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Neutrophil elastase and proteinase 3 trafficking routes in myelomonocytic cells.

Källquist, Linda LU ; Rosén, Hanna ; Nordenfelt, Pontus LU orcid ; Calafat, Jero ; Janssen, Hans ; Persson, Ann-Maj LU ; Hansson, Markus LU orcid and Olsson, Inge LU (2010) In Experimental Cell Research Okt. p.3182-3196
Abstract
Neutrophil elastase (NE) and proteinase 3 (PR3) differ in intracellular localization, which may reflect different trafficking mechanisms of the precursor forms when synthesized at immature stages of neutrophils. To shed further light on these mechanisms, we compared the trafficking of precursor NE (proNE) and precursor PR3 (proPR3). Like proNE [1], proPR3 interacted with CD63 upon heterologous co-expression in COS cells but endogenous interaction was not detected although cell surface proNE/proPR3/CD63 were co-endocytosed in myelomonocytic cells. Cell surface proNE/proPR3 turned over more rapidly than cell surface CD63 consistent with processing/degradation of the pro-proteases but recycling of CD63. Colocalization of proNE/proPR3/CD63... (More)
Neutrophil elastase (NE) and proteinase 3 (PR3) differ in intracellular localization, which may reflect different trafficking mechanisms of the precursor forms when synthesized at immature stages of neutrophils. To shed further light on these mechanisms, we compared the trafficking of precursor NE (proNE) and precursor PR3 (proPR3). Like proNE [1], proPR3 interacted with CD63 upon heterologous co-expression in COS cells but endogenous interaction was not detected although cell surface proNE/proPR3/CD63 were co-endocytosed in myelomonocytic cells. Cell surface proNE/proPR3 turned over more rapidly than cell surface CD63 consistent with processing/degradation of the pro-proteases but recycling of CD63. Colocalization of proNE/proPR3/CD63 with clathrin and Rab 7 suggested trafficking through coated vesicles and late endosomes. Partial caveolar trafficking of proNE/CD63 but not proPR3 was suggested by colocalization with caveolin-1. Blocking the C-terminus of proNE/proPR3 by creating a fusion with FK506 binding protein inhibited endosomal re-uptake of proNE but not proPR3 indicating "pro(C)"-peptide-dependent structural/conformational requirements for proNE but not for proPR3 endocytosis. The NE aminoacid residue Y199 of a proposed NE sorting motif that interacts with AP-3 [2] was not required for proNE processing, sorting or endocytosis in rat basophilic leukemia (RBL) cells expressing heterologous Y199-deleted proNE; this suggests operation of another AP-3-link for proNE targeting. Our results show intracellular multi-step trafficking to be different between proNE and proPR3 consistent with their differential subcellular NE/PR3 localization in neutrophils. (Less)
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author
; ; ; ; ; ; and
organization
publishing date
type
Contribution to journal
publication status
published
subject
in
Experimental Cell Research
volume
Okt
pages
3182 - 3196
publisher
Academic Press
external identifiers
  • wos:000285218600007
  • pmid:20828556
  • scopus:77958101368
  • pmid:20828556
ISSN
1090-2422
DOI
10.1016/j.yexcr.2010.08.016
language
English
LU publication?
yes
id
9fb4c6b8-1393-4e25-9eeb-567252e6ba7d (old id 1688332)
alternative location
http://www.ncbi.nlm.nih.gov/pubmed/20828556?dopt=Abstract
date added to LUP
2016-04-04 07:54:23
date last changed
2022-01-29 02:43:42
@article{9fb4c6b8-1393-4e25-9eeb-567252e6ba7d,
  abstract     = {{Neutrophil elastase (NE) and proteinase 3 (PR3) differ in intracellular localization, which may reflect different trafficking mechanisms of the precursor forms when synthesized at immature stages of neutrophils. To shed further light on these mechanisms, we compared the trafficking of precursor NE (proNE) and precursor PR3 (proPR3). Like proNE [1], proPR3 interacted with CD63 upon heterologous co-expression in COS cells but endogenous interaction was not detected although cell surface proNE/proPR3/CD63 were co-endocytosed in myelomonocytic cells. Cell surface proNE/proPR3 turned over more rapidly than cell surface CD63 consistent with processing/degradation of the pro-proteases but recycling of CD63. Colocalization of proNE/proPR3/CD63 with clathrin and Rab 7 suggested trafficking through coated vesicles and late endosomes. Partial caveolar trafficking of proNE/CD63 but not proPR3 was suggested by colocalization with caveolin-1. Blocking the C-terminus of proNE/proPR3 by creating a fusion with FK506 binding protein inhibited endosomal re-uptake of proNE but not proPR3 indicating "pro(C)"-peptide-dependent structural/conformational requirements for proNE but not for proPR3 endocytosis. The NE aminoacid residue Y199 of a proposed NE sorting motif that interacts with AP-3 [2] was not required for proNE processing, sorting or endocytosis in rat basophilic leukemia (RBL) cells expressing heterologous Y199-deleted proNE; this suggests operation of another AP-3-link for proNE targeting. Our results show intracellular multi-step trafficking to be different between proNE and proPR3 consistent with their differential subcellular NE/PR3 localization in neutrophils.}},
  author       = {{Källquist, Linda and Rosén, Hanna and Nordenfelt, Pontus and Calafat, Jero and Janssen, Hans and Persson, Ann-Maj and Hansson, Markus and Olsson, Inge}},
  issn         = {{1090-2422}},
  language     = {{eng}},
  pages        = {{3182--3196}},
  publisher    = {{Academic Press}},
  series       = {{Experimental Cell Research}},
  title        = {{Neutrophil elastase and proteinase 3 trafficking routes in myelomonocytic cells.}},
  url          = {{http://dx.doi.org/10.1016/j.yexcr.2010.08.016}},
  doi          = {{10.1016/j.yexcr.2010.08.016}},
  volume       = {{Okt}},
  year         = {{2010}},
}