| Literature DB >> 26209628 |
Michael Thiele1, Randolf J Kerschbaumer2, Frederick W K Tam3, Dirk Völkel1, Patrice Douillard1, Alexander Schinagl1, Harald Kühnel1, Jennifer Smith3, John P McDaid3, Gurjeet Bhangal3, Mei-Ching Yu3, Charles D Pusey3, H Terence Cook3, Josef Kovarik4, Erica Magelky5, Atul Bhan6, Manfred Rieger1, Geert C Mudde1, Hartmut Ehrlich1, Bernd Jilma7, Herbert Tilg8, Alexander Moschen8, Cox Terhorst5, Friedrich Scheiflinger1.
Abstract
Macrophage migration inhibitory factor (MIF), a proinflammatory cytokine and counterregulator of glucocorticoids, is a potential therapeutic target. MIF is markedly different from other cytokines because it is constitutively expressed, stored in the cytoplasm, and present in the circulation of healthy subjects. Thus, the concept of targeting MIF for therapeutic intervention is challenging because of the need to neutralize a ubiquitous protein. In this article, we report that MIF occurs in two redox-dependent conformational isoforms. We show that one of the two isoforms of MIF, that is, oxidized MIF (oxMIF), is specifically recognized by three mAbs directed against MIF. Surprisingly, oxMIF is selectively expressed in the plasma and on the cell surface of immune cells of patients with different inflammatory diseases. In patients with acute infections or chronic inflammation, oxMIF expression correlated with inflammatory flare-ups. In addition, anti-oxMIF mAbs alleviated disease severity in mouse models of acute and chronic enterocolitis and improved, in synergy with glucocorticoids, renal function in a rat model of crescentic glomerulonephritis. We conclude that oxMIF represents the disease-related isoform of MIF; oxMIF is therefore a new diagnostic marker for inflammation and a relevant target for anti-inflammatory therapy.Entities:
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Year: 2015 PMID: 26209628 PMCID: PMC4543907 DOI: 10.4049/jimmunol.1500572
Source DB: PubMed Journal: J Immunol ISSN: 0022-1767 Impact factor: 5.422