junctional fold opening (measured from our TEM data, n = 50). Error bars represent the SD. Average width values at center of each bar.