Abstract
α-Lipoic acid (ALA) and its reduced form dihydrolipoic acid (DHLA) are powerful antioxidants both in hydrophilic and lipophylic environments with diverse pharmacological properties including anti-inflammatory activity. The mechanism of anti-inflammatory activity of ALA and DHALA is not known. The present study describes the interaction of ALA and DHALA with pro-inflammatory secretory PLA 2 enzymes from inflammatory fluids and snake venoms. In vitro enzymatic inhibition of sPLA 2 from Vipera russellii, Naja naja and partially purified sPLA 2 enzymes from human ascitic fluid (HAF), human pleural fluid (HPF) and normal human serum (HS) by ALA and DHLA was studied using 14C-oleate labeled Escherichia coli as the substrate. Biophysical interaction of ALA with sPLA 2 was studied by fluorescent spectral analysis and circular dichroism studies. In vivo anti-inflammatory activity was checked using sPLA 2 induced mouse paw edema model. ALA but not DHLA inhibited purified sPLA 2 enzymes from V. russellii, N. naja and partially purified HAF, HPF and HS in a dose dependent manner. This data indicated that ALA is critical for inhibition. IC 50 value calculated for these enzymes ranges from 0.75 to 3.0 μM. The inhibition is independent of calcium and substrate concentration. Inflammatory sPLA 2 enzymes are more sensitive to inhibition by ALA than snake venom sPLA 2 enzymes. ALA quenched the fluorescence intensity of sPLA 2 enzyme in a dose dependent manner. Apparent shift in the far UV-CD spectra of sPLA 2 with ALA indicated change in its α-helical confirmation and these results suggest its direct interaction with the enzyme. ALA inhibits the sPLA 2 induced mouse paw edema in a dose dependent manner and confirms the sPLA 2 inhibitory activity in vivo also. These data suggest that ALA may act as an endogenous regulator of sPLA 2 enzyme activity and suppress inflammatory reactions.
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