Your search keyword '"Granzyme M"' showing total 99 results

51. New Paradigm for Lymphocyte Granule-mediated Cytotoxicity

Author

Girish M. Shah, B M Babior, R. Christopher Bleackley, Jane Turbov, Roberta A. Gottlieb, Kim Orth, W. L. Hanna, Vishva M. Dixit, Prem Seth, and Christopher J. Froelich

Subjects

biology, Pinocytosis, Cell Biology, Biochemistry, Jurkat cells, Cell biology, Granzyme B, Granzyme, Perforin, Apoptosis, Annexin, biology.protein, Granzyme M, Molecular Biology

Abstract

Lymphocyte granule-mediated apoptosis is postulated to entail the formation of membrane pores by perforin. Then soluble granzyme reaches the cytosol either through these pores or by reparative pinocytosis. We demonstrate here that Jurkat cells bind and internalize granzyme B via high affinity binding sites without toxic consequence. Apoptosis occurs, however, if sublytic perforin is added to targets washed free of soluble granzyme B. We suggest that granule-mediated apoptosis mimics viral strategies for cellular entry. Accordingly, co-internalization of granzyme B with adenovirus, a virus that escapes endosomes to reach the cytosol, also induced apoptosis. Poly(ADP-ribose) polymerase cleavage and processing of CPP32, ICE-LAP3, and Mch2 were detected at 30 min, while cytosolic acidification and DNA fragmentation occurred at 60 min. Annexin V binding and membrane permeabilization arose at 4 h. The concurrent activation of the Ced-3 proteases differed from the rate at which each cysteine protease is cleaved in vitro by granzyme B. Thus, granzyme B may not directly process these proteases in whole cells but rather may function by activating a more proximal enzyme. These results indicate that adenovirus-mediated delivery of granzyme B is suitable for elucidating biochemical events that accompany granule-mediated apoptosis.

Published

1996

52. Granzyme A is critical for recovery of mice from infection with the natural cytopathic viral pathogen, ectromelia

Author

Ron Tha Hla, Klaus Ebnet, Markus M. Simon, Thomas Stehle, Robert V. Blanden, Crisan Museteanu, and Arno Müllbacher

Subjects

Multidisciplinary, Effector, Serine Endopeptidases, Orthopoxvirus, Poxviridae Infections, Biology, Granzymes, Cell Line, Cell biology, Granzyme B, Mice, Cytolysis, Liver, Perforin, Granzyme, Cell culture, Granzyme A, biology.protein, Animals, Genetic Predisposition to Disease, Granzyme M, Spleen, Research Article

Abstract

Cytolytic lymphocytes are of cardinal importance in the recovery from primary viral infections. Both natural killer cells and cytolytic T cells mediate at least part of their effector function by target cell lysis and DNA fragmentation. Two proteins, perforin and granzyme B, contained within the cytoplasmic granules of these cytolytic effector cells have been shown to be directly involved in these processes. A third protein contained within these granules, granzyme A, has so far not been attributed with any biological relevance. Using mice deficient for granzyme A, we show here that granzyme A plays a crucial role in recovery from the natural mouse pathogen, ectromelia, by mechanisms other than cytolytic activity.

Published

1996

53. Localization of Granzyme B in the Nucleus

Author

Joseph A. Trapani, Mark J. Smyth, Kylie A. Browne, and David A. Jans

Subjects

Proteases, biology, Cell Biology, Biochemistry, Cell biology, Granzyme B, Cell nucleus, medicine.anatomical_structure, Perforin, Granzyme, biology.protein, medicine, Cytotoxic T cell, Nuclear transport, Granzyme M, Molecular Biology

Abstract

One mechanism used by cytotoxic T cells and natural killer cells to kill target cells involves synergy between the pore-forming protein, perforin, and a serine protease termed granzyme B, both constituents of the cytoplasmic granules of cytolytic lymphocytes. Exposing susceptible cells to perforin and granzyme B results in apoptosis, the morphological consequences of which are most clearly seen in the nucleus. It is conventionally accepted that perforin acts by perforating the target cell membrane; however, the site and mode of action of granzyme B are unknown. We have addressed this issue using Western blotting, proteolytic assays, and confocal laser scanning microscopy to demonstrate that purified human granzyme B can be taken up in large amounts and bound within nuclei. By contrast, perforin and nongranzyme serine proteases did not undergo nuclear uptake. Both unglycosylated human granzyme B (26 kDa) and that bearing high mannose glycosylation (32 kDa) were internalized and bound within nuclei, but forms greater than 32 kDa with complex carbohydrate addition were excluded. The uptake of granzymes was not dependent on net charge, as nuclei absorbed similar quantities of granzyme B at neutral pH and through a range of basic pHs but did not take up other very basic serine proteases such as the mouse mast cell protease 5. Confocal laser scanning microscopy indicated nuclear and nucleolar accumulation of fluoresceinated granzyme B by isolated nuclei. Measurement of the kinetics of nuclear import using an in vitro nuclear transport assay indicated maximal levels of nuclear accumulation of granzyme about 2.5-fold above those in the cytoplasm and nucleolar accumulation a further 3-4-fold higher. Nuclear and nucleolar accumulation were exceedingly rapid, reaching half-maximal levels within 3.3 and 7.5 min, respectively, implying that nuclear accumulation probably occurs prior to transport to the nucleolus. Our observations may provide a mechanism explaining how aspartate-specific cell death proteases access the nuclear substrate poly(ADP-ribose) polymerase, the cleavage of which is an early event in apoptosis.

Published

1996

54. Granzyme M has a critical role in providing innate immune protection in ulcerative colitis

Author

Y Krasnova, Gabrielle T. Belz, Hazel Tye, Kim Miles, Nicholas D. Huntington, Lisa A. Mielke, Mark J. Smyth, W Shi, L McDade, Glenda C. Gobe, Kelli P. A. MacDonald, Seth L. Masters, Liam Town, Graham L. Radford-Smith, Tracy L Putoczki, and Fernando Souza-Fonseca-Guimaraes

Subjects

0301 basic medicine, Cancer Research, Colon, Immunology, Gene Expression, Inflammation, Biology, Inflammatory bowel disease, Granzymes, Permeability, 03 medical and health sciences, Cellular and Molecular Neuroscience, Mice, Immune system, Crohn Disease, medicine, Animals, Humans, RNA, Messenger, Colitis, Intestinal Mucosa, Innate immune system, Dextran Sulfate, Cell Biology, medicine.disease, Ulcerative colitis, digestive system diseases, Immunity, Innate, Killer Cells, Natural, Mice, Inbred C57BL, 030104 developmental biology, Granzyme, Neutrophil Infiltration, biology.protein, Original Article, Colitis, Ulcerative, Female, medicine.symptom, Granzyme M

Abstract

Inflammatory bowel disease (IBD) is an immunoregulatory disorder, associated with a chronic and inappropriate mucosal immune response to commensal bacteria, underlying disease states such as ulcerative colitis (UC) and Crohn’s disease (CD) in humans. Granzyme M (GrzM) is a serine protease expressed by cytotoxic lymphocytes, in particular natural killer (NK) cells. Granzymes are thought to be involved in triggering cell death in eukaryotic target cells; however, some evidence supports their role in inflammation. The role of GrzM in the innate immune response to mucosal inflammation has never been examined. Here, we discover that patients with UC, unlike patients with CD, display high levels of GrzM mRNA expression in the inflamed colon. By taking advantage of well-established models of experimental UC, we revealed that GrzM-deficient mice have greater levels of inflammatory indicators during dextran sulfate sodium (DSS)-induced IBD, including increased weight loss, greater colon length reduction and more severe intestinal histopathology. The absence of GrzM expression also had effects on gut permeability, tissue cytokine/chemokine dynamics, and neutrophil infiltration during disease. These findings demonstrate, for the first time, that GrzM has a critical role during early stages of inflammation in UC, and that in its absence colonic inflammation is enhanced.

Published

2016

55. Granzymes: exogenous porteinases that induce target cell apoptosis

Author

Joseph A. Trapani and Mark J. Smyth

Subjects

Programmed cell death, biology, Cell Cycle, Serine Endopeptidases, Immunology, Apoptosis, Cell cycle, Biological Evolution, Models, Biological, Rats, Cell biology, Killer Cells, Natural, Mice, Granzyme, Perforin, Viruses, biology.protein, Animals, Humans, Cytotoxic T cell, Neoplastic transformation, Granzyme M, T-Lymphocytes, Cytotoxic

Abstract

Cytotoxic lymphocytes mediate immunity against viruses and surveillance against neoplastic transformation. They kill target cells by multiple mechanisms, but utilize a pore-forming protein, perforin, and a family of serine proteinases as their principal means of inflicting cell death. Recent studies have demonstrated that perforin and serine proteinases synergistically trigger an endogenous pathway of apoptosis resulting in dissolution of the target cell nuclear membrane and DNA fragmentation. These changes may be secondary to inappropriate activation of p34cdc2 kinase and the subsequent derangement of cell cycle control. As discussed by Mark Smyth and Joseph Trapani, the immediate molecular targets of perforin/granzyme-mediated apoptosis are still unclear, though candidate molecules with homology to cell death gene products from primitive organisms are currently under close scrutiny.

Published

1995

56. Cytotoxic lymphocytes require granzyme B for the rapid induction of DNA fragmentation and apoptosis in allogeneic target cells

Author

Sujan Shresta, Jonathan W. Heusel, Robin L. Wesselschmidt, John H. Russell, and Timothy J. Ley

Subjects

Apoptosis, Lymphocyte Activation, Granzymes, General Biochemistry, Genetics and Molecular Biology, Mice, Animals, Cytotoxic T cell, Fragmentation (cell biology), biology, Stem Cells, Serine Endopeptidases, DNA, Embryo, Mammalian, Molecular biology, Mice, Mutant Strains, Hematopoiesis, Killer Cells, Natural, Mice, Inbred C57BL, Granzyme B, Granzyme, Multigene Family, Mutation, biology.protein, Granzyme A, DNA fragmentation, Granzyme K, Lymphocyte Culture Test, Mixed, Granzyme M, T-Lymphocytes, Cytotoxic

Abstract

We have generated H-2b mice with a homozygous null mutation in the granzyme (gzm) B gene. Gzm B is a neutral serine protease with Aspase activity that is found only in the granules of activated cytolytic T cells, natural killer cells, and lymphokine-activated killer cells. Gzm B-/- mice develop normally and have normal hematopoiesis and lymphopoiesis. In vitro, cytotoxic T lymphocytes (CTL) derived from gzm B-/- animals are able to induce 51Cr release from allotarget cells, but with reduced efficiency. However, gzm B-/- CTL have a profound defect in their ability to induce rapid DNA fragmentation and apoptosis in allogeneic target cells. This defect is kinetic since DNA fragmentation is partially compensated and 51Cr release is completely rescued with long incubation times. We conclude that gzm B serves a critical and nonredundant role for the rapid induction of target cell DNA fragmentation and apoptosis by alloreactive cytotoxic T lymphocytes.

Published

1994

57. FADD cleavage by NK cell granzyme M enhances its self-association to facilitate procaspase-8 recruitment for auto-processing leading to caspase cascade

Author

Pengyan Xia, Zusen Fan, Linyu Shi, and Shuo Wang

Subjects

Fas-Associated Death Domain Protein, Apoptosis, Caspase 8, urologic and male genital diseases, Jurkat cells, Granzymes, Jurkat Cells, Humans, FADD, CASP, Molecular Biology, Caspase, Death domain, Original Paper, biology, Cell Biology, humanities, Cell biology, Enzyme Activation, Killer Cells, Natural, Granzyme, Gene Knockdown Techniques, Proteolysis, biology.protein, Cancer research, Granzyme M, biological phenomena, cell phenomena, and immunity, Protein Multimerization, HeLa Cells

Abstract

Granzyme M (GzmM), an orphan Gzm, is constitutively and abundantly expressed in innate effector natural killer cells. We previously demonstrated that GzmM induces caspase (casp)-dependent apoptosis and cytochrome c release from mitochondria. We also resolved the crystal structure for GzmM and generated its specific inhibitor. However, how GzmM causes casp activation has not been defined. Here we found that casp-8 is an initiator caspase in GzmM-induced casp cascade, which causes other casp activation and Bid cleavage. GzmM does not directly cleave procaspase-3 and Bid, whose processing is casp dependent. Casp-8 knockdown or deficient cells attenuate or abolish GzmM-induced proteolysis of procaspase-3 and Bid. Extrinsic death receptor pathway adaptor Fas-associated protein with death domain (FADD) contributes to GzmM-induced casp-8 activation. GzmM specifically cleaves FADD after Met 196 to generate truncated FADD (tFADD) that enhances its self-association for oligomerization. The oligomerized tFADD facilitates procaspase-8 recruitment to promote its auto-processing leading to casp activation cascade. FADD-deficient cells abrogate GzmM-induced activation of casp-8 and apoptosis as well as significantly inhibit lymphokine-activated killer cell-mediated cytotoxicity. FADD processing by GzmM can potentiate killing efficacy against tumor cells and intracellular pathogens.

Published

2011

58. Intracellular Serine Protease Inhibitor SERPINB4 Inhibits Granzyme M-Induced Cell Death

Author

Bart Devreese, Razi Quadir, Stefanie A. H. de Poot, D. Margaret Worrall, Anne F. McGettrick, Wayne J. Higgins, Niels Bovenschen, Pieter J.A. de Koning, Roel Broekhuizen, and J. Alain Kummer

Subjects

Cytotoxicity, Immunologic, TUMOR-CELLS, Tumor Physiology, Intracellular Space, lcsh:Medicine, NK cells, CARCINOMA ANTIGEN, LYMPHOCYTES, Jurkat cells, Biochemistry, Granzymes, MEDIATED APOPTOSIS, Substrate Specificity, Jurkat Cells, Molecular Cell Biology, Basic Cancer Research, Cytotoxic T cell, lcsh:Science, Immune Response, Multidisciplinary, Immune System Proteins, Cell Death, Immune cells, Recombinant Proteins, Cell biology, Enzymes, Killer Cells, Natural, B INHIBITOR, Oncology, ENDOGENOUS INHIBITOR, Medicine, Intracellular, Research Article, Protein Binding, EXPRESSION, Programmed cell death, PROTEINS, Immunology, Immunoblotting, T cells, Serpin, Biology, Transfection, Enzyme Regulation, Antigens, Neoplasm, Humans, Immunoprecipitation, Protein Interactions, Serpins, lcsh:R, Biology and Life Sciences, Proteins, CATHEPSIN-G, Molecular biology, Kinetics, HEK293 Cells, Granzyme, Apoptosis, Mutation, biology.protein, lcsh:Q, Granzyme M, MONOCLONAL-ANTIBODIES, HeLa Cells

Abstract

Granzyme-mediated cell death is the major pathway for cytotoxic lymphocytes to kill virus-infected and tumor cells. In humans, five different granzymes (i.e. GrA, GrB, GrH, GrK, and GrM) are known that all induce cell death. Expression of intracellular serine protease inhibitors (serpins) is one of the mechanisms by which tumor cells evade cytotoxic lymphocyte-mediated killing. Intracellular expression of SERPINB9 by tumor cells renders them resistant to GrB-induced apoptosis. In contrast to GrB, however, no physiological intracellular inhibitors are known for the other four human granzymes. In the present study, we show that SERPINB4 formed a typical serpin-protease SDS-stable complex with both recombinant and native human GrM. Mutation of the P2-P1-P1' triplet in the SERPINB4 reactive center loop completely abolished complex formation with GrM and N-terminal sequencing revealed that GrM cleaves SERPINB4 after P1-Leu. SERPINB4 inhibited GrM activity with a stoichiometry of inhibition of 1.6 and an apparent second order rate constant of 1.3x10(4) M(-1) s(-1). SERPINB4 abolished cleavage of the macromolecular GrM substrates alpha-tubulin and nucleophosmin. Overexpression of SERPINB4 in tumor cells inhibited recombinant GrM-induced as well as NK cell-mediated cell death and this inhibition depended on the reactive center loop of the serpin. As SERPINB4 is highly expressed by squamous cell carcinomas, our results may represent a novel mechanism by which these tumor cells evade cytotoxic lymphocyte-induced GrM-mediated cell death.

Published

2011

59. Human and mouse granzyme M display divergent and species-specific substrate specificities

Author

Roel Broekhuizen, Daniel R. Hostetter, Stefanie A. H. de Poot, Kris Gevaert, Charles S. Craik, Marijn Westgeest, Kimberly Demeyer, Kim Plasman, Niels Bovenschen, and Petra Van Damme

Subjects

Models, Molecular, Protein Conformation, Molecular Sequence Data, Biology, Cleavage (embryo), Biochemistry, Granzymes, Cell Line, Substrate Specificity, chemistry.chemical_compound, Mice, Species Specificity, Tubulin, Animals, Humans, Amino Acid Sequence, Molecular Biology, Serine protease, Nucleophosmin, Methionine, Tetrapeptide, Cell Death, Genetic Variation, Nuclear Proteins, Cell Biology, Granzyme, chemistry, Gene Expression Regulation, biology.protein, Leucine, Granzyme M

Abstract

Cytotoxic lymphocyte protease GrM (granzyme M) is a potent inducer of tumour cell death and a key regulator of inflammation. Although hGrM (human GrM) and mGrM (mouse GrM) display extensive sequence homology, the substrate specificity of mGrM remains unknown. In the present study, we show that hGrM and mGrM have diverged during evolution. Positional scanning libraries of tetrapeptide substrates revealed that mGrM is preferred to cleave after a methionine residue, whereas hGrM clearly favours a leucine residue at the P1 position. The kinetic optimal non-prime subsites of both granzymes were also distinct. Gel-based and complementary positional proteomics showed that hGrM and mGrM have a partially overlapping set of natural substrates and a diverged prime and non-prime consensus cleavage motif with leucine and methionine residues being major P1 determinants. Consistent with positional scanning libraries of tetrapeptide substrates, P1 methionine was more frequently used by mGrM as compared with hGrM. Both hGrM and mGrM cleaved α-tubulin with similar kinetics. Strikingly, neither hGrM nor mGrM hydrolysed mouse NPM (nucleophosmin), whereas human NPM was hydrolysed efficiently by GrM from both species. Replacement of the putative P1′–P2′ residues in mouse NPM with the corresponding residues of human NPM restored cleavage of mouse NPM by both granzymes. This further demonstrates the importance of prime sites as structural determinants for GrM substrate specificity. GrM from both species efficiently triggered apoptosis in human but not in mouse tumour cells. These results indicate that hGrM and mGrM not only exhibit divergent specificities but also trigger species-specific functions.

Published

2011

60. A role for granzyme M in TLR4-driven inflammation and endotoxicosis

Author

Phillip I. Bird, Shizou Akira, Sally V. Watt, Desiree A Anthony, Melvyn T. Chow, Joseph A. Trapani, Mark J. Smyth, Daniel M. Andrews, and Colin M. House

Subjects

Lipopolysaccharides, medicine.medical_treatment, Immunology, Inflammation, Biology, Ligands, Granzymes, Mice, medicine, Immunology and Allergy, Cytotoxic T cell, Animals, Myeloid Cells, Mice, Knockout, Shock, Septic, Immunity, Innate, Cell biology, Killer Cells, Natural, Mice, Inbred C57BL, Toll-Like Receptor 4, Cytokine, Granzyme, Perforin, TLR4, biology.protein, Tumor necrosis factor alpha, medicine.symptom, Granzyme M, Inflammation Mediators, Signal Transduction

Abstract

Lymphocyte perforin and serine protease granzymes are well-recognized extrinsic mediators of apoptosis. We now demonstrate that cytotoxic lymphocyte granule components profoundly augment the myeloid cell inflammatory cytokine cascade in response to TLR4 ligation. Whereas caspase-1–deficient mice were completely resistant to LPS, reduced serum cytokine production and resistance to lethal endotoxicosis were also obtained with perforin-deficient mice, indicating a role for granzymes. Consistently, a lack of granzyme M (GrzM) resulted in reduced serum IL-1α, IL-1β, TNF, and IFN-γ levels and significantly reduced susceptibility to lethal endotoxicosis. These altered responses were also observed in granzyme A-deficient but not granzyme B-deficient mice. A role for APC–NK cell cross-talk in the inflammatory cascade was highlighted, as GrzM was exclusively expressed by NK cells and resistance to LPS was also observed on a RAG-1/GrzM-double deficient background. Collectively, the data suggest that NK cell GrzM augments the inflammatory cascade downstream of LPS-TLR4 signaling, which ultimately results in lethal endotoxicosis. Most importantly, these data demonstrate that granzymes should no longer be considered solely as mediators of apoptosis, but additionally as potential key regulators of inflammation.

Published

2010

61. Cleavage of survivin by Granzyme M triggers degradation of the survivin-X-linked inhibitor of apoptosis protein (XIAP) complex to free caspase activity leading to cytolysis of target tumor cells

Author

Lei Shi, Shengwu Liu, Zusen Fan, Chong Li, Deqing Hu, and Lianfeng Wu

Subjects

Programmed cell death, Survivin, X-Linked Inhibitor of Apoptosis Protein, Biology, Inhibitor of apoptosis, Biochemistry, Granzymes, Inhibitor of Apoptosis Proteins, Jurkat Cells, Leucine, Neoplasms, Two-Hybrid System Techniques, Gene silencing, Humans, Gene Silencing, Molecular Biology, Hydrolysis, Cell Biology, Caspase 9, XIAP, Enzyme Activation, Cytolysis, Apoptosis, Caspases, Cancer research, Enzymology, RNA Interference, Granzyme M, Microtubule-Associated Proteins, HeLa Cells

Abstract

Granzyme M (GzmM) is a chymotrypsin-like serine protease that preferentially cuts its substrates after Met or Leu. GzmM is constitutively expressed in activated innate effector natural killer (NK) cells. GzmM-induced cell death is consistent with the kinetics of cytotoxicity of NK cells. These suggest that GzmM may play an important role in innate immunity. Our previous work demonstrated that GzmM induces caspase-dependent apoptosis. However, it is unknown about how GzmM causes caspase activation. Here, we showed that the inhibitor of the apoptosis gene family member Survivin is a physiological substrate for GzmM. GzmM hydrolyzes Survivin at Leu-138 to remove the last four C-terminal residues. The truncated form (sur-TF) is more rapidly hydrolyzed through proteasome-mediated degradation. In addition, Survivin is in complex with X-linked inhibitor of apoptosis protein (XIAP) to inhibit caspase activation as an endogenous inhibitor. Survivin cleavage by GzmM abolishes the stability of the Survivin-XIAP complex and enhances XIAP hydrolysis, which amplifies caspase-9 and 3 activation of target tumor cells. The noncleavable L138A Survivin overexpression can significantly inhibit GzmM-mediated XIAP degradation, caspase activation, and GzmM- and NK cell-induced cytotoxicity. Moreover, Survivin silencing promotes XIAP degradation and enhances GzmM-induced caspase activation as well as GzmM- and NK cell-induced cytolysis of target tumor cells.

Published

2010

62. Purification and cloning of a novel serine protease, RNK-Met-1, from the granules of a rat natural killer cell leukemia

Author

T Wiltrout, J C Powers, Mark J. Smyth, C M Kam, T J Sayers, R Sowder, H A Young, Joseph A. Trapani, L E Henderson, and K S Ottaway

Subjects

chemistry.chemical_classification, Serine protease, Proteases, Norleucine, Cell Biology, Biology, Biochemistry, Molecular biology, Amino acid, Serine, chemistry.chemical_compound, chemistry, biology.protein, Granzyme M, Molecular Biology, Peptide sequence, MASP1

Abstract

We have purified a 30-kDa serine protease (designated RNK-Met-1) from the granules of the rat large granular lymphocyte leukemia cell line (RNK-16) that hydrolytically cleaves model peptide substrates after methionine, leucine, and norleucine (Met-ase activity). Utilizing molecular sieve chromatography, heparin-agarose, chromatography, and reverse-phase high pressure liquid chromatography, RNK-Met-1 was purified to homogeneity and 25 NH2-terminal amino acids were sequenced. By using the polymerase chain reaction, oligonucleotide primers derived from amino acids at position 14-25 and from a downstream active site conserved in other serine protease genes were used to generate a 534-base pair cDNA clone encoding a novel serine protease from RNK-16 mRNA. This cDNA clone was used to isolate a full-length 867-base pair RNK-Met-1 cDNA from an RNK-16 lambda-gt11 library. The open reading frame predicts a mature protein of 238 amino acids with two potential sites for N-linked glycosylation. The cDNA also encodes a leader peptide of at least 20 amino acids. The characteristic Ile-Ile-Gly-Gly amino acids of the NH2 terminus and the His, Asp, and Ser residues that form the catalytic triad of serine proteases were both conserved. The amino acid sequence has less than 45% identity with any other member of the serine protease family, indicating that RNK-Met-1 is distinct and may itself represent a new subfamily of serine proteases. Northern blot analysis of total cellular RNA detected a single 0.9-kilobase mRNA in the in vitro and in vivo variants of RNK-16 and in spleen-derived plastic-adherent rat lymphokine-activated killer cells. RNK-Met-1 mRNA was not detectable in freshly isolated rat splenocytes, thymocytes, brain, colon, and liver or activated nonadherent rat splenocytes and thymocytes. These data indicate that RNK-Met-1 is a serine protease with unique activity that is expressed in the granules of large granular lymphocytes.

