Figure 1
Figure 1. Characterization of collagen nano-mechanical properties. (A) Coomassie staining of type I collagen and N-acetylated collagen. A total of 2 μg of proteins was loaded on 6% gel of polyacrylamide; > 85% of lysine residue were modified in the native protein determining a different migration in electrophoresis. (B) In vitro analysis of collagens structure. (i) Atomic force microscopy images of 3 μm2 of dehydrated collagen coating. (ii) Second harmonic generation images of collagen supramolecular structure were acquired through a 63× (1.2 NA) objective on a Leica DMIRE2 microscope with a TCS SP2 scanner. Analysis was performed with the Leica confocal software and ImageJ (NIH). Scale bar represents 10 μm. (C) Atomic force microscopy images of collagens in fluid (PBS). A total of 5 μm2 fields were analyzed in contact mode using an MFP-3D Bio-atomic force microscope (Asylum Research). (D) Roles of α2-integrin and GPVI on MK adhesion and spreading on type I collagen. Cord blood-derived MKs were seeded for 2 hours on type I collagen in the presence of 20 μg/mL of anti-α2 (clone P1E6) and Fab GPVI (clone 9012.2) antibodies, fixed, and then stained for actin (red) and CD41 (green). Images were acquired through an Olympus BX51 using a 20×/0.5 UPlan objective. Scale bar represents 50 μm. (E) Effect of chemical modification of type I collagen on α2 integrin and GPVI engagement. MKs were seeded on type I collagen and N-acetylated type I collagen for 1 hour, and cell adhesion was evaluated in the presence of increasing concentrations of anti-α2 and GPVI antibodies. Cell adhesion values are expressed relative to control (absence of inhibitor).

Characterization of collagen nano-mechanical properties. (A) Coomassie staining of type I collagen and N-acetylated collagen. A total of 2 μg of proteins was loaded on 6% gel of polyacrylamide; > 85% of lysine residue were modified in the native protein determining a different migration in electrophoresis. (B) In vitro analysis of collagens structure. (i) Atomic force microscopy images of 3 μm2 of dehydrated collagen coating. (ii) Second harmonic generation images of collagen supramolecular structure were acquired through a 63× (1.2 NA) objective on a Leica DMIRE2 microscope with a TCS SP2 scanner. Analysis was performed with the Leica confocal software and ImageJ (NIH). Scale bar represents 10 μm. (C) Atomic force microscopy images of collagens in fluid (PBS). A total of 5 μm2 fields were analyzed in contact mode using an MFP-3D Bio-atomic force microscope (Asylum Research). (D) Roles of α2-integrin and GPVI on MK adhesion and spreading on type I collagen. Cord blood-derived MKs were seeded for 2 hours on type I collagen in the presence of 20 μg/mL of anti-α2 (clone P1E6) and Fab GPVI (clone 9012.2) antibodies, fixed, and then stained for actin (red) and CD41 (green). Images were acquired through an Olympus BX51 using a 20×/0.5 UPlan objective. Scale bar represents 50 μm. (E) Effect of chemical modification of type I collagen on α2 integrin and GPVI engagement. MKs were seeded on type I collagen and N-acetylated type I collagen for 1 hour, and cell adhesion was evaluated in the presence of increasing concentrations of anti-α2 and GPVI antibodies. Cell adhesion values are expressed relative to control (absence of inhibitor).

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal