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From
The Irreversible Inhibition of the MAPK
p38
Pathway Downregulates LPS-augmented Release of Interleukin-Related Inflammatory Cytokines (IL-1β, IL-6): Immune Surveillance Unraveling IκB-α/NF-κB Phosphorylation State-independent Mechanism
in vitro
John J Haddad
American Journal of Medical and Biological Research
.
2015
, 3(5), 133-138 doi:10.12691/ajmbr-3-5-3
Figure 1
.
Histogram analysis of the cell culture supernatant levels of pro-inflammatory cytokines with selective MAPK
p38
inhibition.
(A)
The levels of IL-1β in the presence or absence of LPS/SB203580.
(B)
The levels of IL-6 in the presence or absence of LPS/SB203580.
(C)
The levels of TNF-α in the presence or absence of LPS/SB203580, shown here for comparison purposes with interleukins, mainly IL-1β and IL-6 . The number of experimental observations is n = 3 – 5, for separate and independently prepared cell cultures of alveolar epithelial cells with or without pre-treatments with LPS/SB203580. *
P
< 0.05, **
P
< 0.01, ***
P
< 0.001, as compared with LPS.
ϕ
P
< 0.001 (LPS), as compared with control baseline
Full size figure and legend
Figure 2
.
Electrophoretic typical gel analysis for the effect of LPS/SB203580 on IκB-α cytosolic phosphorylation.
(A)
Cell cultures were pretreated with ascending concentrations of SB203580 for 1h, followed by incubation with LPS for 24h. The phosphorylated (
p
IκB-α) and non-phosphorylated forms of IκB-α were subsequently determined. Semi-quantitative loading per lane is verified by the consistent expression of the constitutive form of β-actin
(B)
Histogram analysis of the relative levels of
p
IκB-α and IκB-α with selective MAPK
p38
inhibition. The number of experimental observations is n = 3 – 5, for separate and independently prepared cell cultures of alveolar epithelial cells with or without pre-treatments with LPS/SB203580
Full size figure and legend
Figure 3
.
Hypothetical putative pathways depicting the intertwined signaling crosstalk between the MAPK
p38
and NF-κB pathways. The involvement of upstream and downstream kinases in regulating either pathway is also shown. In addition, the selective inhibition of the MAPK
p38
pathway attenuated the release of pro-inflammatory cytokines, however, it contributes to phosphorylation of IκB-α and subsequent NF-κB activation (see Results section for further details)
Full size figure and legend