Published

1992

63. Purification of three cytotoxic lymphocyte granule serine proteases that induce apoptosis through distinct substrate and target cell interactions

Author

Arnold H. Greenberg, Lianfa Shi, J. C. Powers, R. Aebersold, and Chih-Min Kam

Subjects

Proteases, Immunology, Molecular Sequence Data, Apoptosis, Tripeptide, Cytoplasmic Granules, Substrate Specificity, Tumor Cells, Cultured, Immunology and Allergy, Animals, Protease Inhibitors, Amino Acid Sequence, Cycloheximide, Serine protease, Deoxyribonucleases, biology, Serine Endopeptidases, Articles, Molecular biology, Rats, Granzyme B, Molecular Weight, Kinetics, Biochemistry, Granzyme, biology.protein, DNA fragmentation, Granzyme K, Electrophoresis, Polyacrylamide Gel, Granzyme M, Oligopeptides, DNA Damage, T-Lymphocytes, Cytotoxic

Abstract

We recently reported the purification of a lymphocyte granule protein called "fragmentin," which was identified as a serine protease with the ability to induce oligonucleosomal DNA fragmentation and apoptosis (Shi, L., R. P. Kraut, R. Aebersold, and A. H. Greenberg. 1992. J. Exp. Med. 175:553). We have now purified two additional proteases with fragmentin activity from lymphocyte granules. The three proteases are of two types; one has the unusual ability to cleave a tripeptide thiobenzyl ester substrate after aspartic acid, similar to murine cytotoxic cell protease I/granzyme B, while two are tryptase-like, preferentially hydrolyzing after arginine, and bear some homology to human T cell granule tryptases, granzyme 3, and Hanukah factor/granzyme A. Using tripeptide chloromethyl ketones, the pattern of inhibition of DNA fragmentation corresponded to the inhibition of peptide hydrolysis. The Asp-ase fragmentin was blocked by aspartic acid-containing tripeptide chloromethyl ketones, while the tryptase fragmentins were inhibited by arginine-containing chloromethyl ketones. The two tryptase fragmentins were slow acting and were partly suppressed by blocking proteins synthesis with cycloheximide in the YAC-1 target cell. In contrast, the Asp-ase fragmentin was fast acting and produced DNA damage in the absence of protein synthesis. Using a panel of unrelated target cells of lymphoma, thymoma, and melanoma origin, distinct patterns of sensitivity to the three fragmentins were observed. Thus, these three granule proteases make up a family of fragmentins that activate DNA fragmentation and apoptosis by acting on unique substrates in different target cells.

Published

1992

64. A natural killer cell granule protein that induces DNA fragmentation and apoptosis

Author

R. P. Kraut, Arnold H. Greenberg, R. Aebersold, and Lianfa Shi

Subjects

Serine Proteinase Inhibitors, DNA damage, Immunology, Molecular Sequence Data, Biology, Granzymes, Coumarins, Sequence Homology, Nucleic Acid, Tumor Cells, Cultured, Immunology and Allergy, Animals, Amino Acid Sequence, Egtazic Acid, Deoxyribonucleases, Cell Death, Serine Endopeptidases, Articles, Molecular biology, Rats, Inbred F344, Chromatin, Rats, Granzyme B, Killer Cells, Natural, Isocoumarins, Apoptosis, Chromatography, Gel, DNA fragmentation, bacteria, Granzyme K, Calcium, Electrophoresis, Polyacrylamide Gel, Cytolysin, Granzyme M, DNA Damage

Abstract

We report the purification from a rat natural killer (RNK) large granular lymphocyte leukemia of a 32-kD granule protein that induces rapid DNA fragmentation and apoptosis. The protein, which we have called "fragmentin," was capable of causing DNA from intact YAC-1 cells to be cleaved into oligonucleosomal-sized fragments and producing severe chromatin condensation within 1 h. Amino acid sequence of tryptic peptides indicated that fragmentin was highly homologous to the NK and T cell granule serine proteases RNK protease 1 and mouse cytotoxic T cell protease I (CCPI)/granzyme B. Preincubation with the serine esterase inhibitor 3,4-dichloroisocoumarin blocked fragmentin-induced DNA damage, but had no effect on cytolysin. Fragmentin activity against four lymphoma target cells was completely dependent on the presence of cytolysin. Fragmentin produced rapid membrane damage as well as DNA fragmentation at nonlytic cytolysin doses, suggesting that fragmentin activity was not limited to its effects on the nucleus. Fragmentin and cytolysin activity were completely inhibited by EGTA, indicating the process was Ca2+ dependent. A role for cytolysin in endocytosis of fragmentin was suggested by the observation that treatment of YAC-1 with cytochalasin B or sodium azide and 2-deoxyglucose blocked DNA fragmentation but not cytolysin activity. A 30-kD N alpha-CBZ-L-lysine thiobenzyl esterase, which copurified with fragmentin, was inactive on its own but was able to synergistically amplify the DNA damage induced by fragmentin in the presence of cytolysin. Fragmentin activity was not dependent on protein synthesis, as cycloheximide treatment of YAC-1 cells did not prevent DNA damage. We postulate that fragmentin is the molecular mediator of NK cell-mediated DNA fragmentation and apoptosis.

Published

1992

65. Granzyme M: characterization with sites of post-translational modification and specific sites of interaction with substrates and inhibitors

Author

Muhammad Saleem Akhtar, Rukhshan Khurshid, Asmat Salim, and Mahjabeen Saleem

Subjects

Models, Molecular, Serine Proteinase Inhibitors, Molecular Sequence Data, Apoptosis, Granzymes, Substrate Specificity, Serine, Genetics, Humans, Binding site, Molecular Biology, Caspase, Myristoylation, Binding Sites, biology, Hydrogen Bonding, General Medicine, Cell biology, Protein Structure, Tertiary, Isoenzymes, Biochemistry, Granzyme, Cytoplasm, biology.protein, Phosphorylation, Granzyme M, Protein Processing, Post-Translational

Abstract

Granzymes kill cells in a variety of ways. They induce mitochondrial dysfunction through caspase dependent and caspase-independent pathways and destroy DNA and the integrity of the nucleus. For gaining a better understanding of the molecular function of granzyme M and its NK cell specificity, structural characterization of this enzyme by molecular modeling as well as its detailed comparison with other granzymes is presented in this study. The study includes mode of action of granzyme M using cationic binding sites, substrate specificity, post-translational structural modification and its functional relationship and interaction of the enzyme with inhibitor in an attempt to explore how the activity of human granzyme M is controlled under physiological conditions. It is concluded from the present study that the post-translational modification, including Oglycosylation of serine, phosphorylation of serine and threonine and myristoylation of glycine, play an important role in the interaction of enzyme with the cell surface membrane and regulate protein trafficking and stability. Phosphorylated serine and threonine also plays a role in tumor elimination, viral clearance and tissue repair. In Gzm M there are cationic sites, cs1 and cs2 that may participate in binding of Gzm M to the cell surface, thereby promoting its uptake and eventual release into the cytoplasm. Gzm M shows apoptotic activity both by caspase dependent and independent pathways. Modeling of inhibitors bound to the granzyme active site shows that the dimer also contributes to substrate specificity in a unique manner by extending the active-site cleft.

Published

2009

66. Structural basis for proteolytic specificity of the human apoptosis-inducing granzyme M

Author

Li Wang, Guoqiang Hua, Lianfeng Wu, Mark Bartlam, Xuan Yang, Kan Liu, Fei Sun, Zusen Fan, and Yujia Zhai

Subjects

Conformational change, Immunology, Biology, Crystallography, X-Ray, Granzymes, Substrate Specificity, Jurkat Cells, Structure-Activity Relationship, Protein structure, Catalytic Domain, Catalytic triad, Hydrolase, Enzyme Stability, Immunology and Allergy, Humans, chemistry.chemical_classification, Serine protease, Tetrapeptide, Hydrolysis, Peptide Fragments, Recombinant Proteins, Protein Structure, Tertiary, Enzyme, chemistry, Biochemistry, Amino Acid Substitution, biology.protein, Mutagenesis, Site-Directed, Granzyme M, Apoptosis Regulatory Proteins

Abstract

Granzyme M (GzmM), a unique serine protease constitutively expressed in NK cells, is important for granule-mediated cytolysis and can induce rapid caspase-dependent apoptosis of tumor cells. However, few substrates of GzmM have been reported to date, and the mechanism by which this enzyme recognizes and hydrolyzes substrates is unknown. To provide structural insights into the proteolytic specificity of human GzmM (hGzmM), crystal structures of wild-type hGzmM, the inactive D86N-GzmM mutant with bound peptide substrate, and the complexes with a catalytic product and with a tetrapeptide chloromethylketone inhibitor were solved to 1.96 Å, 2.30 Å, 2.17 Å and 2.70 Å, respectively. Structure-based mutagenesis revealed that the N terminus and catalytic triad of hGzmM are most essential for proteolytic function. In particular, D86N-GzmM was found to be an ideal inactive enzyme for functional studies. Structural comparisons indicated a large conformational change of the L3 loop upon substrate binding, and suggest this loop mediates the substrate specificity of hGzmM. Based on the complex structure of GzmM with its catalytic product, a tetrapeptide chloromethylketone inhibitor was designed and found to specifically block the catalytic activity of hGzmM.

Published

2009

67. The cytotoxic protease granzyme M is expressed by lymphocytes of both the innate and adaptive immune system

Author

Razi Quadir, Kiki Tesselaar, Pieter J.A. de Koning, Thomas J.H. Volman, J. Alain Kummer, Selcuk Colak, and Niels Bovenschen

Subjects

Cytotoxicity, Immunologic, Lymphocyte, T cell, Immunology, Adaptive Immunity, CD8-Positive T-Lymphocytes, Gene Expression Regulation, Enzymologic, Granzymes, Cell Line, T-Lymphocyte Subsets, medicine, Cytotoxic T cell, Humans, Lymphocytes, Molecular Biology, Innate immune system, biology, Perforin, Antibodies, Monoclonal, Natural killer T cell, Acquired immune system, Immunity, Innate, Cell biology, Killer Cells, Natural, medicine.anatomical_structure, Granzyme, Immune System, biology.protein, Granzyme M

Abstract

The cytotoxic serine protease granzyme M (GrM) is one of the five human granzymes, which are mainly expressed by cytotoxic T lymphocytes and/or NK cells. Upon perforin-dependent entry into a target cell, GrM cleaves specific substrates resulting in the onset of a unique cell death mechanism. However, the role of GrM in pathophysiological conditions is not clear yet. Knowledge of the expression and regulation of GrM by lymphocyte populations is instrumental for a better understanding of the contribution of this unique granzyme in health and disease. Two previous studies demonstrated GrM protein expression by lymphocytes of the innate immune system, i.e., NK cells, NKT cells, and gammadelta T cells, whereas its expression by CD8(+) T cells remained controversial. In the present study, we have investigated the expression and regulation of GrM in lymphocyte subsets in more detail. Flow cytometry analysis with a novel specific antibody against human GrM confirmed high expression of this protease by NK cells, NKT cells, and gammadelta T cells. CD8(+) T cells also expressed GrM and comparing the naive to early effector-memory, to late effector-memory, to effector subset, this expression gradually increased during differentiation. In contrast, CD4(+) T cells hardly expressed GrM. Quantitative PCR analysis for GrM mRNA levels in the diverse lymphocyte sub-populations confirmed the FACS results. GrM protein expression by lymphocyte populations was not significantly affected by a panel of GrB-inducing cytokines, indicating that GrM expression is differentially regulated as compared to GrB. In conclusion, the human cytotoxic protease GrM is, besides by innate immune cells, also expressed by CD8(+) effector T cells, in particular by the differentiated effector CD27(-) CD45RO(-) subset. Our current findings support not only a role for GrM in the innate but also in the adaptive immune response.

