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Figure 3


Fig. 3. The esophagi of Sulf1-/-;Sulf2-/- mice have normal skeletal muscle function, but impaired smooth muscle contractility. (A) Postnatal development of the esophageal skeletal muscles in control and Sulf1-/-;Sulf2-/- pups. The cross-sections of Sulf1+/-;Sulf2+/- control and Sulf1-/-;Sulf2-/- mice were immunostained with antibodies against skeletal muscle markers including myosin heavy chain (MHC) and MYF5 or incubated with Cy3-conjugated alpha-bungarotoxin (alpha-BTx) to identify acetylcholine (ACh) receptors on muscle. The completion of the esophageal skeletal muscle formation at P15 was assayed by immunostaining of the abdominal segments with an alkaline phosphatase-conjugated mouse antibody against fast skeletal myosin (sk-Myosin). The antigen-antibody complex was visualized using the substrate BM purple. Arrowheads mark the junction between the esophagus and the stomach. The Sulf1-/-;Sulf2-/- esophagi have completed skeletal muscle formation in the esophagus at P15. Scale bars: 100 µm. (B) Physiological measurements of the esophageal skeletal muscles. The lower-half thoracic segments of the esophagi of the adult Sulf1+/-;Sulf2+/- control and Sulf1-/-;Sulf2-/- mice were subject to twitch and tetanus stimuli. Muscle contractility was measured and compared with those in the presence of selective ion-channel blockers (n=3). The Sulf1-/-;Sulf2-/- esophagi exhibited comparable skeletal muscle contractility in response to the electrical stimuli and ion-channel blocks as the control esophagi. (C) Physiological tests of esophageal smooth muscle contractility. The smooth muscle of the control and the Sulf1-/-;Sulf2-/- mutant esophagi were dissected and their contractile forces in response to various stimuli measured (n=3). The Sulf1-/-;Sulf2-/- esophagi showed diminished smooth muscle contractility in response to carbachol, and partially reduced contractility in response to other chemicals. (D) Quantification of the esophageal smooth muscle contractility induced by various stimuli as shown in C.





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