Application of anisomycin to the axonal compartment for 4 hr resulted in a 62.8% decrease in total axonal SMAD1/5/8 levels, compared to treatment with vehicle (Figures 4A, S4E, and S4F). Together, these data indicate that maintenance of SMAD1/5/8 selleck chemical levels requires intra-axonal protein synthesis. As a second strategy to examine the source of axonal SMAD1/5/8, we performed FRAP (fluorescence recovery after photobleaching) analysis using a photoconvertible reporter of SMAD1 translation. Trigeminal neurons were transfected with a construct
comprising the photoconvertible protein Dendra2 (Chudakov et al., 2007) fused to SMAD1, including its 3′UTR. The axons were severed after 2 days. By examining only severed axons, any possible contribution to axonal SMAD levels by anterograde SMAD transport from the cell body is eliminated. Dendra2-SMAD1-3′UTRSMAD1 was photobleached
in distal axons. Following photobleaching, recovery of green fluorescent Dendra2-SMAD1 was detected within 10 min, with continued increases over 30 min (Figure 4B). This effect was completely blocked by treatment with anisomycin, indicating that local synthesis of SMAD1 accounts for the increase in Dendra2-SMAD1 in distal axons. We next asked if anterograde transport from cell bodies substantially contributes to the levels of SMAD proteins in axons. Dendra2 or Dendra2-SMAD1 was expressed and photoconverted to the red fluorescent form in the cell body. The increase selleck chemicals llc in red signals in distal axons was monitored over 60 min. Red fluorescent Dendra2-SMAD1 protein could not be detected in distal axons, while Dendra2 was readily detected (Figure S4G). These data further support that the idea that axonal SMAD is derived primarily from local synthesis and
not from transport from the cell body. These experiments, as well as an additional approach using axon-specific knockdown of SMAD1, 5, and 8 mRNA (see Figure 6A, below), indicate that SMAD1/5/8 levels in axons are mainly dependent on local synthesis. The rapid decline in axonal SMAD1/5/8 levels following protein synthesis inhibition suggests that SMAD1/5/8 is rapidly turned over in axons. To determine the Isotretinoin mechanism that leads to the loss of SMAD1/5/8 after protein synthesis inhibition, we examined SMAD1/5/8 levels in severed trigeminal axons. Severed axons can remain in culture for at least 2 hr before displaying signs of degeneration (Figure S5A). As expected, axonal SMAD1/5/8 levels dropped significantly upon axonal application of anisomycin (Figure 5A). However, the rapid decline in SMAD1/5/8 levels was not due to proteasomal degradation, since the proteasome inhibitor N-acetyl-L-leucinyl-L-leucinal-L-norleucinal (LLnL), which prevents SMAD degradation ( Gruendler et al., 2001), did not block the decline in axonal SMAD1/5/8 levels ( Figure 5A).