Published

2009

68. Nucleophosmin Is Cleaved and Inactivated by the Cytotoxic Granule Protease Granzyme M during Natural Killer Cell-mediated Killing

Author

Roberta Donadini, Sean P. Cullen, Phillip I. Bird, Alexander U. Lüthi, Jan Paul Medema, Seamus J. Martin, Inna S. Afonina, Cancer Center Amsterdam, and Radiotherapy

Subjects

EXPRESSION, CYTOCHROME-C RELEASE, MONOCLONAL-ANTIBODY, Cell Survival, CYTOMEGALOVIRUS, Cell, Apoptosis, Biology, Biochemistry, Jurkat cells, NUCLEOLAR PHOSPHOPROTEIN B23, Granzymes, Natural killer cell, ACTIVATION, Jurkat Cells, medicine, Cytotoxic T cell, Humans, Viability assay, RIBOSOME BIOGENESIS, Molecular Biology, Immunity, Cellular, ACUTE MYELOGENOUS LEUKEMIA, integumentary system, Biology and Life Sciences, Nuclear Proteins, Cell Biology, Molecular biology, Cell biology, APOPTOSIS, Killer Cells, Natural, SERINE-PROTEASE, medicine.anatomical_structure, Granzyme, Virus Diseases, Granzyme A, biology.protein, RNA Interference, Granzyme M, Nucleophosmin

Abstract

Natural killer (NK) cells kill virus-infected or transformed target cells by delivering cytotoxic proteases called granzymes to the target cell cytosol. One of these proteases, granzyme M, is specifically expressed in NK cells and is thought to instigate a form of cell death distinct from that mediated by granzyme A or granzyme B. However, the mechanism of granzyme M-induced cell death is unclear at present, and few substrates for this granzyme have been reported to date. Here we show that the abundant nucleolar phosphoprotein, nucleophosmin (NPM), is cleaved and inactivated by granzyme M. NPM is essential for cell viability as RNA interference-mediated ablation of NPM expression in human cells resulted in spontaneous apoptosis. Significantly, overexpression of wild-type NPM rescued cells treated with NPM small interference RNA, whereas overexpression of the granzyme M-cleaved form of NPM did not. Because NPM is essential for cell viability, these data suggest that targeting of NPM by granzyme M may contribute to tumor cell eradication by abolishing NPM function.

Published

2009

69. Human cytotoxic lymphocyte granzyme B. Its purification from granules and the characterization of substrate and inhibitor specificity

Author

H J Zweerink, D. Boulton, J T Blake, Maureen C. Gammon, Martin Poe, Joseph K. Wu, and Nolan H. Sigal

Subjects

chemistry.chemical_classification, biology, Cell Biology, Trypsin, Biochemistry, Macroglobulin, Granzyme B, chemistry.chemical_compound, Scissile bond, Enzyme, chemistry, Granzyme, biology.protein, medicine, Granzyme M, Molecular Biology, Pepstatin, medicine.drug

Abstract

Granzyme B has been purified to homogeneity from the granules of a human cytolytic lymphocyte line, Q31, in an enzymatically active form by a three-step procedure. Q31 granzyme B hydrolyzed Na-t-butyloxycarbonyl-L-alanyl-L-alanyl-L-aspartyl (Boc-Ala-Ala-Asp) thiobenzyl ester with a kcat of 11 +/- 5 mol/s/mol enzyme and catalytic efficiency kcat/Km of 76,000 +/- 44,000 M-1 s-1. The hydrolysis of Boc-Ala-Ala-Asp thiobenzyl ester by crude Q31 Percoll fractions paralleled the tryptase activity for granule-containing fractions, which showed that granzyme B was associated with granules. When chromatographed on Sephacryl S-300, Q31 granzyme B eluted in two broad bands corresponding to dimer and monomer, both of which electrophoresed at 35 kDa in reducing NaDodSo4 polyacrylamide, and both of which showed a lag phase in assays. The lag phase in assays could be extended with 0.03 mM pepstatin. Upon elution from ion-exchange chromatography Q31 granzyme B electrophoresed at 32 kDa in reducing NaDodSO4 polyacrylamide and did not have a lag phase in assays. The amino-terminal sequence of the 32-kDa Q31 granzyme B was identical to four other human cytotoxic T-lymphocyte granzymes B in 18 of 18 positions sequenced. Purified Q31 granzyme B had a preference for substrates with Glu or Asp as the residue amino-terminal to the scissile bond; little or no activity was noted with oligopeptide substrates for trypsin-like, chymotrypsin-like, and elastase-like proteases. Human plasma alpha 1-protease inhibitor, human plasma alpha 2-protease macroglobulin, soybean and lima-bean trypsin inhibitors, bovine aprotinin, phosphoramidon, and chymostatin inhibited Q31 granzyme B. The inhibition by alpha 1-protease inhibitor was rapid enough to be of physiological significance.

Published

1991

70. The expression of the novel cytotoxic protein granzyme M by large granular lymphocytic leukaemias of both T-cell and NK-cell lineage: an unexpected finding with implications regarding the pathobiology of these disorders

Author

Curtis A. Hanson, Dragan Jevremovic, and William G. Morice

Subjects

Adult, Leukemia, T-Cell, T cell, chemical and pharmacologic phenomena, Poly(A)-Binding Proteins, Granzymes, Natural killer cell, medicine, Cytotoxic T cell, Humans, Cell Lineage, Aged, Aged, 80 and over, Innate immune system, biology, Hematology, Middle Aged, Acquired immune system, Natural killer T cell, Immunohistochemistry, Leukemia, Lymphoid, T-Cell Intracellular Antigen-1, Killer Cells, Natural, medicine.anatomical_structure, Granzyme, Immunology, biology.protein, Granzyme M, T-Lymphocytes, Cytotoxic

Abstract

Granzyme M (GrM) is a novel cytotoxic protein normally exclusively expressed by natural killer (NK)-cells and cytotoxic T-cells with innate immune function. As most T-cell granular lymphocytic leukaemias (T-LGL) are thought to be derived from the adaptive immune system it was predicted that T-LGL would be GrM negative. Contrary to this hypothesis, bone marrow biopsy immunohistochemistry revealed that GrM was frequently expressed in both T-LGL (16 / 18) and NK-LGL (6 / 9). These unexpected results suggest commonality between T- and NK-LGL, providing further support to the notion that T-LGL is a disorder of dysregulated, chronically stimulated, adaptive cytotoxic T-cells.

Published

2007

71. Granzyme M directly cleaves inhibitor of caspase-activated DNase (CAD) to unleash CAD leading to DNA fragmentation

Author

Hongxia Lu, Tongbiao Zhao, Honglian Zhang, Zusen Fan, Qixiang Zhang, Qiang Hou, and Lianfeng Wu

Subjects

DNA damage, Immunology, DNA, Single-Stranded, Apoptosis, DNA Fragmentation, Transfection, Granzymes, Caspase-activated DNase, Jurkat Cells, Immunology and Allergy, Humans, Fragmentation (cell biology), Enzyme Inhibitors, Polymerase, Cell Nucleus, Deoxyribonucleases, biology, Cell Death, Hydrolysis, Serine Endopeptidases, Apoptotic DNA fragmentation, Proteins, Molecular biology, Protein Transport, Granzyme, Caspases, biology.protein, DNA fragmentation, Granzyme M, Poly(ADP-ribose) Polymerases, Apoptosis Regulatory Proteins, Signal Transduction

Abstract

Granzyme (Gzm)M is constitutively highly expressed in NK cells that may play a critical role in NK cell-mediated cytolysis. However, the function of GzmM has been less defined. Just one report showed GzmM induces a caspase-independent death pathway. In this study, we demonstrate a protein transfection reagent Pro-Ject can efficiently transport GzmM into target cells. GzmM initiates caspase-dependent apoptosis with typical apoptotic nuclear morphology. GzmM induces DNA fragmentation, not DNA nicking. GzmM can directly degrade inhibitor of caspase-activated DNase to release the nuclease activity of caspase-activated DNase for damaging DNA. Furthermore, GzmM cleaves the DNA damage sensor enzyme poly(ADP-ribose) polymerase to prevent cellular DNA repair and force apoptosis.

Published

2006

72. KHYG-1, a model for the study of enhanced natural killer cell cytotoxicity

Author

Soad Fahim, Richard G. Miller, Mark J. Smyth, Armand Keating, Garnet Suck, Donald R. Branch, and Joanna Vergidis

Subjects

Cytotoxicity, Immunologic, Pore Forming Cytotoxic Proteins, Cancer Research, medicine.medical_treatment, Granzymes, Natural killer cell, Interleukin 21, Cancer immunotherapy, Cell Line, Tumor, Genetics, medicine, Humans, Receptors, Immunologic, Molecular Biology, Adaptor Proteins, Signal Transducing, Immunity, Cellular, Lymphokine-activated killer cell, Leukemia, Membrane Glycoproteins, biology, Natural Cytotoxicity Triggering Receptor 2, Perforin, Serine Endopeptidases, Models, Immunological, Membrane Proteins, Cell Biology, Hematology, NKG2D, Cell biology, Killer Cells, Natural, medicine.anatomical_structure, Granzyme, biology.protein, Granzyme M

Abstract

Objective. To compare the cytotoxicity of KHYG-1 with other natural killer (NK)/NK T-cell lines and identify molecules that may be associated with enhanced cytotoxicity, thereby eventually leading to improved NK cell-mediated cancer immunotherapy. Materials and Methods. NK/NK T-cell lines KHYG-1, NK-92, YT, and SNT-8 were compared with a novel flow cytometric cytotoxicity assay under different culture conditions. Transcription, expression, and phosphorylation studies were performed using polymerase chain reaction sequence-specific primers, reverse transcription polymerase chain reaction, immunoblotting, and flow cytometry. Results. KHYG-1 is a highly cytotoxic cell line, exceeding the cytolytic capacity of the other cell lines against K562. KHYG-1 is also highly cytotoxic against the leukemia cell lines EM2, EM3, and HL60. The novel activation receptor NKp44 and its adaptor, DAP12, NKG2D, and constitutively phosphorylated ERK2 may be associated with the enhanced cytotoxicity of KHYG-1. This cell line most likely mediates cytolysis by granzyme M (but not granzymes A and B) together with perforin, which is constitutively fully cleaved to the 60-kD form, in contrast to the other cell lines. Conclusion. KHYG-1 is a valuable model for the study of enhanced cytotoxicity by NK cells. In addition to the activation of NKp44, KHYG-1 may induce apoptosis of tumor cells by the newly described granzyme M/perforin pathway. Targeted modifications of effector molecules demonstrated in this model could generate NK cells with even greater killing ability that may be particularly attractive for clinical application. Moreover, our demonstration of greater cytotoxicity of KHYG-1 versus NK-92 cells, already in clinical trials, suggests a direct therapeutic role for KHYG-1.

Published

2005

73. Cleaving the oxidative repair protein Ape1 enhances cell death mediated by granzyme A

Author

Paul J. Beresford, Zusen Fan, Carl D. Novina, Dong Zhang, Yves Pommier, Zhan Xu, Judy Lieberman, and Akira Yoshida

Subjects

Pore Forming Cytotoxic Proteins, Programmed cell death, DNA Repair, DNA repair, Macromolecular Substances, Immunology, Carbon-Oxygen Lyases, Apoptosis, Granzymes, DNA-(Apurinic or Apyrimidinic Site) Lyase, Immunology and Allergy, Animals, Humans, AP site, Gene Silencing, Membrane Glycoproteins, biology, Base Sequence, Perforin, Endoplasmic reticulum, Serine Endopeptidases, DNA, Molecular biology, DNA-(apurinic or apyrimidinic site) lyase, Recombinant Proteins, Cell biology, Granzyme, Granzyme A, biology.protein, RNA Interference, Granzyme M, K562 Cells, Oxidation-Reduction, HeLa Cells, T-Lymphocytes, Cytotoxic

Abstract

The cytolytic T lymphocyte protease granzyme A (GzmA) initiates a caspase-independent cell death pathway. Here we report that the rate-limiting enzyme of DNA base excision repair, apurinic endonuclease-1 (Ape1), which is also known as redox factor-1 (Ref-1), binds to GzmA and is contained in the SET complex, a macromolecular complex of 270–420 kDa that is associated with the endoplasmic reticulum and is targeted by GzmA during cell-mediated death. GzmA cleaves Ape1 after Lys31 and destroys its known oxidative repair functions. In so doing, GzmA may block cellular repair and force apoptosis. In support of this, cells with silenced Ape1 expression are more sensitive, whereas cells overexpressing noncleavable Ape1 are more resistant, to GzmA-mediated death.

