Caveolin-1 Silencing by siRNA

The small interfering (si)RNA that were designed to specifically target the coding region of Cav1 (siCav1) mRNA was purchased from Dharmacon Inc (Lafayette, CO). Scrambled control siRNA (C‐siRNA), which had no sequence homology to any known genes, was used as the control. The siCav1 and C‐siRNA were transfected into cells as described previously (Rao et al. 2006 (link), 2010 (link); Zhuang et al. 2013 (link)). Briefly, for each 60‐mm cell culture dish, 20 μL of the 5 μmol/L stock siCav1, or C‐siRNA was mixed with 500 μL of Opti‐MEM medium (Invitrogen). This mixture was added to a solution containing LipofectAMINE 2000 in 500 μL of Opti‐MEM. The solution was incubated for 20 min at room temperature and gently overlaid onto monolayers of cells in 3 mL of medium, and cells were harvested for various assays after 48‐h incubation.

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Rathor N., Chung H.K., Wang S.R., Wang J., Turner D.J, & Rao J.N. (2014). Caveolin‐1 enhances rapid mucosal restitution by activating TRPC1‐mediated Ca2+ signaling. Physiological Reports, 2(11), e12193.

Publication 2014

siCav1) C‐siRNA Opti‐MEM medium

Assays Cav1 Cell culture Cells Dish Genes Lipofectamine 2000 Mrna Sirna

Corresponding Organization : Baltimore VA Medical Center

Top 5 similar protocols

Variable analysis

independent variables

SiCav1 (small interfering RNA that targets the coding region of Cav1 mRNA)
C-siRNA (scrambled control siRNA)

dependent variables

Not explicitly mentioned

control variables

Cell culture dish size (60-mm)
Volume of Opti-MEM medium (500 μL)
Incubation time (20 min at room temperature)
Volume of medium for cell monolayers (3 mL)
Incubation time for cells (48-h)

controls

Positive control: siCav1 (small interfering RNA that targets the coding region of Cav1 mRNA)
Negative control: C-siRNA (scrambled control siRNA)

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