Identification of Nuclear Export Signals in Antizyme-1

Murai, Noriyuki; Murakami, Yasuko; Matsufuji, Senya

doi:10.1074/jbc.m308059200

Cited by 38 publications

(35 citation statements)

References 38 publications

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“…We did not, however, observe a preferential association of GFP-antizyme with one centriole which might be due to non-physiological expression of the fusion protein. Consistent with previous reports (Murai et al, 2003), the GFP-antizyme 1 signal was otherwise mostly cytoplasmic and not nuclear.…”

Section: Resultssupporting

confidence: 92%

“…Treatment with the microtubule-depolymerizing drug nocodazole did not displace the centrosomal antizyme 1 signal demonstrating that the localization of antizyme 1 is microtubule independent (Supplementary data S1). In addition to its centrosomal localization, antizyme 1 was also detected in the nucleus (Figures 1a and d and Supplementary data S1) as reported previously (Murai et al, 2003). The nuclear localization of antizyme 1 was, however, only detected in a fraction of U2OS and NIH-3T3 cells (Figures 1a and d).…”

Section: Resultssupporting

confidence: 85%

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Antizyme, a mediator of ubiquitin-independent proteasomal degradation and its inhibitor localize to centrosomes and modulate centriole amplification

et al. 2007

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The potential tumor suppressor antizyme and its endogenous inhibitor (antizyme inhibitor, AZI) have been implicated in the ubiquitin-independent proteasomal degradation of proteins involved in cell proliferation as well as in the regulation of polyamine levels. We show here that both antizyme and AZI concentrate at centrosomes and that antizyme preferentially associates with the maternal centriole. Interestingly, alterations in the levels of these proteins have opposing effects on centrosomes. Depletion of antizyme in various cell lines and primary cells leads to centrosome overduplication, whereas overexpression of antizyme reduces numerical centrosome abnormalities. Conversely, silencing of the antizyme inhibitor, AZI, results in a decrease of numerical centrosome abnormalities, whereas overexpression of AZI leads to centrosome overduplication. We further show that the numerical centrosome abnormalities are due to daughter centriole amplification. In summary, our results demonstrate that alterations in the antizyme/AZI balance cause numerical centrosomal defects and suggest a role for ubiquitin-independent proteasomal degradation in centrosome duplication.

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Section: Resultssupporting

confidence: 92%

Section: Resultssupporting

confidence: 85%

Antizyme, a mediator of ubiquitin-independent proteasomal degradation and its inhibitor localize to centrosomes and modulate centriole amplification

et al. 2007

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“…In accordance with our results with alanine scanning, this substitution resulted in nuclear accumulation of K259N GAPDH (Fig. 6, G and H) (7,(23)(24)(25)(26).…”

Section: Discussionsupporting

confidence: 78%

A Novel CRM1-mediated Nuclear Export Signal Governs Nuclear Accumulation of Glyceraldehyde-3-phosphate Dehydrogenase following Genotoxic Stress

Brown

Krynetski

Krynetskaia

et al. 2004

Journal of Biological Chemistry

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Glyceraldehyde-3-phosphate dehydrogenase (GAPDH) is a multifunctional protein with glycolytic and nonglycolytic functions, including pro-apoptotic activity. GAPDH accumulates in the nucleus after cells are treated with genotoxic drugs, and it is present in a protein complex that binds DNA modified by thioguanine incorporation. We identified a novel CRM1-dependent nuclear export signal (NES) comprising 13 amino acids (KKVVKQASEGPLK) in the C-terminal domain of GAPDH, truncation or mutation of which abrogated CRM1 binding and caused nuclear accumulation of GAPDH. Alanine scanning of the sequence encompassing the putative NES demonstrated at least two regions important for nuclear export. Site mutagenesis of Lys 259 did not affect oligomerization but impaired nuclear efflux of GAPDH, indicating that this amino acid residue is essential for proper functioning of this NES. This novel NES does not contain multiple leucine residues unlike other CRM1-interacting NES, is conserved in GAPDH from multiple species, and has sequence similarities to the export signal found in feline immunodeficiency virus Rev protein. Similar sequences (KKVV*7-13PLK) were found in two other human proteins, U5 small nuclear ribonucleoprotein, and transcription factor BT3.

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“…The previous report showed that AZ1 is primarily localized in the nucleus where it transports ODC from the cytosol for degradation by nuclear proteasome (Gritli-Linde et al 2001, Murai et al 2003, Schipper et al 2004. By contrast, we found that AZ1 was mainly localized in the cytosol during conversion of AsPC-1 cells to the differentiated state (Fig.…”

Section: J-i Suzuki Et Al: Glucagon-producing Cell Differentiationcontrasting

confidence: 52%

“…Rat AZ1 has an w85% homology to human AZ1. It expresses a full-length AZ1 without the frameshift because of the deletion of one thymine nucleotide (Murai et al 2003). Transfection was carried out with 4.0 mg plasmid DNA/well using Lipofectamine 2000.…”

Section: Transfection and Stably Expression Of Egfp-rat Az1mentioning

confidence: 99%

Antizyme is necessary for conversion of pancreatic tumor cells into glucagon-producing differentiated cells

Suzuki¹,

Murakami²,

Samejima³

et al. 2009

Endocrine-Related Cancer

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Human pancreatic tumor cell lines -AsPC-1, PANC-1, MIA paca2, KP-1 and KP-59 cellscan be induced to differentiate into pancreatic hormone-producing cells by brief trypsin treatment and subsequent culture in a serum-free, chemically defined medium. During culture, AsPC-1 cells formed cell clusters resembling the pancreatic islets, expressed genes associated with the pancreatic development and produced glucagon but not insulin. When PANC-1, MIA paca2, KP-1 and KP-59 cells were treated and cultured the same way, they underwent similar morphological changes and produced insulin and glucagon. We used these systems to identify intracellular regulatory molecules involved in the conversion of pancreatic tumor cells into glucagon-producing cells. We found that the expression of antizyme 1 (AZ1), a negative regulator of ornithine decarboxylase, was increased and its localization was altered from the nucleus to the cytoplasm during AsPC-1 cell differentiation. Transient transfection of AsPC-1 cells with AZ1 siRNA resulted in inhibition of the morphological and functional cell differentiation as well as the specific suppression of AZ1 expression. By contrast, constitutive overexpression of AZ1 in AsPC-1 cells led to the enhancement of glucagon production. We also found that PANC-1 cells reduced the expression of glucagon mRNA when treated with AZ1 siRNA. These results suggested that AZ1 was necessary for the conversion of pancreatic tumor cells into glucagon-producing cells. Glucagon production in AsPC-1 cells was not affected by addition of putrescine, suggesting that the polyamines were not directly involved in the AZ1-mediated conversion of pancreatic tumor cells to differentiated state.

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Identification of Nuclear Export Signals in Antizyme-1

Cited by 38 publications

References 38 publications

Antizyme, a mediator of ubiquitin-independent proteasomal degradation and its inhibitor localize to centrosomes and modulate centriole amplification

Antizyme, a mediator of ubiquitin-independent proteasomal degradation and its inhibitor localize to centrosomes and modulate centriole amplification

A Novel CRM1-mediated Nuclear Export Signal Governs Nuclear Accumulation of Glyceraldehyde-3-phosphate Dehydrogenase following Genotoxic Stress

Antizyme is necessary for conversion of pancreatic tumor cells into glucagon-producing differentiated cells

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