Published

2002

74. Lymphocyte-mediated cytotoxicity

Author

Timothy J. Ley and John H. Russell

Subjects

Cytotoxicity, Immunologic, Pore Forming Cytotoxic Proteins, Lymphocyte, Fas-Associated Death Domain Protein, Immunology, Graft vs Leukemia Effect, Fas ligand, Exocytosis, Granzymes, Autoimmune Diseases, Graft vs Host Reaction, Mice, medicine, Immunology and Allergy, Cytotoxic T cell, Animals, Humans, Lymphocytes, Adaptor Proteins, Signal Transducing, Membrane Glycoproteins, biology, Perforin, Serine Endopeptidases, Cell biology, medicine.anatomical_structure, Granzyme, Apoptosis, Virus Diseases, biology.protein, Granzyme K, Granzyme M, Carrier Proteins, Signal Transduction

Abstract

Virtually all of the measurable cell-mediated cytotoxicity delivered by cytotoxic T lymphocytes and natural killer cells comes from either the granule exocytosis pathway or the Fas pathway. The granule exocytosis pathway utilizes perforin to traffic the granzymes to appropriate locations in target cells, where they cleave critical substrates that initiate DNA fragmentation and apoptosis; granzymes A and B induce death via alternate, nonoverlapping pathways. The Fas/FasL system is responsible for activation-induced cell death but also plays an important role in lymphocyte-mediated killing under certain circumstances. The interplay between these two cytotoxic systems provides opportunities for therapeutic interventions to control autoimmune diseases and graft vs. host disease, but oversuppression of these pathways may also lead to increased viral susceptibility and/or decreased tumor cell killing.

Published

2002

75. Cloning and characterization of cDNA clones encoding CD9 from Atlantic salmon (Salmo salar) and rainbow trout (Oncorhynchus mykiss)

Author

Niels C. Bols, Julie Gauley, Kazuhiro Fujiki, and Brian Dixon

Subjects

clone (Java method), endocrine system, DNA, Complementary, Sequence analysis, animal diseases, Immunology, Molecular Sequence Data, Salmo salar, Biology, Tetraspanin 29, Antigens, CD, Complementary DNA, Genetics, Animals, Tissue Distribution, Amino Acid Sequence, RNA, Messenger, Salmo, Cloning, Molecular, Phylogeny, Membrane Glycoproteins, Base Sequence, biology.organism_classification, Molecular biology, Trout, Suppression subtractive hybridization, Oncorhynchus mykiss, embryonic structures, Rainbow trout, Granzyme M, Sequence Alignment

Abstract

In comparison to mammals, relatively few of the molecules involved in teleost immune responses have been isolated and characterized. A rapid method of isolating molecules important for immune function is subtractive hybridization. One such experiment using infectious hematopoietic necrosis virus-infected Atlantic salmon produced several cDNA clones with similarity to mammalian immune-specific genes, including granzyme M (accession no. AF434669) and CD9. After cloning the rainbow trout version of CD9, sequence analysis showed that both salmonid sequences contained many features of the tetraspanin receptor family to which CD9 belongs. Phylogenetic analysis revealed a close association of the trout and salmon sequences to known CD9 and CD81 receptors. Southern blotting demonstrated that the rainbow trout gene is single copy. Reverse transcriptase PCR showed strong expression of this clone in many tissues, but liver expression was very low – an observation consistent with the clone being a CD9, not a CD81, equivalent. The evidence suggests that the sequences reported here are bona fide teleost CD9 homologues and we are currently producing recombinant proteins and polyclonal antisera for use in functional studies.

Published

2002

76. NK cell intrinsic regulation of MIP-1α by granzyme M

Author

Joseph A. Trapani, Richard A. Strugnell, Nancy Wang, Colin M. House, Phillip I. Bird, Heloise Halse, Mark J. Smyth, Sally V. Watt, Nikola Baschuk, and Daniel M. Andrews

Subjects

Cancer Research, Programmed cell death, Time Factors, MIP-1α, T cell, Immunology, NK cells, Granzymes, Microbiology, Mice, Cellular and Molecular Neuroscience, Immune system, medicine, Animals, Humans, Listeriosis, Secretion, Granzyme M, Cells, Cultured, Chemokine CCL3, Mice, Knockout, Innate immune system, biology, Interleukins, Cell Biology, Listeria monocytogenes, Coculture Techniques, Immunity, Innate, 3. Good health, Cell biology, Killer Cells, Natural, Chemotaxis, Leukocyte, Disease Models, Animal, medicine.anatomical_structure, Granzyme, biology.protein, Original Article, Intracellular, Listeria monocytogenes infection

Abstract

Granzymes are generally recognized for their capacity to induce various pathways of perforin-dependent target cell death. Within this serine protease family, Granzyme M (GrzM) is unique owing to its preferential expression in innate effectors such as natural killer (NK) cells. During Listeria monocytogenes infection, we observed markedly reduced secretion of macrophage inflammatory protein-1 alpha (MIP-1α) in livers of GrzM-deficient mice, which resulted in significantly impaired NK cell recruitment. Direct stimulation with IL-12 and IL-15 demonstrated that GrzM was required for maximal secretion of active MIP-1α. This effect was not due to reduced protein induction but resulted from heightened intracellular accumulation of MIP-1α, with reduced release. These results demonstrate that GrzM is a critical mediator of innate immunity that can regulate chemotactic networks and has an important role in the initiation of immune responses and pathogen control.

Published

2014

77. The restricted expression of granzyme M in human lymphocytes

Author

T J, Sayers, A D, Brooks, J M, Ward, T, Hoshino, W E, Bere, G W, Wiegand, J M, Kelly, M J, Smyth, and J M, Kelley

Subjects

Pore Forming Cytotoxic Proteins, CD3 Complex, T cell, CD3, T-Lymphocytes, Immunology, Blotting, Western, Cell Separation, Jurkat cells, Granzymes, Cell Line, Jurkat Cells, medicine, Immunology and Allergy, Cytotoxic T cell, Humans, Membrane Glycoproteins, biology, Perforin, Serine Endopeptidases, Receptors, Antigen, T-Cell, gamma-delta, U937 Cells, Flow Cytometry, Molecular biology, CD56 Antigen, Lymphocyte Subsets, Clone Cells, Killer Cells, Natural, medicine.anatomical_structure, Granzyme, biology.protein, Granzyme M, CD8

Abstract

We have analyzed the expression of human granzyme M (Gzm M) in various human leukocyte subsets using the specific mAb 4H10. Using FACS and Western blotting analysis we compared the expression of Gzm M with that of other granzymes (Gzm A and Gzm B) and the lytic protein perforin. Human Gzm M was constitutively highly expressed in NK cells as was perforin and Gzm A. Surprisingly, freshly isolated NK cells had very low (sometimes undetectable) levels of Gzm B. In contrast to Gzm B and perforin, Gzm M was not detected in highly purified CD4+ and CD8+ T cells either constitutively or after short term activation in vitro. However, low levels of Gzm M were observed in some T cell clones on prolonged passage in vitro. Gzm M was not detected in highly purified neutrophils, monocytes, or tumor cells of the myelomonocytic lineage. Examination of minor T cell subsets from human peripheral blood showed detectable Gzm M in CD3+, CD56+ T cells and γδ T cells. A histological staining procedure was developed that demonstrated a granular staining pattern for Gzm M and a cellular distribution similar to that observed by Western blotting. These data indicate that the expression of Gzm M does not always correlate with the lytic activity of cytotoxic cells. However, expression of Gzm M in NK cells, CD3+, CD56+ T cells, and γδ T cells suggests that this enzyme may play some role in innate immune responses.

Published

2001

78. DFF45/ICAD can be directly processed by granzyme B during the induction of apoptosis

Author

Ming Xu, Xiaodong Wang, Timothy J. Ley, Dori A. Thomas, and Chunying Du

Subjects

Cytotoxicity, Immunologic, ICAD, Immunology, Caspase 3, Apoptosis, DNA Fragmentation, Granzymes, GZMB, Cell Line, Substrate Specificity, 03 medical and health sciences, Mice, 0302 clinical medicine, Immunology and Allergy, Animals, Enzyme Inhibitors, Killer Cells, Lymphokine-Activated, Caspase, 030304 developmental biology, 0303 health sciences, Deoxyribonucleases, biology, Serine Endopeptidases, Proteins, Fibroblasts, Embryo, Mammalian, Immunity, Innate, Recombinant Proteins, Cell biology, Granzyme B, Infectious Diseases, Granzyme, 030220 oncology & carcinogenesis, Caspases, biology.protein, Granzyme M, Apoptosis Regulatory Proteins, Protein Processing, Post-Translational, T-Lymphocytes, Cytotoxic

Abstract

Granzyme B (GzmB) is a component of cytotoxic lymphocyte granules that can rapidly initiate apoptosis in target cells. While several procaspases are cleaved and activated by GzmB, the absolute requirement of caspase activation for GzmB-induced apoptosis is controversial. In this report, we demonstrate that GzmB can initiate apoptosis in the absence of caspase-3 activity by directly cleaving DFF45/ICAD to liberate activated DFF40/CAD. DFF45/ICAD cleavage occurs less efficiently in cells that lack caspase-3 activity, suggesting that the caspases normally amplify the GzmB death signal. DFF45/ICAD-deficient mouse embryo fibroblasts are partially resistant to GzmB-induced death, demonstrating the biological importance of DFF45/ICAD for GzmB-mediated apoptosis.

Published

2000

79. Granzymes are the essential downstream effector molecules for the control of primary virus infections by cytolytic leukocytes

Author

Thao Tran, Ron Tha Hla, Seow Chin, Crisan Museteanu, Thomas Stehle, Arno Müllbacher, Markus M. Simon, and Paul Waring

Subjects

Cytotoxicity, Immunologic, Male, Pore Forming Cytotoxic Proteins, Ectromelia virus, chemical and pharmacologic phenomena, Granzymes, GZMB, Cell Line, Mice, Chromium Isotopes, Leukocytes, Animals, Humans, Ectromelia, Infectious, Mice, Knockout, Multidisciplinary, Membrane Glycoproteins, biology, Cell Death, Effector, Perforin, Serine Endopeptidases, hemic and immune systems, Biological Sciences, biology.organism_classification, Virology, Cell biology, Granzyme B, Mice, Inbred C57BL, Granzyme, Liver, biology.protein, Granzyme A, Female, Granzyme M, Spleen, T-Lymphocytes, Cytotoxic

Abstract

Analysis of perforin-deficient mice has identified the cytolytic pathway and perforin as the preeminent effector molecule in T cell-mediated control of virus infections. In this paper, we show that mice lacking both granzyme A (gzmA) and granzyme B (gzmB), which are, beside perforin, key constituents of cytolytic vesicles, are as incapable as are perforin-deficient mice of controlling primary infections by the natural mouse pathogen ectromelia, a poxvirus. Death of gzmA×gzmB double knockout mice occurred in a dose-dependent manner, despite the expression of functionally active perforin and the absence of an intrinsic defect to generate splenic cytolytic T cells. These results establish that both gzmA and gzmB are indispensable effector molecules acting in concert with perforin in granule exocytosis-mediated host defense against natural viral pathogens.

