Table 1.
siRNA Sequences.
Figure 1.
Downregulation of RanGAP1 in arrested, differentiated smooth muscle cells (A).
To induce differentiation, CASMCs were depleted from serum. RanGAP1 expression in CASMC was assessed by Western Blotting 12(∼70 kDa) form as well as the SUMO-1 conjugated (∼90 kDa) form of the RanGAP-1 protein. Both bands revealed reduced RanGAP1 expression over time in cells entering quiescence. α-SM Actin protein, a marker of cell differentiation, is increased over time. Actin levels are displayed as loading control. Effect of posttranscriptional gene silencing of RanGAP1 by small interfering RNA (siRNA) on cell cycle and differentiation markers (B). siRNA mediated gene silencing of RanGAP1 was able to reduce the 90 kD band by 31.8±21.2% (90 kD band) and 75%±14.7% (70 kD band) 48 h post transfection, respectively (average of three different experiments). RanGAP1 depletion was associated with a strong increase of p27Kip1 expression by 60±34%. RanGAP1 deficiency was also associated with a sharp increase in desmin expression with levels even higher than in quiescent cells. CASMC denotes coronary artery smooth muscle cells; (+) denotes serum stimulated CASMC; (−) denotes quiescent CASMC (≥72 h serum depletion); “control” denotes oligofectamine transfected cells without siRNAs; siRNA-SCR denotes scrambled (control) siRNA.
Figure 2.
Gene silencing of RanGAP1 by siRNA in CASMC.
CASMC fixed and permeabilized with 4% PFA and 0.2% Triton X-100 were subjected to indirect immunofluorescence with an RanGAP1 antibody. CASMC treated with control scrambled siRNA reveal accumulation of RanGAP1 expression at the nuclear rim rather than in the cytosol (a–c). Likewise, siRNA-RanGAP1 mediated gene silenced CASMC show a residual RanGAP1 expression mainly at the nuclear rim (d–f). Gene silencing of RanGAP1 by means of specific siRNA transfection lead to inhibition of proliferation by 57.4±4.8% (p<0.0001) (g). Similarly, mitogen-induced CASMC migration was sharply inhibited by 48±9% in RanGAP1 siRNA transfected cells (p = 0.0001) (h). Concomitantly, the phenotype of siRNA RanGAP1 treated CASMC showed a significant difference in the cellular size index (length/width; 7.8±2.5 vs. 2.5±0.9 p = 0.002) (i), indicating a phenotypic change that is consistent with contractile, quiescent CASMC.
Figure 3.
RanGAP1 expression in the rat carotid artery injury model.
To determine the spatiotemporal expression pattern of RanGAP1 during the course of neointima formation, the rat carotid injury model was applied. Immunohistochemical staining revealed upregulation of RanGAP1 at day 3 (b, f, j, and day 7 (c, g, k) whereas RanGAP1 expression ceased when SMC proliferation decreases at day 14 (d, h, l) subsequent to balloon injury.
Figure 4.
Quantitative morphometric and immunohistochemical analysis of neointima formation and RanGAP1 expression in the rat carotid artery injury model.
No significant difference was detectable between the injured group compared to non-injured control arteries with respect to medial area at 3 days, 7 days and 14 days post injury (A) (p = 0.58). Of note, we observed in the media a trend towards a cellular upregulation of RanGAP1 (p = 0.08) 3 days after injury concomitantly with the beginning of cellular proliferation as a response to vascular injury. The increase of neointimal area was detectable at day 7 and peaked at 14 days following vascular injury (B) (p<0.0001). RanGAP1 expression in the media was the highest at the initiation of cellular proliferation and decreased to barely detectable levels at the completion of neointima formation (C). 3 days post injury, almost all cells in the neointima stained positive for RanGAP1 and subsequently, levels decrementally decreased at later time points, e.g. at day 7 and day 14 (D). In non-injured control sections, RanGAP1 expression was virtually undetectable.
Figure 5.
Model: RanGAP1, a key player in nucleocytoplasmic transport, plays a critical role in smooth muscle cell differentiation, migration and proliferation.
Appropriate modulation of RanGAP1 expression may thus be a strategy to modulate vascular proliferative disease development such as restenosis.