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PTPN1 protein, human OR C516607 Dotaz Zobrazit nápovědu

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2 záznamů v PubMed

Článek

Autoinflammatory encephalopathy due to PTPN1 haploinsufficiency: a case series

I interferon (IFN) signalling, we identified a cohort of individuals heterozygous for mutations in PTPN1 ...

Zhu, Gaofeng
Autor Zhu, Gaofeng MRC Human Genetics Unit, Institute of Genetics and Cancer, University of Edinburgh, Edinburgh, UK
Didry-Barca, Blaise
Autor Didry-Barca, Blaise Laboratory of Neurogenetics and Neuroinflammation, Imagine Institute, INSERM UMR1163, Université Paris Cité, Paris, France
Seabra, Luis
Autor Seabra, Luis Laboratory of Neurogenetics and Neuroinflammation, Imagine Institute, INSERM UMR1163, Université Paris Cité, Paris, France
Rice, Gillian I
Autor Rice, Gillian I Division of Evolution and Genomic Sciences, School of Biological Sciences, Faculty of Biology, Medicine, and Health, University of Manchester, Manchester Academic Health Science Centre, Manchester, UK
Uggenti, Carolina
Autor Uggenti, Carolina MRC Human Genetics Unit, Institute of Genetics and Cancer, University of Edinburgh, Edinburgh, UK
Touimy, Moncef
Autor Touimy, Moncef Laboratory of Neurogenetics and Neuroinflammation, Imagine Institute, INSERM UMR1163, Université Paris Cité, Paris, France
Rodero, Mathieu P
Autor Rodero, Mathieu P Laboratory of Neurogenetics and Neuroinflammation, Imagine Institute, INSERM UMR1163, Université Paris Cité, Paris, France
Trapero, Rolando Hernandez
Autor Trapero, Rolando Hernandez MRC Human Genetics Unit, Institute of Genetics and Cancer, University of Edinburgh, Edinburgh, UK
Bondet, Vincent
Autor Bondet, Vincent Translational Immunology Unit, Institut Pasteur, Université Paris Cité, Paris, France
Duffy, Darragh
Autor Duffy, Darragh Translational Immunology Unit, Institut Pasteur, Université Paris Cité, Paris, France

The Lancet. Neurology. 2025 Mar ; 24 (3) : 218-229.

Lancet Neurol
ISSN 1474-4465 | 1474-4422
Zdroj

BACKGROUND: Through the agnostic screening of patients with uncharacterised disease phenotypes for an upregulation of type I interferon (IFN) signalling, we identified a cohort of individuals heterozygous for mutations in PTPN1, encoding the protein-tyrosine phosphatase 1B (PTP1B). We aimed to describe the clinical phenotype and molecular and cellular pathology of this new disease. METHODS: In this case series, we identified patients and collected clinical and neuroradiological data through collaboration with paediatric neurology and clinical genetics colleagues across Europe (Czechia, France, Germany, Italy, Slovenia, and the UK) and Israel. Variants in PTPN1 were identified by exome and directed Sanger sequencing. The expression of IFN-stimulated genes was determined by quantitative (q) PCR or NanoString technology. Experiments to assess RNA and protein expression and to investigate type 1 IFN signalling were undertaken in patient fibroblasts, hTERT-immortalised BJ-5ta fibroblasts, and RPE-1 cells using CRISPR-Cas9 editing and standard cell biology techniques. FINDINGS: Between Dec 20, 2013, and Jan 11, 2023, we identified 12 patients from 11 families who were heterozygous for mutations in PTPN1. We found ten novel or very rare variants in PTPN1 (frequency on gnomAD version 4.1.0 of <1·25 × 10:sup>-6). Six variants were predicted as STOP mutations, two involved canonical splice-site nucleotides, and two were missense substitutions. In three patients, the variant occurred de novo, whereas in nine affected individuals, the variant was inherited from an asymptomatic parent. The clinical phenotype was characterised by the subacute onset (age range 1-8 years) of loss of motor and language skills in the absence of seizures after initially normal development, leading to spastic dystonia and bulbar involvement. Neuroimaging variably demonstrated cerebral atrophy (sometimes unilateral initially) or high T2 white matter signal. Neopterin in CSF was elevated in all ten patients who were tested, and all probands demonstrated an upregulation of IFN-stimulated genes in whole blood. Although clinical stabilisation and neuroradiological improvement was seen in both treated and untreated patients, in six of eight treated patients, high-dose corticosteroids were judged clinically to result in an improvement in neurological status. Of the four asymptomatic parents tested, IFN signalling in blood was normal (three patients) or minimally elevated (one patient). Analysis of patient blood and fibroblasts showed that tested PTPN1 variants led to reduced levels of PTPN1 mRNA and PTP1B protein, and in-vitro assays demonstrated that loss of PTP1B function was associated with impaired negative regulation of type 1 IFN signalling. INTERPRETATION: PTPN1 haploinsufficiency causes a type 1 IFN-driven autoinflammatory encephalopathy. Notably, some patients demonstrated stabilisation, and even recovery, of neurological function in the absence of treatment, whereas in others, the disease appeared to be responsive to immune suppression. Prospective studies are needed to investigate the safety and efficacy of specific immune suppression approaches in this disease population. FUNDING: The UK Medical Research Council, the European Research Council, and the Agence Nationale de la Recherche.