Published

1999

80. The human cytotoxic T cell granule serine protease granzyme H has chymotrypsin-like (chymase) activity and is taken up into cytoplasmic vesicles reminiscent of granzyme B-containing endosomes

Author

Joseph A. Trapani, Chih-Min Kam, Kirsten M Edwards, and James C. Powers

Subjects

Endosomes, Spodoptera, Cytoplasmic Granules, Transfection, Biochemistry, Granzymes, Cell Line, Substrate Specificity, Jurkat Cells, Chymases, medicine, Tumor Cells, Cultured, Cytotoxic T cell, Animals, Chymotrypsin, Humans, Protease Inhibitors, Amino Acid Sequence, Molecular Biology, Serine protease, biology, Serine Endopeptidases, Cell Biology, Trypsin, Molecular biology, Recombinant Proteins, Granzyme B, Granzyme, biology.protein, Cytokine secretion, Granzyme M, Oligopeptides, Granzyme H, medicine.drug, T-Lymphocytes, Cytotoxic

Abstract

Serine proteases (granzymes) contained within the cytoplasmic granules of cytotoxic T cells and natural killer cells play a variety of roles including the induction of target cell apoptosis, breakdown of extracellular matrix proteins and induction of cytokine secretion by bystander leukocytes. Different granzymes display proteolytic specificities that mimic the activities of trypsin or chymotrypsin, or may cleave substrates at acidic ("Asp-ase") or at long unbranched amino acids such as Met ("Met-ase"). Here, we report that recombinant granzyme H has chymotrypsin-like (chymase) activity, the first report of a human granzyme with this proteolytic specificity. Recombinant 32-kDa granzyme H expressed in the baculovirus vector pBacPAK8 was secreted from Sf21 cells and recovered by Ni-affinity chromatography, using a poly-His tag encoded at the predicted carboxyl terminus of full-length granzyme H cDNA. The granzyme H efficiently cleaved Suc-Phe-Leu-Phe-SBzl (v = 185 nM/s at [S] = 0.217 mM) and also hydrolyzed Boc-Ala-Ala-X-SBzl (X = Phe, Tyr, Met, Nle, or Nva) with slower rates but had little tryptase or Asp-ase activity. Enzymatic activity was inhibited completely by 0.1 mM 3,4-dichloroisocoumarin and 84% by 1.0 mM phenylmethylsulfonyl fluoride. Fluoresceinated granzyme H was internalized in a temperature-dependent manner by Jurkat cells into endosome-like vesicles, suggesting that it can bind to cell surface receptors similar to those that bind granzyme B. This suggests a hitherto unsuspected intracellular function for granzyme H.

Published

1999

81. Granzyme A loading induces rapid cytolysis and a novel form of DNA damage independently of caspase activation

Author

Zhinan Xia, Judy Lieberman, Arnold H. Greenberg, and Paul J. Beresford

Subjects

Cytotoxicity, Immunologic, DNA damage, Poly ADP ribose polymerase, Immunology, Gene Expression, Apoptosis, Granzymes, Tumor Cells, Cultured, Immunology and Allergy, Animals, Humans, Caspase, biology, Serine Endopeptidases, Esterases, Molecular biology, Genes, bcl-2, Enzyme Activation, Cytolysis, Infectious Diseases, Perforin, Granzyme, Caspases, biology.protein, Granzyme K, Granzyme M, K562 Cells, DNA Damage, T-Lymphocytes, Cytotoxic

Abstract

Cytotoxic lymphocytes trigger apoptosis by releasing perforin and granzymes (Grn). GrnB activates the caspase apoptotic pathway, but little is known about GrnA-induced cell death. Perforin was used to load recombinant GrnA and GrnB and enzymatically inactive variants into target cells. GrnA induces single-strand DNA breaks that can be labeled with Klenow polymerase and visualized on alkaline gels. GrnA-induced DNA damage but not cytolysis requires GrnA proteolysis. GrnA-induced membrane perturbation, nuclear condensation, and DNA damage are unimpaired by caspase blockade. GrnA fails to induce cleavage of caspase-3, lamin B, rho-GTPase, or PARP. GrnA-induced cytotoxicity and cleavage of PHAP II, a previously identified GrnA substrate, are unimpaired in Jurkat cells that overexpress bcl-2. Therefore, GrnA activates a novel apoptotic pathway.

Published

1999

82. A cytosolic granzyme B inhibitor related to the viral apoptotic regulator cytokine response modifier A is present in cytotoxic lymphocytes

Author

Joseph A. Trapani, Phillip I. Bird, Paul Bernard Coughlin, Lisa McDonald, Tanya A. De Jong, Catherina H. Bird, Vivien R. Sutton, and Jiuru Sun

Subjects

Cytotoxicity, Immunologic, Transcription, Genetic, Molecular Sequence Data, Serpin, Biochemistry, Peripheral blood mononuclear cell, Granzymes, Cell Line, Viral Proteins, Bone Marrow, Cytotoxic T cell, Humans, Amino Acid Sequence, Molecular Biology, Serpins, DNA Primers, Binding Sites, biology, Base Sequence, Sequence Homology, Amino Acid, Serine Endopeptidases, Degranulation, Cell Biology, Molecular biology, Recombinant Proteins, Granzyme B, Granzyme, Cell culture, biology.protein, Granzyme M, T-Lymphocytes, Cytotoxic

Abstract

Using a polymerase chain reaction strategy we identified a serine proteinase inhibitor (serpin) in human bone marrow that is related to the cellular serpin proteinase inhibitor 6 (PI-6) and the viral serpin cytokine response modifier A (CrmA). This serpin, proteinase inhibitor 9 (PI-9), has an unusual reactive center P1(Glu)-P1'(Cys), which suggests that it inhibits serine proteinases that cleave after acidic residues. The only known serine proteinase with this specificity is granzyme B, a granule cytotoxin produced by cytotoxic lymphocytes. To test the interaction of PI-9 with granzyme B we prepared recombinant hexa-histidine tagged PI-9 in a yeast expression system. Addition of the recombinant protein to native granzyme B resulted in an SDS-resistant complex typical of serpin-serine proteinase interactions. Further analysis showed that complex formation followed bimolecular kinetics with a second order rate constant of 1.7 +/- 0.3 x 10(6) M-1 s-1, which is in the range for a physiologically significant serpin-proteinase interaction. Recombinant PI-9 also completely abrogated granzyme B and perforin-mediated cytotoxicity in vitro. Examination of PI-9 mRNA distribution demonstrated that it is expressed in immune tissue, primarily in lymphocytes. The highest levels of PI-9 mRNA and protein were observed in natural killer cell leukemia cell lines and in interleukin-2 stimulated peripheral blood mononuclear cells, which also produce granzyme B. Like PI-6, PI-9 was shown to be a cytosolic protein that is not secreted. Fractionation of natural killer cells and stimulated peripheral blood mononuclear cells demonstrated that PI-9 is in a separate subcellular compartment to granzyme B. These results suggest that PI-9 serves to inactivate misdirected granzyme B following cytotoxic cell degranulation. This may explain why cytotoxic cells are not damaged by their own granzyme B during destruction of abnormal cells.

Published

1996

83. Expression of recombinant human Met-ase-1: a NK cell-specific granzyme

Author

Mark J. Smyth, K. Y. T. Thia, Michael D O'Connor, Pangayachelvi Ganesvaran, Janice M. Kelly, and Joseph A. Trapani

Subjects

Proteases, animal structures, medicine.medical_treatment, Molecular Sequence Data, Biophysics, Biochemistry, Cell Line, Substrate Specificity, Serine, Methionine, Chlorocebus aethiops, medicine, Cytotoxic T cell, Animals, Humans, Molecular Biology, DNA Primers, Serine protease, Protease, COS cells, biology, Base Sequence, Serine Endopeptidases, Antibodies, Monoclonal, Cell Biology, Molecular biology, Recombinant Proteins, Killer Cells, Natural, Granzyme, biology.protein, Granzyme M, Protein Processing, Post-Translational

Abstract

Human Met-ase-1 is a member of a family of cytotoxic lymphocyte serine proteases (granzymes), but is expressed specifically in CD3- large granular lymphocytes with natural killer cell activity. We have devised a polymerase chain reaction strategy to delete the predicted hexapropeptide of human Met-ase-1 (Ser-6 to Gln-1), to enable its expression and activation in mammalian COS cells. In addition, using peptide immunization we have derived a unique and specific monoclonal antibody detecting human Met-ase-1. Western blot analysis and protease assays of transfected COS cell lysates against a panel of thiobenzyl ester substrates formally demonstrated that the human Met-ase-1 gene encodes a serine proteinase that specifically hydrolyzes substrates containing a methionine (Met-) side chain at P1. The expression of active human Met-ase-1 and the generation of a specific anti-human Met-ase-1 monoclonal antibody will now enable a detailed structure/function analysis of key amino acids that confer this unusual serine protease specificity.

Published

1995

84. Granzyme A-deficient mice retain potent cell-mediated cytotoxicity

Author

Marinus C. Lamers, Klaus Ebnet, Lehmann-Grube F, Arno Mullbacher, Hausmann M, Manfred Kopf, and Markus M. Simon

Subjects

Cytotoxicity, Immunologic, Molecular Sequence Data, Gene Expression, Apoptosis, Lymphocytic Choriomeningitis, Lymphocyte Activation, Polymerase Chain Reaction, General Biochemistry, Genetics and Molecular Biology, Granzymes, Interleukin 21, Mice, Tumor Cells, Cultured, Cytotoxic T cell, Animals, Lymphocytic choriomeningitis virus, Listeriosis, Amino Acid Sequence, RNA, Messenger, Molecular Biology, DNA Primers, General Immunology and Microbiology, biology, Base Sequence, General Neuroscience, Serine Endopeptidases, Exons, Natural killer T cell, Flow Cytometry, Molecular biology, Listeria monocytogenes, Mice, Mutant Strains, Hematopoiesis, Killer Cells, Natural, Mutagenesis, Insertional, Granzyme, Perforin, Granzyme A, biology.protein, DNA fragmentation, Granzyme M, Research Article, T-Lymphocytes, Cytotoxic

Abstract

Granzyme A, a granule-associated serine proteinase of activated cytotoxic T cells and natural killer cells, has been reported to play a critical role in DNA fragmentation of target cells. To address the question of the biological role of granzyme A, we have now generated a granzyme A-deficient mouse mutant by homologous recombination. Western blot analysis, enzyme assays and reverse transcription-PCR confirmed the absence of granzyme A in activated T cells. In addition, deletion of granzyme A does not alter the expression patterns of other granule components, such as granzymes B-G and perforin. Granzyme A-deficient mice are healthy and show normal hematopoietic development. Most notably, their in vitro- and ex vivo-derived cytotoxic T cells and natural killer cells are indistinguishable from those of normal mice in causing membrane disruption, apoptosis and DNA fragmentation in target cells. Furthermore, granzyme A-deficient mice readily recover from both lymphocytic choriomeningitis virus and Listeria monocytogenes infections and eradicate syngeneic tumors with kinetics similar to the wild-type strain. These results demonstrate that granzyme A does not play a primary role in cell-mediated cytotoxicity, as has been assumed previously.

Published

1995

85. Natural killer and lymphokine-activated killer cells require granzyme B for the rapid induction of apoptosis in susceptible target cells

Author

John H. Russell, Jonathan W. Heusel, Debra M. MacIvor, Sujan Shresta, and Timothy J. Ley

Subjects

Cytotoxicity, Immunologic, Molecular Sequence Data, chemical and pharmacologic phenomena, Apoptosis, Granzymes, Interleukin 21, Mice, NK-92, Animals, Amino Acid Sequence, Killer Cells, Lymphokine-Activated, Cells, Cultured, Multidisciplinary, Lymphokine-activated killer cell, biology, Serine Endopeptidases, hemic and immune systems, Natural killer T cell, Cell biology, Granzyme B, Killer Cells, Natural, Granzyme, Immunology, biology.protein, Interleukin 12, Granzyme M, Research Article

Abstract

Granzyme (Gzm) B-deficient mice obtained by gene targeting were used to assess the role of Gzm B in the mechanisms used by natural killer (NK) and lymphokine-activated killer (LAK) cells to destroy target cells. Gzm B-/- NK cells, LAK cells, and cytotoxic T lymphocytes (CTL) all are defective in their ability to rapidly induce DNA fragmentation/apoptosis in susceptible target cells. This defect can be partially corrected with long incubation times of effector and target cells. Moreover, Gzm B-/- NK cells (but not CTL or LAK cells) exhibit a defect in 51Cr release from susceptible target cells. This 51Cr release defect in Gzm B-deficient NK cells is also not overcome by prolonged incubation times or high effector-to-target cell ratios. We conclude that Gzm B plays a critical and nonredundant role in the rapid induction of DNA fragmentation/apoptosis by NK cells, LAK cells, and CTL. Gzm B may have an additional role in NK cells (but not in CTL or LAK cells) for mediating 51Cr release.

