Apolipoprotein A-I mimetics mitigate intestinal inflammation in a COX2-dependent inflammatory disease model
David Meriwether, Dawoud Sulaiman, Carmen Volpe, Anna Dorfman, Victor Grijalva, Nasrin Dorreh, R. Sergio Solorzano-Vargas, Jifang Wang, Ellen O’Connor, Jeremy Papesh, Muriel Larauche, Hannah Trost, Mayakonda N. Palgunachari, G.M. Anantharamaiah, Harvey R. Herschman, Martin G. Martin, Alan M. Fogelman, Srinivasa T. Reddy
David Meriwether, Dawoud Sulaiman, Carmen Volpe, Anna Dorfman, Victor Grijalva, Nasrin Dorreh, R. Sergio Solorzano-Vargas, Jifang Wang, Ellen O’Connor, Jeremy Papesh, Muriel Larauche, Hannah Trost, Mayakonda N. Palgunachari, G.M. Anantharamaiah, Harvey R. Herschman, Martin G. Martin, Alan M. Fogelman, Srinivasa T. Reddy
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Research Article Gastroenterology

Apolipoprotein A-I mimetics mitigate intestinal inflammation in a COX2-dependent inflammatory disease model

Abstract

Cyclooxygenase 2 (Cox2) total knockout and myeloid knockout (MKO) mice develop Crohn’s-like intestinal inflammation when fed cholate-containing high-fat diet (CCHF). We demonstrated that CCHF impaired intestinal barrier function and increased translocation of endotoxin, initiating TLR/MyD88-dependent inflammation in Cox2-KO but not WT mice. Cox2-MKO increased proinflammatory mediators in LPS-activated macrophages, and in the intestinal tissue and plasma upon CCHF challenge. Cox2-MKO also reduced inflammation resolving lipoxin A4 (LXA4) in intestinal tissue, whereas administration of an LXA4 analog rescued disease in Cox2-MKO mice fed CCHF. The apolipoprotein A-I (APOA1) mimetic 4F mitigated disease in both the Cox2-MKO/CCHF and piroxicam-accelerated Il10–/– models of inflammatory bowel disease (IBD) and reduced elevated levels of proinflammatory mediators in tissue and plasma. APOA1 mimetic Tg6F therapy was also effective in reducing intestinal inflammation in the Cox2-MKO/CCHF model. We further demonstrated that APOA1 mimetic peptides (a) inhibited LPS and oxidized 1-palmitoyl-2-arachidonoyl-sn-phosphatidylcholine–dependent (oxPAPC-dependent) proinflammatory responses in human macrophages and intestinal epithelium, and (b) directly cleared proinflammatory lipids from mouse intestinal tissue and plasma. Our results support a causal role for proinflammatory and inflammation-resolving lipids in IBD pathology and a translational potential for APOA1 mimetic peptides for the treatment of IBD.

Authors

David Meriwether, Dawoud Sulaiman, Carmen Volpe, Anna Dorfman, Victor Grijalva, Nasrin Dorreh, R. Sergio Solorzano-Vargas, Jifang Wang, Ellen O’Connor, Jeremy Papesh, Muriel Larauche, Hannah Trost, Mayakonda N. Palgunachari, G.M. Anantharamaiah, Harvey R. Herschman, Martin G. Martin, Alan M. Fogelman, Srinivasa T. Reddy

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Figure 6

4F inhibits the LPS-mediated proinflammatory response of human macrophages and intestinal epithelium.

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4F inhibits the LPS-mediated proinflammatory response of human macrophag...
(*P < 0.05; **P < 0.01; ***P < 0.001; ****P < 0.0001. (AB) Human THP1 macrophages were treated with 4F (15 μg/mL), LPS (20 ng/mL), or LPS + 4F. (A) 4F significantly inhibited total PGE2 in cell lysates and media for 24 hours (n = 3/group). (B) 4F (4) significantly inhibited LPS dependent (L) IκBα degradation at 30 minutes, as determined by Western blot (NT, no treatment) (left: representative blot; right: densitometric analysis of 3 experiments) (noncontiguous sections of same blots). (C) 4F binds both LPS (left; KD = 0.86 nM) and lipid A (right; KD = 17.5 nM) with high affinity, as determined by surface plasmon resonance analysis. (D) Crypts were isolated from human small intestine and grown into enteroids in matrigel (representative image; scale bar: 200 μm). (EI) Conditioned media from THP-1 cells treated with LPS or LPS + 4F for 4 hours (LPS 4h; LPS + 4F 4h) or 12 hours (LPS 12h; LPS + 4F 12h) was added to the enteroids, and proinflammatory gene expression at 12 hours was determined by qPCR (n = 3/group; Media indicates THP1 media only; fold change vs. NT). For statistical analyses, 1-way (B, E) or 2-way (A) ANOVA with Tukey’s multiple comparisons test and adjusted P values were used.