Regulation of Signal Transducer and Activator of Transcription Signaling by the Tyrosine Phosphatase PTP-BL

Nakahira, Masakiyo; Tanaka, Takashi; Robson, Bryanne E.; Mizgerd, Joseph P.; Grusby, Michael J.

doi:10.1016/j.immuni.2007.01.010

Cited by 52 publications

(57 citation statements)

References 57 publications

(65 reference statements)

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“…Genetic and biochemical approaches have implicated several phosphatases in the decay of cytokine receptors and JAKs, including SHP-1, SHP-2, and potentially CD45 (2,33). Similar approaches have underscored a role for SHP-2, PTP1B, TC-PTP, and PTP-BL in STAT dephosphorylation (2,33,34). However, only two of these phosphatases, SHP-2 and TC-PTP, have been implicated in nuclear STAT dephosphorylation, which appears to be critical for STAT nuclear export (16,17,33).…”

Section: Regulation Of Stat Activitymentioning

confidence: 99%

JAK-STAT Signaling: From Interferons to Cytokines

Schindler

Levy

Decker

2007

Journal of Biological Chemistry

1,085

899

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50 years ago Isaacs and Lindenmann (1) first described interferons (IFNs) 2 as founding members of the cytokine family. Over the next 25 years, these and several other four-helix bundle cytokines were characterized. The subsequent 25 years witnessed an exponential growth in number of four-helix bundle cytokines and their corresponding receptors.The early availability of recombinant IFNs afforded an opportunity to investigate how cytokines induce gene expression, culminating in the identification of the JAK-STAT signaling paradigm (see Fig. 1). Subsequent studies identified 7 STATs and 4 JAKs, providing important insight into how the ϳ50 members of the four-helix bundle cytokine family transduce their potent biological responses. This review will briefly summarize this signaling paradigm (reviewed in Refs. 2-5) and then focus on STAT-dependent transcription.

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Section: Regulation Of Stat Activitymentioning

confidence: 99%

JAK-STAT Signaling: From Interferons to Cytokines

Schindler

Levy

Decker

2007

Journal of Biological Chemistry

1,085

899

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“…These PTP-BL deleted mice demonstrated increased STAT4 phosphorylation in CD4 + -T cells upon IL-12 and T-cell receptor activation [37]. The PTP-BL deleted mice also demonstrated enhanced maturation of T-cells and increased immune modulated killing following the inoculation of bacteria into their lungs [37]. These studies suggest that while PTPL1 is not critical for normal murine development, this phosphatase may participate in very different aspects of cellular physiology.…”

Section: Effects Of Gene Targeting Experiments For Ptp-bl In Micementioning

confidence: 98%

“…The second model created was a complete knock-out of PTP-BL. These PTP-BL deleted mice demonstrated increased STAT4 phosphorylation in CD4 + -T cells upon IL-12 and T-cell receptor activation [37]. The PTP-BL deleted mice also demonstrated enhanced maturation of T-cells and increased immune modulated killing following the inoculation of bacteria into their lungs [37].…”

Section: Effects Of Gene Targeting Experiments For Ptp-bl In Micementioning

confidence: 99%

“…In a similar experimental design, a substrate-trapping mutant of PTPL1 co-immunoprecipitated with HER2 in epidermal growth factor stimulated HEK293 cells that over-expressed exogenous HER2, thus making it a putative substrate [21]. STAT4 was identified as a putative substrate of PTP-BL, the mouse homolog of PTPL1 [37]. Additional work will be necessary in order to definitively prove that IκBα, IRS-1, HER2, and STAT4 are bona fide substrates of PTPL1.…”

Section: Substratesmentioning

confidence: 99%

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PTPL1: a large phosphatase with a split personality

Abaan

Toretsky

2008

Cancer Metastasis Rev

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Protein tyrosine phosphatase, PTPL1, (also known as PTPN13, FAP-1, PTP-BAS, PTP1E) is a non-receptor type PTP and, at 270 kDa, is the largest phosphatase within this group. In addition to the well-conserved PTP domain, PTPL1 contains at least 7 putative macromolecular interaction domains. This structural complexity indicates that PTPL1 may modulate diverse cellular functions, perhaps exerting both positive and negative effects. In accordance with this idea, while certain studies suggest that PTPL1 can act as a tumor-promoting gene other experimental studies have suggested that PTPL1 may function as a tumor suppressor. The role of PTPL1 in the cancer cell is therefore likely to be both complex and context dependent with possible roles including the modulation of growth, stress-response, and cytoskeletal remodeling pathways. Understanding the nature of molecular complexes containing PTPL1, its interaction partners, substrates, regulation and subcellular localization are key to unraveling the complex personality of this protein phosphatase.

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“…Published studies using mutant mice that lack PTPN13 protein product or phosphatase activity did not report any effect on tumor susceptibility. Indeed none phenotypic consequences have been reported for PTPN13 KO mice 35 and studies of mice that lack PTPN13 phosphatase activity have focused on hematopoietic cell lineages and the peripheral nervous system, 36 which were previously shown to express this phosphatase. 37,38 Thus, crossbreeding of these mice with mammary tumor model mice could be used to evaluate the role of PTPL1 in tumor progression and susceptibility.…”

mentioning

confidence: 99%

Expression of the putative tumor suppressor gene PTPN13/PTPL1 is an independent prognostic marker for overall survival in breast cancer

Révillion

Puech

Rabenoelina

et al. 2008

Intl Journal of Cancer

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Although it is well established that some protein tyrosine kinases have a prognostic value in breast cancer, the involvement of protein tyrosine phosphatases (PTPs) is poorly substantiated for breast tumors. Three of these enzymes (PTP-gamma, LAR, and PTPL1) are already known to be regulated by estrogens or their antagonists in human breast cancer cells. We used a real-time reverse transcriptase polymerase chain reaction method to test the expression levels of PTP-gamma, LAR and its neuronal isoform, and PTPL1 in a training set of RNA from 59 breast tumors. We sought correlations between levels of these molecular markers, current tumor markers, and survival. We then quantified the expression level of the selected phosphatase in 232 additional samples, resulting in a testing set of 291 breast tumor RNAs from patients with a median follow-up of 6.4 years. The Spearman nonparametric test revealed correlations between PTPL1 expression and differentiation markers. Cox univariate analysis of the overall survival studies demonstrated that PTPL1 is a prognostic factor [risk ratio (RR) 5 0.45], together with the progesterone receptor (PR) (RR 5 0.52) and node involvement (RR 5 1.58). In multivariate analyses, PTPL1 and PR retained their prognostic value (RRs of 0.48 and 0.55, respectively). This study demonstrates for the first time that PTPL1 expression level is an independent prognostic indicator of favorable outcome for patients with breast cancer. In conjunction with our mechanistic studies, this finding identifies PTPL1 as an important regulatory element of human breast tumor aggressiveness and sensitivity to treatments such as antiestrogens and antiaromatase.

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Regulation of Signal Transducer and Activator of Transcription Signaling by the Tyrosine Phosphatase PTP-BL

Cited by 52 publications

References 57 publications

JAK-STAT Signaling: From Interferons to Cytokines

JAK-STAT Signaling: From Interferons to Cytokines

PTPL1: a large phosphatase with a split personality

Expression of the putative tumor suppressor gene PTPN13/PTPL1 is an independent prognostic marker for overall survival in breast cancer

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