Figure 4.
Figure 4. Multigranular compartments result from the homotypic fusion of α granules. (A-B) Ultrastructural TEM analysis of multigranular compartments in platelets stimulated with 1 U/mL thrombin for 10 seconds. Two representative TEM images illustrate the presence of nucleoids (arrows) in the aggregates. (C-D) IEM characterization of the multigranular compartments. Electron micrographs of ultrathin cryosections of platelets stimulated with 0.1 U/mL thrombin. Antibodies were detected with protein A coupled to 10-nm gold particles. (C) Multigranular compartments (*) were identified as fused α granules by immunolabeling with an antifibrinogen antibody. Labeling with antiserotonin was absent from these structures (*), whereas δ granules (δ) were positive. (E-F) Representative TEM images showing that the limiting membrane of the multigranular compartments (*) is not electron-dense (white arrowheads) whereas the plasma membrane is positive for tannic acid (black arrowheads). Note the presence of a δ granule close to the multigranular compartment in (E) without any fusing profile. (G-H) FIB-SEM analysis of the unstained multigranular compartments in platelets stimulated with 1 U/mL thrombin for 10 seconds. An example of the FIB-SEM raw observations and the corresponding 3D reconstruction of stained granules (in red) and an unstained multigranular compartment (in yellow) are shown. Scale bars, 500 nm.

Multigranular compartments result from the homotypic fusion of α granules. (A-B) Ultrastructural TEM analysis of multigranular compartments in platelets stimulated with 1 U/mL thrombin for 10 seconds. Two representative TEM images illustrate the presence of nucleoids (arrows) in the aggregates. (C-D) IEM characterization of the multigranular compartments. Electron micrographs of ultrathin cryosections of platelets stimulated with 0.1 U/mL thrombin. Antibodies were detected with protein A coupled to 10-nm gold particles. (C) Multigranular compartments (*) were identified as fused α granules by immunolabeling with an antifibrinogen antibody. Labeling with antiserotonin was absent from these structures (*), whereas δ granules (δ) were positive. (E-F) Representative TEM images showing that the limiting membrane of the multigranular compartments (*) is not electron-dense (white arrowheads) whereas the plasma membrane is positive for tannic acid (black arrowheads). Note the presence of a δ granule close to the multigranular compartment in (E) without any fusing profile. (G-H) FIB-SEM analysis of the unstained multigranular compartments in platelets stimulated with 1 U/mL thrombin for 10 seconds. An example of the FIB-SEM raw observations and the corresponding 3D reconstruction of stained granules (in red) and an unstained multigranular compartment (in yellow) are shown. Scale bars, 500 nm.

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