Published

1995

86. Granzyme B is inhibited by the cowpox virus serpin cytokine response modifier A

Author

R. Chris Bleackley, David J. Pickup, Guy S. Salvesen, Antonio Caputo, and Long T. Quan

Subjects

viruses, Cowpox, Serpin, In Vitro Techniques, Biochemistry, Binding, Competitive, Virus, Granzymes, Viral Proteins, medicine, Cytotoxic T cell, Cowpox virus, Molecular Biology, Serpins, biology, Caspase 1, Serine Endopeptidases, Cell Biology, medicine.disease, Virology, Molecular biology, Recombinant Proteins, Granzyme B, Cysteine Endopeptidases, Kinetics, Granzyme, biology.protein, Granzyme M, Protein Binding

Abstract

The ability of cytolytic cells to cause apoptosis in target cells is in part due to the action of the serine proteinase granzyme B. We demonstrate that granzyme B is inhibited, with an association rate constant of 2.9 x 10(5) M-1 s-1, by the cowpox viral serpin cytokine response modifier A (CrmA). Previously we have shown CrmA to be an inhibitor of the cysteine proteinase interleukin-1 beta-converting enzyme (ICE). Thus the mechanism of CrmA involves the unusual ability to efficiently inhibit proteinases from two distinct catalytic classes, in this case serine and cysteine proteinases. Granzyme B and ICE are both used to combat viral infection, and we propose that cowpox virus uses CrmA to evade the contribution of these two proteinases. Thus, through CrmA, the virus may influence two of the pathways normally used to kill virus-infected cells: acting on endogenous proteinases such as ICE and on exogenous proteinases delivered by cytotoxic lymphocytes to infected cells.

Published

1995

87. Hematologic malignancies of cytotoxic cells: Introduction

Author

Thomas P. Loughran

Subjects

medicine.medical_specialty, Hematology, business.industry, Pure red cell aplasia, chemical and pharmacologic phenomena, medicine.disease, Lymphoma, Leukemia, medicine.anatomical_structure, hemic and lymphatic diseases, Internal medicine, Immunology, medicine, Cytotoxic T cell, Granzyme M, Aplastic anemia, business, B cell

Abstract

THIS ISSUE OF Seminars in Hematology is devoted to leukemias and lymphomas of killer cell origin. These hematologic malignancies can be derived from either cytotoxic T lymphocytes (CTL) or natural killer (NK) cells. These lymphoid malignancies are much less common than B cell lymphoproliferative disease. For example, it is estimated that approximately 10% of non-Hodgkin’s lymphomas fall into the category of either T-cell or NK cell disorders. The relative infrequency of such patients, varied terminology, recent recognition of most of these entities, and perhaps most importantly lack of an easily determined marker of clonality for the NK cell neoplasms has led to a considerable degree of confusion in this area of hematologic malignancies. Therefore one goal of the current issue is to summarize diagnostic criteria and clinicopathologic features of hematologic malignancies originating from CTL or NK cells. Elaine Jaffe and colleagues review the current classification of CTL and NK cell lymphomas based on the World Health Organization (WHO) system. Jaffe et al emphasize that the WHO classification is based on a multiparameter approach. In particular, they highlight the important role of the clinical presentation in classification as these malignancies show great morphologic diversity. In addition to providing a good overview of many of the entities discussed in further detail in subsequent chapters, other lesions such as the enteropathy type of T-cell lymphoma and subcutaneous panniculitis-like T-cell lymphomas are discussed in detail. Particularly valuable for discrimination of the differential diagnostic possibilities among this group of hematologic malignancies are the immunophenotypic properties. Jaffe’s group recently used granzyme M staining to distinguish NK lymphomas, T-cell lymphomas, and enteropathyassociated T-cell lymphomas from other lymphomas arising from cytotoxic precursors. The five chapters that follow focus on various aspects of large granular lymphocyte (LGL) leukemia. Clonal cytogenetic abnormalities and tissue invasion of marrow, spleen, and liver characterized the first description of LGL leukemia. Subsequently it was recognized that LGL leukemia could be derived from either T cells or NK cells, leading to the designations of T-LGL and NK-LGL leukemia, respectively. Lamy and Loughran provide an update on the clinical features of LGL leukemia. A fascinating aspect of LGL leukemia is the strong clinical association with autoimmune diseases such as rheumatoid arthritis. There may be a common pathogenesis and indeed LGL leukemia and Felty’s syndrome may be the same disease. There is also growing recognition that LGL leukemia may overlap clinically with disease states characterized by failure of hematopoiesis. The Mayo Clinic experience describing the association of LGL leukemia with either aplastic anemia or pure red cell aplasia is detailed by Go et al. Although not widely recognized, the most common identifiable

Published

2003

88. The human Met-ase gene (GZMM): structure, sequence, and close physical linkage to the serine protease gene cluster on 19p13.3

Author

Dieter E. Jenne, Peter Lichter, Hartmut Wekerle, Thomas M. Fink, Michael Zimmer, Daniel Pilat, and Brigitte Obermaier-Skrobanek

Subjects

animal structures, Genetic Linkage, Molecular Sequence Data, Restriction Mapping, Biology, Homology (biology), Exon, Mice, Gene mapping, Complementary DNA, Gene cluster, Genetics, Animals, Humans, Amino Acid Sequence, Cloning, Molecular, Gene, In Situ Hybridization, Fluorescence, Base Sequence, Serine Endopeptidases, DNA, Exons, Cosmids, Molecular biology, Introns, Rats, Killer Cells, Natural, Multigene Family, Cosmid, Granzyme M, Chromosomes, Human, Pair 19

Abstract

Cosmid clones containing the genes for the human and murine natural killer cell serine protease Met-ase (gene symbol GZMM; granzyme M) were identified by screening human and murine cosmid libraries with rat Met-ase (RNK-Met-1) cDNA. The human gene has a size of 7.5 kb and an exon-intron structure identical to that of serine protease genes located on human chromosomes 5q11-q12, 14q11.2, and 19p13.3 that are expressed by lymphocytes, mast cells, or myelomonocyte precursors. Using cosmid DNA as a probe for fluorescence in situ hybridization, we identified the chromosomal position of human Met-ase as 19p13.3. Interphase studies with two differentially labeled probes for Met-ase and the azurocidin (AZU1), proteinase 3 (PRTN3), and neutrophil elastase (ELA2) gene cluster revealed that the distance of Met-ase from this gene cluster is in the range of 200 to 500 kb. Using differentially labeled mouse cosmid probes, we also mapped the murine gene for Met-ase to chromosomal band 10C, close to the gene for lamin B2. Thus, the Met-ase, AZU1, PRTN3, and ELA2 genes fall into an established region of homology between mouse chromosomal band 10C and human 19p13.3.

Published

1994

89. Lymphocyte-mediated cytotoxicity: two pathways and multiple effector molecules

Author

Pierre A. Henkart

Subjects

Pore Forming Cytotoxic Proteins, Membrane Glycoproteins, Cytotoxins, Perforin, Lymphocyte, Immunology, Biology, Cell biology, CTL, Infectious Diseases, medicine.anatomical_structure, In vivo, Knockout mouse, medicine, biology.protein, Immunology and Allergy, Cytotoxic T cell, Animals, Humans, Granzyme M, CD8, Gene Deletion, T-Lymphocytes, Cytotoxic

Abstract

Pierre A. Henkart Experimental Immunology Branch National Cancer Institute National Institutes of Health Bethesda, Maryland 20892 Important progress has been made over the last several years in our understanding of the mechanism of lympho- cyte cytotoxicity. Experiments published in recent months have built on this to provide definitive answers to basic questions, as I will review here. The Granule Exocytosis Pathway: Effects of CytolysinlPerforin Deletion Until recently, the granule exocytosis pathway had been the only molecularly defined cytotoxicity pathway, and is diagrammed in the right portion of Figure 1. This basic process and the considerable evidence supporting it have been reviewed elsewhere (Podack et al., 1991; Henkart et al., 1994). The functional cytotoxic mediator delivered by the killer lymphocyte in this pathway has traditionally been thought to be the membrane-damaging agent cytolysin or perforin. This interesting protein is found uniquely in cytotoxic T lymphocyte (CTL) granules, and is a potent lytic agent after its release into the physiological ionic environment. The pores it forms in the target cell have been shown to allow passage of large proteins, as well as ions, and it was proposed that this damage was lethal to the target cell. Although avery considerable body of evidence had been developed to support the granule exocytosis model, per- sistent questions arose regarding its in vivo relevance (Berke, 1991). The issue came down to whether the rela- tively small level of granule components in in vivo CTL, detectable in some studies but not others, could account for the cytotoxic function, and no definitive answer emerged. The recent development of knockout mice in which the gene for cytolysinlperforin is disrupted either in the germ- line or in B and T lymphocytes selectively has allowed these in vivo questions to be addressed in a particularly clear way. The report of Kagi et al. (1994a), one of four labs that have developed such mice, is a beautiful example of the success of the gene disruption appproach, since problems with indirect effects of the knockout and redun- dant molecular pathways seem not to be significant. Thus, CD8’ T cells were found in normal levels in lymphoid or- gansof the knockout mice, and became activated normally in response to LCMV infection. However, specific in vitro cytotoxic activity was negligible when spleen cells from virus- infected knockout mice were compared with infected con- trol mice. Alloreactive CTL originating from primary in vitro cultures as well as in vivo immunizations likewise were severely crippled in terms of their ability to lyse the appro- priate allospecific fibroblasts, and to a considerable ex- tent, allogeneic tumor cells as well. NK activity also ap

Published

1994

90. Cytotoxicity with target DNA breakdown by rat basophilic leukemia cells expressing both cytolysin and granzyme A

Author

Lishan Su, John W. Shiver, and Pierre A. Henkart

Subjects

Cytotoxicity, Immunologic, Pore Forming Cytotoxic Proteins, animal structures, viruses, Apoptosis, Transfection, General Biochemistry, Genetics and Molecular Biology, Exocytosis, Granzymes, Tumor Cells, Cultured, Cytotoxic T cell, Animals, Cytotoxicity, Membrane Glycoproteins, biology, Perforin, Serine Endopeptidases, Degranulation, Membrane Proteins, hemic and immune systems, Molecular biology, Cell biology, Basophils, Rats, Granzyme, biology.protein, Granzyme A, bacteria, lipids (amino acids, peptides, and proteins), Cytolysin, Granzyme M, DNA Damage

Abstract

The noncytotoxic rat mast cell tumor line RBL was transfected with genes for the cytotoxic lymphocyte granule proteins cytolysin (perforin) and granzyme A, giving transfectants with mRNA and protein expression levels comparable with cloned cytotoxic T lymphocytes. Both RBL-cytolysin and RBL-cytolysin-granzyme A transfectants showed extremely potent killing of red cell targets and lysed 20%–60% of EL4 lymphoma targets at an effector-to-target ratio of 30. RBL transfectants expressing only granzyme A were not cytotoxic. Significant EL4 DNA breakdown accompanying lysis was observed only with RBL that was transfected with both cytolysin and granzyme A. These results support the granule-exocytosis model for lymphocyte cytotoxicity and show that effector granzyme A plays a role in target cell DNA breakdown.

Published

1992

91. The orphan granzymes of humans and mice

Author

Hillary Johnson, Andrew J. Bredemeyer, William Grossman, Timothy J. Ley, Paula A. Revell, and Zhi Hong Lu

Subjects

Pore Forming Cytotoxic Proteins, Immunology, Down-Regulation, Granzymes, Mice, Immune system, Animals, Humans, Immunology and Allergy, Phylogeny, Mice, Knockout, Membrane Glycoproteins, Cell Death, biology, Perforin, Serine Endopeptidases, CTL, Granzyme, Multigene Family, biology.protein, Tumor necrosis factor alpha, Granzyme K, Granzyme M, Granzyme H

Abstract

The granzyme/perforin pathway is a central pathway for lymphocyte-mediated killing in both the innate and adaptive immune systems. This pathway is important in a variety of host defenses, including viral clearance and tumor cell killing, and its dysregulation results in several human and rodent diseases. To date, the majority of reports in this field have concentrated on the functions of granzymes A and B. Recent reports, however, suggest that the non-A/non-B 'orphan' granzymes found in both humans and mice are potentially significant. Although the functions of these orphan granzymes have yet to be fully established, initial data suggests their importance in both immune and nonimmune cells.

Published

2003

92. Granzyme M, a profiler of innate immune lymphocytes?

Author

Thomas J. Sayers

Subjects

Innate immune system, Cellular origin, Immunology, Proteome, Malignant cells, Tumor cells, Cell Biology, Hematology, Biology, Granzyme M, Biochemistry, Protein expression, Cell biology

Abstract

There is currently a major effort underway to identify the protein expression patterns (proteome) of various tumor cells. Indeed, characteristic patterns of protein expression may help determine the specific cellular origin of the malignant cell. In this issue, Krenacs and colleagues (page [3590][1

Published

2003

93. Granzyme M expressed by tumor cells promotes chemoresistance and EMT in vitro and metastasis in vivo associated with STAT3 activation.

