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The substratum. To conclude, functions for caveolae have been identified in biomechanical remodeling or mechanosensing [3,4,28]. Indeed, Cav1 and caveolae are abundant in cells experiencing high mechanical stress such as muscle, skin and endothelial cells. The fact that Cav1 and caveolae levels at the cell surface are regulated by cell adhesion provide a rational for the regulation of caveolae assembly by mechanical clues.(Rutgers University, NJ). Monoclonal against human vinculin was a kind gift of Dr Marina Glukhova (Institut get Itacitinib Curie-Paris). HRPconjugated anti-mouse IgG, Cy3-conjugated anti-mouse and Cy5conjugated F(ab)2 anti-mouse antibodies were purchased from Jackson ImmunoResearch Laboratories. Alexa-Fluor-labeled antimouse IgG antibodies were purchased from Molecular Probes (Invitrogen).Caveolin1 trafficking assay and quantificationHela cells transfected with the indicated constructs were detached, held in suspension in culture medium supplemented with 20 mM Hepes at 37uC for 1 h and replated on fibronectin (10 mg/ml) coated glass dish. After the indicated time of replating, the cells were fixed for immunfluorescence analysis or observed in live using spinning disk or TIRF-M. For quantification of co-localization between a5-integrin-GFP and Cav1-mRFP at the cell periphery, the area of cell surface was drawn with the Threshold command of MetaMorph 7. A 20-pixel width region from the cell periphery was created using both the Erode and Create Region commands of MetaMorph 7. The percentage of co-localization of the two proteins was measured using the Measure Colocalization command of MetaMorph 7 in the 20-pixel region. Statistical analyses were performed using Student’s t test in GraphPad Prism 5 software.Live cell imaging by TIRF and spinning disk confocal AZ876 web microscopyFor live cell imaging by TIRF-M, HeLa cells seeded onto glassbottom dish were transfected with the indicated constructs and imaged the next day with a 1006 1.49 NA TIRF objective on a Nikon TE2000 (Nikon France SAS, Champigny sur Marne, France) inverted microscope equipped with a QuantEM EMCCD camera (Roper Scientific SAS, Evry, France/Photometrics, AZ, USA), a dual output laser launch which included 491 and 561 nm 50 mW DPSS lasers (Roper Scientific), and driven by Metamorph 24195657 7 software (MDS Analytical Technologies). A DV2 beam-splitter system (Roper Scientific/Photometrics) mounted on the light path enabled the simultaneous acquisition of the two emission channels. A motorized device driven by Metamorph allowed accurate positioning of the illumination light for evanescent wave excitation. For spinning disk microscopy, HeLa cells plated onto a glassbottom dish coated with fibronectin (Sigma, 10 mg/ml) and transfected with the indicated constructs. Images were acquired with 100 ms exposure time at 2 or 5 s interval as indicated using a spinning disk microscope based on a CSU22 Yokogawa head mounted on the lateral port of an inverted microscope Leica IRE2 equipped with a 1006 1.4NA Plan-Apo objective and a dual output laser launch which included 491 and 561 nm ERROL laser bench 491 nm, 561 nm (Roper Scientific). Images were acquired with a Camera EMCCD Cascade 5126512 (Photometrics). The system was steered by Metamorph 7 software.Materials and Methods Cell Culture, transfection and siRNA treatmentHela cells were cultured in DMEM medium (GIBCO) containing 15 FCS and 2 mM glutamine at 37uC and 5 CO2. For treatment with cytoskeleton-disassembling drugs, cells were treated fo.The substratum. To conclude, functions for caveolae have been identified in biomechanical remodeling or mechanosensing [3,4,28]. Indeed, Cav1 and caveolae are abundant in cells experiencing high mechanical stress such as muscle, skin and endothelial cells. The fact that Cav1 and caveolae levels at the cell surface are regulated by cell adhesion provide a rational for the regulation of caveolae assembly by mechanical clues.(Rutgers University, NJ). Monoclonal against human vinculin was a kind gift of Dr Marina Glukhova (Institut Curie-Paris). HRPconjugated anti-mouse IgG, Cy3-conjugated anti-mouse and Cy5conjugated F(ab)2 anti-mouse antibodies were purchased from Jackson ImmunoResearch Laboratories. Alexa-Fluor-labeled antimouse IgG antibodies were purchased from Molecular Probes (Invitrogen).Caveolin1 trafficking assay and quantificationHela cells transfected with the indicated constructs were detached, held in suspension in culture medium supplemented with 20 mM Hepes at 37uC for 1 h and replated on fibronectin (10 mg/ml) coated glass dish. After the indicated time of replating, the cells were fixed for immunfluorescence analysis or observed in live using spinning disk or TIRF-M. For quantification of co-localization between a5-integrin-GFP and Cav1-mRFP at the cell periphery, the area of cell surface was drawn with the Threshold command of MetaMorph 7. A 20-pixel width region from the cell periphery was created using both the Erode and Create Region commands of MetaMorph 7. The percentage of co-localization of the two proteins was measured using the Measure Colocalization command of MetaMorph 7 in the 20-pixel region. Statistical analyses were performed using Student’s t test in GraphPad Prism 5 software.Live cell imaging by TIRF and spinning disk confocal microscopyFor live cell imaging by TIRF-M, HeLa cells seeded onto glassbottom dish were transfected with the indicated constructs and imaged the next day with a 1006 1.49 NA TIRF objective on a Nikon TE2000 (Nikon France SAS, Champigny sur Marne, France) inverted microscope equipped with a QuantEM EMCCD camera (Roper Scientific SAS, Evry, France/Photometrics, AZ, USA), a dual output laser launch which included 491 and 561 nm 50 mW DPSS lasers (Roper Scientific), and driven by Metamorph 24195657 7 software (MDS Analytical Technologies). A DV2 beam-splitter system (Roper Scientific/Photometrics) mounted on the light path enabled the simultaneous acquisition of the two emission channels. A motorized device driven by Metamorph allowed accurate positioning of the illumination light for evanescent wave excitation. For spinning disk microscopy, HeLa cells plated onto a glassbottom dish coated with fibronectin (Sigma, 10 mg/ml) and transfected with the indicated constructs. Images were acquired with 100 ms exposure time at 2 or 5 s interval as indicated using a spinning disk microscope based on a CSU22 Yokogawa head mounted on the lateral port of an inverted microscope Leica IRE2 equipped with a 1006 1.4NA Plan-Apo objective and a dual output laser launch which included 491 and 561 nm ERROL laser bench 491 nm, 561 nm (Roper Scientific). Images were acquired with a Camera EMCCD Cascade 5126512 (Photometrics). The system was steered by Metamorph 7 software.Materials and Methods Cell Culture, transfection and siRNA treatmentHela cells were cultured in DMEM medium (GIBCO) containing 15 FCS and 2 mM glutamine at 37uC and 5 CO2. For treatment with cytoskeleton-disassembling drugs, cells were treated fo.

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