Role for Cathepsin F in Invariant Chain Processing and Major Histocompatibility Complex Class II Peptide Loading by Macrophages

doi:10.1084/jem.191.7.1177

Published online 3 April 2000.

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© The Rockefeller University Press, 0022-1007/2000/4/1177/ $5.00
The Journal of Experimental Medicine, Volume 191, Number 7, April 3, 2000 1177-1186

Original Article

Role for Cathepsin F in Invariant Chain Processing and Major Histocompatibility Complex Class II Peptide Loading by Macrophages

Guo-Ping Shi^a, Rebecca A.R. Bryant^b, Richard Riese^a, Steven Verhelst^b, Christoph Driessen^b, Zhenqiang Li^c, Dieter Bromme^c, Hidde L. Ploegh^b, and Harold A. Chapman^a
^a Department of Medicine, Brigham and Women's Hospital and Harvard Medical School, Harvard Medical School, Boston, Massachusetts 02115
^b Department of Pathology, Harvard Medical School, Boston, Massachusetts 02115
^c Department of Human Genetics, Mount Sinai School of Medicine, New York, New York 10029

Correspondence to: Harold A. Chapman, Pulmonary and Critical Care Div., Rm. L1312, University of California at San Francisco, 505 Parnassus Ave., San Francisco, CA 94143-0111. Tel:415-514-0896 Fax:415-476-5712 E-mail:halchap{at}itsa.ucsf.edu.

The major histocompatibility complex (MHC) class II–associatedinvariant chain (Ii) regulates intracellular trafficking andpeptide loading of MHC class II molecules. Such loading occursafter endosomal degradation of the invariant chain to a ~3-kDpeptide termed CLIP (class II–associated invariant chainpeptide). Cathepsins L and S have both been implicated in degradationof Ii to CLIP in thymus and peripheral lymphoid organs, respectively.However, macrophages from mice deficient in both cathepsinsS and L can process Ii and load peptides onto MHC class II dimersnormally. Both processes are blocked by a cysteine proteaseinhibitor, indicating the involvement of an additional Ii-processingenzyme(s). Comparison of cysteine proteases expressed by macrophageswith those found in splenocytes and dendritic cells revealedtwo enzymes expressed exclusively in macrophages, cathepsinsZ and F. Recombinant cathepsin Z did not generate CLIP fromIi–MHC class II complexes, whereas cathepsin F was asefficient as cathepsin S in CLIP generation. Inhibition of cathepsinF activity and MHC class II peptide loading by macrophages exhibitedsimilar specificity and activity profiles. These experimentsshow that cathepsin F, in a subset of antigen presenting cells(APCs), can efficiently degrade Ii. Different APCs can thususe distinct proteases to mediate MHC class II maturation andpeptide loading.

Key Words: cysteine protease, antigen presentation, protease inhibitor,proteolysis, antigen presenting cell

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