On the basis of these consideration

On the basis of these considerations, we next verified the ef-
fect of ESW on nNOS activity and on intracellular NO pro-
duction in the presence of iNOS inducers. As expected, a
mixture of 1 lg/ml LPS, 10 ng/ml IFN-c plus 10 ng/ml TNF-
a (MIX) rapidly and gradually decreased nNOS activity in
C6 cells, reaching an undetectable value after 1 h of treatment
(Fig. 3A). Note that at these concentrations, MIX promoted
maximal activation of NF-jB and iNOS expression (see be-
low). As shown in Fig. 3A, treatment of MIX-stimulated C6
cells with ESW (0.03 mJ/mm2
, 500 shots) fully reversed the
suppressive effect of MIX on nNOS activity at any time point
examined (i.e., 30 min and 1 h). Further analyses using the
DAF-2DA detection system confirmed the above results and
revealed that ESW treatment brought DAF-2T fluorescence
back to the control value, thus counteracting the MIX-trig-gered drop in NO production (Fig. 3B). This persisting effect
strongly suggests that this may take place when ESW are ther-
apeutically employed, the kinetic data being consistent with
the clinically observed long-lasting results of ESW treatment.
Thus, the clinically observed beneficial effects of ESW fit, at
least in part, to their ability of keeping NO amount at the basal
level, despite the presence of pro-inflammatory cytokines.
Because it is well established that suppression of cNOS activ-
ity represents an early, necessary event for cytokine-induced
NF-jB activation and iNOS expression, the effect of ESW in
these responses was investigated next.
In order to address whether ESW could interfere with the
MIX-elicited NF-jB activation, the DNA-binding activity of
NF-jB was measured by using EMSA assay. As expected,
exposure of C6 cells to MIX for 30–60 min caused rapid
activation of NF-jB(Fig. 4A, lanes 3 and 5, respectively). It
is important to recall that under these conditions, MIX was
able to quickly inhibit nNOS activity in C6 cells. Interestingly,
when C6 cells were incubated with MIX in the presence of
concomitant ESW treatment, a downregulation of NF-jB
activation was observed. The maximal effect was reached after
a 60-min treatment (Fig. 4A, lane 6), although a partial
reduction of DNA binding was also found after a 30-min
treatment (Fig. 4A, lane 4). Treatment of cells with ESW alone
did not affect NF-jB activation (Fig. 4A, lane 2).The inhibitory effect of ESW on MIX-elicited NF-jB activa-
tion was mimicked by treating C6 cells with the NO donor
NOR-3 (400 lM) for 30 min (Fig. 4B, lane 5), whereas it was
completely reversed when C6 cells were pre-incubated with
1mM L L-NAME for 30 min (Fig. 4B, lane 4). Finally, treat-
ment of MIX-stimulated cells with 1 mM L L-NAME for
30 min increased NF-jB activation (Fig. 4B, lane 3) with re-
spect to MIX treatment (Fig. 4B, lane 2).
These results indicate that ESW, being able to rapidly en-
hance nNOS activity, efficiently reduced MIX-elicited NF-jB
activation, confirming the notion that physiologically pro-
duced NO levels keep NF-jB activation suppressed
[17,26,27]. In order to prove that the observed downregulation
of NF-jB activation by ESW ended up in transcriptional
depression of NF-jB-dependent genes, iNOS mRNA expres-
sion levels were analyzed. In this respect, C6 cells were treated
with ESW (0.03 mJ/mm2
with 500 and 1000 shots) at the same
time points of MIX administration, and then kept in the incu-
bator for 3–4 h. By using Northern blot analysis, we confirmed
that MIX treatment induced iNOS mRNA expression, the
peak being observed after 4 h of treatment (Fig. 5, lane 7).
Interestingly, ESW downregulated MIX-induced iNOS gene
expression and the maximum effect was reached with 500 shots
(Fig. 5, lane 9). An identical outcome was obtained by using
RT-PCR analysis (Fig. 6).
Since NF-jB activation is a key event in the induction of a
number of inflammatory cytokines, the effect of ESW treat-ment on TNF-a gene expression was also analyzed. By using
RT-PCR, we found that the treatment with ESW (in particular
when used at 500 shots) strongly inhibited TNF-a mRNA
expression induced by MIX for 4 h, although a complete inhi-
bition was never attained (Fig. 6).
Altogether, these results identify ESW therapy as a possible
useful tool for downregulating NF-jB and NF-jB-dependent
genes (e.g., iNOS and TNF-a), leading to a drastic reduction
in the whole inflammatory process. On the other hand, poten-
tially beneficial effects of ESW due to their capacity of enhanc-ing eNOS activity in endothelial cells have been recently re-
ported [13]. Furthermore, the same report indicates that
ESW treatment is capable not only to prevent but also down-
regulate NF-jB activation, in line with clinical observations of
a positive anti-inflammatory action of ESW treatment in most
patients with ongoing inflammatory events.
In conclusion, the results obtained in C6 cells provide evi-
dence that clinically observed ESW anti-inflammatory action
may be exerted, at least in part, by counteracting the cyto-
kine-induced drop in constitutive NOS activity. Maintenance
of the proper amounts of NO may contribute to contrast the
cytokine-elicited NF-jB activation and the successive induc-
tion of NF-jB-dependent genes, including iNOS and TNF-a.
However, further studies are needed to investigate this mecha-
nism in vivo.