Cathepsin L maturation and activity is impaired in macrophages harboring M. avium and M. tuberculosis

doi:10.1093/intimm/dxl029

International Immunology Advance Access originally published online on April 24, 2006
International Immunology 2006 18(6):931-939; doi:10.1093/intimm/dxl029

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Cathepsin L maturation and activity is impaired in macrophages harboring M. avium and M. tuberculosis

Rajeev M Nepal¹, Stephanie Mampe¹, Brian Shaffer¹, Ann H Erickson² and Paula Bryant¹

¹ Department of Microbiology, Ohio State University, 484 West 12th Avenue, Columbus, OH 43210, USA
² Department of Biochemistry and Biophysics, University of North Carolina, Chapel Hill, NC 27599, USA

Correspondence to: P. Bryant; E-mail: bryant.218{at}osu.edu

Mycobacterium tuberculosis-infected macrophages demonstratediminished capacity to present antigens via class II MHC molecules.Since successful class II MHC-restricted antigen presentationrelies on the actions of endocytic proteases, we asked whetherthe activities of cathepsins (Cat) B, S and L—three majorlysosomal cysteine proteases—are modulated in macrophagesinfected with pathogenic Mycobacterium spp. Infection of murinebone marrow-derived macrophages with either Mycobacterium aviumor M. tuberculosis had no obvious effect on Cat B or Cat S activity.In contrast, the activity of Cat L was altered in infected cells.Specifically, whereas the 24-kDa two-chain mature form of activeCat L predominated in uninfected cells, we observed an increasein the steady-state activity of the precursor single-chain (30kDa) and 25-kDa two-chain forms of the enzyme in cells infectedwith either M. avium or M. tuberculosis. Pulse-chase analysesrevealed that maturation of nascent, single-chain Cat L intothe 25-kDa two-chain form was impaired in infected macrophages,and that maturation into the 24-kDa two-chain form did not occur.Consistent with these data, M. avium infection inhibited theIFN ${gamma}$ -induced secretion of active two-chain Cat L by macrophages.Viable bacilli were not required to disrupt Cat L maturation,suggesting that a constitutively expressed mycobacterial componentwas responsible. The absence of the major active form of lysosomalCat L in M. avium- and M. tuberculosis-infected macrophagesmay influence the types of T cell epitopes generated in theseantigen-presenting cells, and/or the rate of class II MHC peptideloading.

Keywords: antigen-presenting cell, class II MHC, cysteine protease, endocytic pathway

Transmitting editor: H. Ploegh

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