The Functional Basis for Hemophagocytic Lymphohistiocytosis in a Patient with Co-inherited Missense Mutations in the Perforin (<i>PFN1</i>) Gene

Voskoboinik, Ilia; Thia, Marie Claude; Bono, Annette De; Browne, Kylie A.; Cretney, Erika; Jackson, Jacob T.; Darcy, Phillip K.; Jane, Stephen M.; Smyth, Mark J.; Trapani, Joseph A.

doi:10.1084/jem.20040776

Cited by 70 publications

(100 citation statements)

References 23 publications

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“…Before recombinant Gzm/Pfp treatment, cells were washed three times in DMEM media containing 0.5% BSA (Fraction V, Roche Diagnostics GmbH, Basel, Switzerland). Recombinant human GzmB, hGzmA or mGzmA were diluted in DMEM/BSA buffer and added to target cells before addition of a sublytic dose of recombinant mouse Pfp (purified in house to a concentration of 300 mg/ml, as previously described 41 ).…”

Section: Methodsmentioning

confidence: 99%

Mouse granzyme A induces a novel death with writhing morphology that is mechanistically distinct from granzyme B-induced apoptosis

et al. 2013

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Human and mouse granzyme (Gzm)B both induce target cell apoptosis in concert with pore-forming perforin (Pfp); however the mechanisms by which other Gzms induce non-apoptotic death remain controversial and poorly characterised. We used timelapse microscopy to document, quantitatively and in real time, the death of target cells exposed to primary natural killer (NK) cells from mice deficient in key Gzms. We found that in the vast majority of cases, NK cells from wild-type mice induced classic apoptosis. However, NK cells from syngeneic Gzm B-deficient mice induced a novel form of cell death characterised by slower kinetics and a pronounced, writhing, 'worm-like' morphology. Dying cells initially contracted but did not undergo membrane blebbing, and annexin-V staining was delayed until the onset of secondary necrosis. As it is different from any cell death process previously reported, we tentatively termed this cell death 'athetosis'. Two independent lines of evidence showed this alternate form of death was due to Gzm A: first, cell death was revealed in the absence of Gzm B, but was completely lost when the NK cells were deficient in both Gzm A and B; second, the athetotic morphology was precisely reproduced when recombinant mouse Gzm A was delivered by an otherwise innocuous dose of recombinant Pfp. Gzm A-mediated athetosis did not require caspase activation, early mitochondrial disruption or generation of reactive oxygen species, but did require an intact actin cytoskeleton and was abolished by latrunculin B and mycalolide B. This work defines an authentic role for mouse Gzm A in granule-induced cell death by cytotoxic lymphocytes.

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Section: Methodsmentioning

confidence: 99%

Mouse granzyme A induces a novel death with writhing morphology that is mechanistically distinct from granzyme B-induced apoptosis

et al. 2013

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“…Western immunoblotting was performed using reducing or nonreducing Laemmli SDS/PAGE loading buffer, and PRF was detected using rat anti-mouse mAb (P1-8, provided by H. Yagita, Juntendo University, Tokyo) as described in ref. 29. Following transfection, the cells were cultured at 37°C in 5% CO 2 (mouse lymphocytes) or 10% CO 2 (RBL-2H3 cells) for 18 -24 h. To test for temperature sensitivity, cells were cultured at 30°C for 18 -24 h after transfection.…”

Section: Methodsmentioning

confidence: 99%

“…Primary CTL culture, transfection using the Amaxa Nucleofector Technology, FACS sorting of transfected lymphocytes, and 51 Cr release cytotoxicity assays were all performed as described (19). The culture of rat basophil leukemia (RBL)-2H3 cells, gene transfection, FACS sorting, and cytotoxicity assays were also carried out as previously described (29). Western immunoblotting was performed using reducing or nonreducing Laemmli SDS/PAGE loading buffer, and PRF was detected using rat anti-mouse mAb (P1-8, provided by H. Yagita, Juntendo University, Tokyo) as described in ref.…”

Section: Methodsmentioning

confidence: 99%

Temperature sensitivity of human perforin mutants unmasks subtotal loss of cytotoxicity, delayed FHL, and a predisposition to cancer

Chia

Yeo

Whisstock

et al. 2009

Proc. Natl. Acad. Sci. U.S.A.

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122

141

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The pore-forming protein perforin is critical for defense against many human pathogens and for preventing a catastrophic collapse of immune homeostasis, manifested in infancy as Type 2 familial hemophagocytic lymphohistiocytosis (FHL). However, no evidence has yet linked defective perforin cytotoxicity with cancer susceptibility in humans. Here, we examined perforin function in every patient reported in the literature who lived to at least 10 years of age without developing FHL despite inheriting mutations in both of their perforin (PRF1) alleles. Our analysis showed that almost 50% of these patients developed at least 1 hematological malignancy in childhood or adolescence. The broad range of pathologies argued strongly against a common environmental or viral cause for the extraordinary cancer incidence. Functionally, what distinguished these patients was their inheritance of PRF1 alleles encoding temperature-sensitive missense mutations. By contrast, truly null missense mutations with no rescue at the permissive temperature were associated with the more common severe presentation with FHL in early infancy. Our study provides the first mechanistic evidence for a link between defective perforinmediated cytotoxicity and cancer susceptibility in humans and establishes the paradigm that temperature sensitivity of perforin function is a predictor of FHL severity.hemophagocytic lymphohistiocytosis ͉ immunodeficiency ͉ leukemia ͉ lymphoma

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“…Loading GzmK with perforin was performed as described previously. 15,40 Briefly, a sublytic dose was first titrated with recombinant perforin. Then the sublytic dose of perforin was used in combination with GzmK or S-AGzmK at each assay.…”

Section: Methodsmentioning

confidence: 99%

Granzyme K cleaves the nucleosome assembly protein SET to induce single-stranded DNA nicks of target cells

et al. 2006

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Although granzymes (Gzms) A-and B-induced cell death pathways have been defined, little is known about how other orphan Gzms function in CTL-mediated cytotoxicity. GzmK and A are tryptases among all the Gzms of humans and they are closely linked on the same chromosome. In this study, we showed that GzmK can be efficiently delivered into target cells with a cationic lipid protein transfection reagent Pro-Ject. We found human GzmK triggers rapid cell death independently of caspase activation. The features of death are characterized by rapid externalization of phosphatidylserine, nuclear morphological changes and single-stranded DNA nicks. GzmK hydrolyzes the nucleosome assembly protein SET in its recombinant and native forms or in intact cells. Cleavage of SET by GzmK abrogates its nucleosome assembly activity. After GzmK loading, SET and DNase NM23H1 rapidly translocate into the nucleus and SET is cleaved, where the nuclease activity of NM23H1 is activated to nick chromosomal DNA.

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The Functional Basis for Hemophagocytic Lymphohistiocytosis in a Patient with Co-inherited Missense Mutations in the Perforin (PFN1) Gene

Cited by 70 publications

References 23 publications

Mouse granzyme A induces a novel death with writhing morphology that is mechanistically distinct from granzyme B-induced apoptosis

Mouse granzyme A induces a novel death with writhing morphology that is mechanistically distinct from granzyme B-induced apoptosis

Temperature sensitivity of human perforin mutants unmasks subtotal loss of cytotoxicity, delayed FHL, and a predisposition to cancer

Granzyme K cleaves the nucleosome assembly protein SET to induce single-stranded DNA nicks of target cells

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