MeSH
dítě MeSH
haploinsuficience * genetika MeSH
kojenec MeSH
lidé MeSH
mladiství MeSH
mutace genetika MeSH
nemoci mozku genetika MeSH
neurozánětlivé nemoci genetika MeSH
předškolní dítě MeSH
tyrosinfosfatasa nereceptorového typu 1 * genetika MeSH
Check Tag
dítě MeSH
kojenec MeSH
lidé MeSH
mladiství MeSH
mužské pohlaví MeSH
předškolní dítě MeSH
ženské pohlaví MeSH
Publikační typ
časopisecké články MeSH
Názvy látek
PTPN1 protein, human MeSH Prohlížeč
tyrosinfosfatasa nereceptorového typu 1 * MeSH

Článek

Tyrosine phosphatases regulate resistance to ALK inhibitors in ALK+ anaplastic large cell lymphoma

By applying genomic loss-of-function screens, we identified PTPN1 and PTPN2 phosphatases as consistent ...

Blood. 2022 Feb 03 ; 139 (5) : 717-731.

ISSN 1528-0020 | 0006-4971
Zdroj

Anaplastic large cell lymphomas (ALCLs) frequently carry oncogenic fusions involving the anaplastic lymphoma kinase (ALK) gene. Targeting ALK using tyrosine kinase inhibitors (TKIs) is a therapeutic option in cases relapsed after chemotherapy, but TKI resistance may develop. By applying genomic loss-of-function screens, we identified PTPN1 and PTPN2 phosphatases as consistent top hits driving resistance to ALK TKIs in ALK+ ALCL. Loss of either PTPN1 or PTPN2 induced resistance to ALK TKIs in vitro and in vivo. Mechanistically, we demonstrated that PTPN1 and PTPN2 are phosphatases that bind to and regulate ALK phosphorylation and activity. In turn, oncogenic ALK and STAT3 repress PTPN1 transcription. We found that PTPN1 is also a phosphatase for SHP2, a key mediator of oncogenic ALK signaling. Downstream signaling analysis showed that deletion of PTPN1 or PTPN2 induces resistance to crizotinib by hyperactivating SHP2, the MAPK, and JAK/STAT pathways. RNA sequencing of patient samples that developed resistance to ALK TKIs showed downregulation of PTPN1 and PTPN2 associated with upregulation of SHP2 expression. Combination of crizotinib with a SHP2 inhibitor synergistically inhibited the growth of wild-type or PTPN1/PTPN2 knock-out ALCL, where it reverted TKI resistance. Thus, we identified PTPN1 and PTPN2 as ALK phosphatases that control sensitivity to ALK TKIs in ALCL and demonstrated that a combined blockade of SHP2 potentiates the efficacy of ALK inhibition in TKI-sensitive and -resistant ALK+ ALCL.

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PTPN1 protein, human OR C516607 Dotaz Zobrazit nápovědu

PTPN1 protein, human OR C516607 Dotaz Zobrazit nápovědu

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