Author

Wang H, Sun Q, Wu Y, Wang L, Zhou C, Ma W, Zhang Y, Wang S, and Zhang S

Subjects

Animals, Cell Line, Tumor, Epithelial-Mesenchymal Transition, Granzymes biosynthesis, HT29 Cells, Hep G2 Cells, Humans, Male, Mice, Mice, Inbred C57BL, Mice, Inbred NOD, Mice, SCID, Neoplasm Metastasis, STAT3 Transcription Factor biosynthesis, Signal Transduction, Granzymes metabolism, STAT3 Transcription Factor metabolism

Abstract

Granzyme M is a serine protease known to be often expressed by natural killer cells and induce target cells apoptosis in combination with perforin. However, we detected granzyme M expression in murine and human cancer cell lines and human tumor samples in our study. Granzyme M increased chemoresistance, colony-formation, cytokine secretion and invasiveness in vitro. Most importantly, granzyme M facilitated tumor growth and metastasis in vivo. Granzyme M induced the epithelial-mesenchymal transition (EMT) in cancer cells associated with STAT3 activation. Our study revealed the role of granzyme M expressed by tumor in chemoresistance, invasion, metastasis and EMT.

Published

2015

94. Cytolytic activity of purified cytoplasmic granules from cytotoxic rat large granular lymphocyte tumors

Author

Craig W. Reynolds, Maryanna Henkart, Paul J. Millard, and Pierre A. Henkart

Subjects

Cytotoxicity, Immunologic, Chemical Phenomena, Lymphocyte, Immunology, chemistry.chemical_element, Pronase, Biology, Calcium, Cytoplasmic Granules, Drug Stability, Nucleated cell, medicine, Immunology and Allergy, Cytotoxic T cell, Animals, Leukemia, Experimental, Chemistry, Physical, Cytotoxins, Granule (cell biology), Antibody-Dependent Cell Cytotoxicity, Articles, Rats, Inbred F344, Cell biology, Rats, Killer Cells, Natural, Cytolysis, Kinetics, medicine.anatomical_structure, chemistry, Granzyme M, Lysosomes

Abstract

Purified cytoplasmic granules from cytotoxic rat large granular lymphocytes (LGL) tumors were cytolytic to erythrocytes, splenocytes, and a number of different lymphoid tumor cells. Granule concentrations of approximately 1 microgram/ml granule protein were adequate to lyse 100% of the erythrocytes, while the nucleated cells required up to 100 micrograms/ml granule protein to achieve complete lysis. Cytoplasmic granules purified from noncytotoxic lymphoid cells did not contain detectable cytolytic activity; purified granules from rat mast cells and rat liver lysosomes likewise failed to display cytolytic activity. However, granules prepared from normal rat peripheral blood LGL were cytolytic. Granule-mediated lysis of erythrocytes and nucleated cells was complete within 3 min at room temperature. The lytic activity required calcium at concentrations of 10(-4)-10(-2) M; magnesium or barium failed to replace calcium, while strontium could replace calcium at 10(-3)-10(-2) M when nucleated cells were the target. Exposure of LGL tumor granules to calcium before the addition of target cells resulted in an inactivation of granule cytolytic activity over the course of 20 min at room temperature. Granule cytolytic activity was heat and Pronase sensitive, and could be solubilized by 2 M salt. Examination of granules exposed to calcium in the electron microscope using negative staining showed that calcium treatment of granules results in the formation of ring-shaped structures previously described to be associated with LGL-mediated cytotoxicity. These results provide support for the hypothesis that the cytotoxic processes mediated by LGL are a secretory event characterized by the release of cytolytic material from the cytoplasmic granules after triggering by a surface receptor. The results further suggest that the ring structures visible in the electron microscope are associated with the lytic event.

Published

1984

95. A family of serine esterases in lytic granules of cytolytic T lymphocytes

Author

Danièle Masson and Jürg Tschopp

Subjects

Serine Endopeptidases, Esterases, Biology, Cytoplasmic Granules, Granzymes, General Biochemistry, Genetics and Molecular Biology, Rats, Granzyme B, Serine, Perforin, Granzyme, Biochemistry, Sequence Homology, Nucleic Acid, Endopeptidases, medicine, biology.protein, Granzyme A, Animals, Diisopropyl fluorophosphate, Granzyme K, Amino Acid Sequence, Granzyme M, T-Lymphocytes, Cytotoxic, medicine.drug

Abstract

Cytoplasmic granules of cytolytic T lymphocytes (CTLs) contain, in addition to the pore-forming protein perforin, a family of highly homologous serine esterases, granzymes A-H. The serine esterase affinity label diisopropyl fluorophosphate reacts strongly with granzymes A and D, to a lesser extent with B, E, F, G, and H, and not at all with C and F. For granzymes A and D, synthetic substrates have been found. Antibodies raised against granzyme B strongly cross-react with A, G, and H, and antibodies to granzyme D recognize C, E, and F. These antigenic relationships correlate with similarities in the N-terminal amino acid sequences. At least 60% homology is observed between the eight proteins, and all are similar to rat mast cell protease 2. Sequence analysis suggests the identity of granzyme A with a protease predicted from a CTL-specific cDNA clone (H factor) and of granzyme B, G, or H with a protein encoded by the CTL-specific cDNA clone CTLA 1/CCP 1.

Published

1987

96. Induction of target cell DNA release by the cytotoxic T lymphocyte granule protease granzyme A

Author

Pierre A. Henkart, G A Berrebi, and M P Hayes

Subjects

Proteases, Lysis, Serine Proteinase Inhibitors, Immunology, Cytoplasmic Granules, Ammonium Chloride, Granzymes, Cell Line, chemistry.chemical_compound, Mice, Immunology and Allergy, Animals, Monensin, biology, Cytotoxins, Serine Endopeptidases, Articles, DNA, Molecular biology, Molecular Weight, Phenylmethylsulfonyl Fluoride, CTL, chemistry, Granzyme, Biochemistry, biology.protein, Granzyme A, Cytolysin, Granzyme M, PMSF, T-Lymphocytes, Cytotoxic

Abstract

The rapid breakdown of target cell DNA during CTL-mediated lysis has been difficult to explain by the granule exocytosis model of cytotoxicity. The involvement of CTL granule proteases in this process was strongly suggested by experiments in which CTL were pretreated with the serine protease inhibitor PMSF, in combination with agents that raise the pH of acidic intracellular compartments. While PMSF pretreatment alone had little effect on target lysis or DNA breakdown, the combination of PMSF and NH4Cl or monensin profoundly reduced target cell DNA release, while little effect was observed on target lysis, as measured by 51Cr release. CTL granule extracts cause release of 125I-DNA from detergent-permeabilized cells. This nuclear DNA-releasing (NDR) activity is inhibited by serine esterase inhibitors that also inhibit the granule BLT-esterase activity, and is specifically immunoabsorbed by antibodies to the CTL granule protease granzyme A. The NDR activity comigrates with BLT-esterase activity during subcellular fractionation, solubilization, gel filtration, and aprotinin-Sepharose affinity chromatography. SDS-PAGE analysis of the affinity-purified product indicates a molecular mass of 60,000 daltons under non-reducing conditions, which moves to 30,000 daltons upon reduction, consistent with previously reported behavior of granzyme A. When the purified material was reduced and alkylated, both esterase and NDR activities comigrated at 30,000 daltons upon gel filtration. Although fully lytic concentrations of purified LGL granule cytolysin alone failed to induce target cell DNA release, a combination of purified granzyme A and the cytolysin induces substantial DNA release.

Published

1989

97. Mechanism of Lymphocyte-Mediated Cytotoxicity

Author

Pierre A. Henkart

Subjects

Cytotoxicity, Immunologic, Lymphocyte, Immunology, In Vitro Techniques, Biology, Cytoplasmic Granules, Exocytosis, Pore forming protein, Natural killer cell, Mice, Osmotic Pressure, medicine, Animals, Humans, Immunology and Allergy, Lymphocytes, Antigens, Cytotoxicity, Lymphotoxin-alpha, Mechanism (biology), Cell Membrane, T lymphocyte, Cell biology, Killer Cells, Natural, medicine.anatomical_structure, Granzyme M, T-Lymphocytes, Cytotoxic

Published

1985

98. Granzymes, a Family of Serine Proteases Released from Granules of Cytolytic T Lymphocytes upon T Cell Receptor Stimulation

Author

Dieter E. Jenne and Jürg Tschopp

Subjects

Signal peptide, Proteases, Molecular Sequence Data, Immunology, Receptors, Antigen, T-Cell, Cathepsin G, Cytoplasmic Granules, Granzymes, Mice, chemistry.chemical_compound, Animals, Immunology and Allergy, Cytotoxic T cell, Amino Acid Sequence, biology, Serine Endopeptidases, Degranulation, DNA, Cell biology, Molecular Weight, Perforin, Biochemistry, chemistry, Granzyme, biology.protein, Granzyme M, T-Lymphocytes, Cytotoxic

Abstract

The cytolytic potential of T effector cells appears to be intimately related to the presence of proteins stored in specialized cytoplasmic granules. A striking biological property of isolated granules is their lytic activity for a variety of target cells in a nonrestricted manner. Proteins contained within these granules of CTLs are specifically released upon target cell recognition. We have isolated and characterized six granule-associated proteins in two murine CTL lines in addition to the pore-forming and target membrane-disrupting perforin. Six full length cDNA clones have been identified in a CTL-specific cDNA expression library which code for the granule-associated serine esterases, designated as granzymes A to F. Granzymes A and B represent the genuine proteins encoded by the H factor/CTLA-3 cDNA and the CTLA-1/CCPI cDNA, respectively. The covalent amino acid structures of all six granzymes show the hallmarks for serine proteases and are highly related to that of rat mast cell protease I and II and cathepsin G, which have been found in granules of mast cells and neutrophilic granulocytes, respectively. The primary translation products are processed by removal of a hydrophobic signal peptide and a two residue-long propeptide at the amino-terminus. Immuno-electron microscopy shows that granzymes and perforin are stored together within secretory granules of CTLs. Simultaneous release of at least two of these granzymes has been observed during degranulation of a murine CTL line by anti-T3 antibodies. The biological role, particularly the proteolytic events elicited by granzyme A and other granzymes in the context of target cell recognition, are not known at present. It is unlikely that they form a proteolytic activation cascade together with pore-forming proteins analogous to the complement system. The strictly regulated secretion of granzymes and the lack of measurable enzymatic activity in the case of granzymes B, C, E and F towards a variety of synthetic substrates suggest a highly specific function for each of them.

Published

1988

99. A novel serine esterase expressed by cytotoxic T lymphocytes

Author

Herman N. Eisen and Mark S. Pasternack

Subjects

Cytotoxicity, Immunologic, Proteases, Multidisciplinary, T-Lymphocytes, Esterases, Affinity Labels, T lymphocyte, Biology, Molecular biology, Esterase, In vitro, Molecular Weight, Phenylmethylsulfonyl Fluoride, Mice, chemistry.chemical_compound, chemistry, Biochemistry, Cell culture, Animals, Cytotoxic T cell, PMSF, Granzyme M, T-Lymphocytes, Cytotoxic

Abstract

Cytotoxic T (Tc) lymphocytes recognize and lyse target cells and are thought to serve as an important defence against viral infections and possibly against neoplasms. The nature of the receptors responsible for antigen recognition by these cells is becoming clearer, but the molecular mechanisms responsible for their cytolytic activity remain largely unknown. The possibility that proteases are involved in this process has been suggested by the effects of certain inhibitors. Here we demonstrate that clones of murine Tc cells possess considerable trypsin-like esterase activity when assayed by a sensitive colorimetric assay. This activity was blocked completely by two serine esterase inhibitors, diisopropylfluorophosphoridate (DFP) and phenylmethylsulphonyl fluoride (PMSF), but not by N alpha-tosyl lysyl chloromethyl ketone (TLCK). The use of 3H-DFP as an affinity-labelling reagent demonstrated that the esterase activity resides in a protein of relative molecular mass (Mr) 28,000 (28K). A wide variety of other lymphocytes, including those from thymus, spleen and lymph node, established lines of B cells and noncytotoxic T cells, and clones of T helper cells, had about 300-fold less esterase activity than the Tc-cell clones and far smaller amounts of the DFP-reactive 28K protein. However, in thymocytes the esterase activity increased 20-50-fold and the 28K protein became more prominent 4 days after these cells had been stimulated in vitro to generate Tc cells.

Published

1985