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Literature DB >> 2454929

An acid protease secreted by transformed cells interferes with antigen processing.

K McCoy¹, S Gal, R H Schwartz, M M Gottesman.

Abstract

The major excreted protein of malignantly transformed mouse fibroblasts (MEP), which is the precursor to lysosomal cathepsin L, was used to study the effect of exogenous acid proteases on antigen processing. When MEP and native pigeon cytochrome c were added to Chinese hamster ovary (CHO) cells expressing transfected major histocompatability complex class II gene products, the antigen-specific T-cell hybridoma 2B4 did not respond to the antigen. MEP appears to destroy the antigen in an acid compartment of the presenting cell because: (a) MEP is only active as a protease under acid conditions; (b) mannose 6-phosphate inhibited the internalization of MEP and blocked its effect on antigen processing; (c) the destruction required the simultaneous entry of the antigen and MEP into the cells; and (d) cytochrome c fragment 66-104 which does not need to be processed stimulated 2B4 in the presence of MEP. These results support the hypothesis that antigen processing requires internalization of the antigen into an acidic compartment, and they provide a new model for the investigation of the contribution of acid proteases to the reduced immunocompetence of tumor-bearing animals.

Entities: CellLine Chemical Disease Gene Species

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Year: 1988 PMID： 2454929 PMCID： PMC2115144 DOI： 10.1083/jcb.106.6.1879

Source DB: PubMed Journal: J Cell Biol ISSN： 0021-9525 Impact factor: 10.539

40 in total

1. Cleavage of the tryptophanyl peptide bond by dimethyl sulfoxide-hydrobromic acid.

Authors: W E Savige; A Fontana
Journal: Methods Enzymol Date: 1977 Impact factor: 1.600

2. Isolation of mutants of cultured mammalian cells.

Authors: L H Thompson; R M Baker
Journal: Methods Cell Biol Date: 1973 Impact factor: 1.441

3. Cleavage of cytochrome c with cyanogen bromide.

Authors: G Corradin; H A Harbury
Journal: Biochim Biophys Acta Date: 1970-12-22

4. Tumor promoters and Kirsten sarcoma virus increase synthesis of a secreted glycoprotein by regulating levels of translatable mRNA.

Authors: M M Gottesman; M E Sobel
Journal: Cell Date: 1980-02 Impact factor: 41.582

5. Differences in secretion of the proteinase cathepsin B at the edges of human breast carcinomas and fibroadenomas.

Authors: A R Poole; K J Tiltman; A D Recklies; T A Stoker
Journal: Nature Date: 1978-06-15 Impact factor: 49.962

6. Transformation-dependent secretion of a low molecular weight protein by murine fibroblasts.

Authors: M M Gottesman
Journal: Proc Natl Acad Sci U S A Date: 1978-06 Impact factor: 11.205

7. The identification of the major excreted protein (MEP) from a transformed mouse fibroblast cell line as a catalytically active precursor form of cathepsin L.

Authors: R W Mason; S Gal; M M Gottesman
Journal: Biochem J Date: 1987-12-01 Impact factor: 3.857

5. Glycosylation of procathepsin L does not account for species molecular-mass differences and is not required for proteolytic activity.

Authors: S M Smith; S E Kane; S Gal; R W Mason; M M Gottesman
Journal: Biochem J Date: 1989-09-15 Impact factor: 3.857

6. Expression and deletion analysis of the Trypanosoma brucei rhodesiense cysteine protease in Escherichia coli.

Authors: E G Pamer; C E Davis; M So
Journal: Infect Immun Date: 1991-03 Impact factor: 3.441

7. Epitope-directed processing of specific antigen by B lymphocytes.

Authors: H W Davidson; C Watts
Journal: J Cell Biol Date: 1989-07 Impact factor: 10.539

7 in total

An acid protease secreted by transformed cells interferes with antigen processing.

1. Cleavage of the tryptophanyl peptide bond by dimethyl sulfoxide-hydrobromic acid.

2. Isolation of mutants of cultured mammalian cells.

3. Cleavage of cytochrome c with cyanogen bromide.

4. Tumor promoters and Kirsten sarcoma virus increase synthesis of a secreted glycoprotein by regulating levels of translatable mRNA.

5. Differences in secretion of the proteinase cathepsin B at the edges of human breast carcinomas and fibroadenomas.

6. Transformation-dependent secretion of a low molecular weight protein by murine fibroblasts.

7. The identification of the major excreted protein (MEP) from a transformed mouse fibroblast cell line as a catalytically active precursor form of cathepsin L.

8. Hybridoma cell lines secreting monoclonal antibodies to mouse H-2 and Ia antigens.

9. Purification and characterization of a transformation-dependent protein secreted by cultured murine fibroblasts.

10. Monoclonal cytolytic T-cell lines.

1. Cathepsins L and S are not required for activation of dipeptidyl peptidase I (cathepsin C) in mice.

2. Expression and immunohistochemical localization of cathepsin L during the progression of human gliomas.

3. Cathepsin L colocalizes with chromogranin a in chromaffin vesicles to generate active peptides.

4. Cathepsin D is up-regulated in inflammatory bowel disease macrophages.

5. Glycosylation of procathepsin L does not account for species molecular-mass differences and is not required for proteolytic activity.

6. Expression and deletion analysis of the Trypanosoma brucei rhodesiense cysteine protease in Escherichia coli.

7. Epitope-directed processing of specific antigen by B lymphocytes.