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1. Pulsed force sequences for fast phase-insensitive quantum gates in trapped ions

Author

Steane, A M, Imreh, G, Home, J P, and Leibfried, D.

Subjects
Quantum Physics
Abstract

We show how to create quantum gates of arbitrary speed between trapped ions, using a laser walking wave, with complete insensitivity to drift of the optical phase, and requiring cooling only to the Lamb-Dicke regime. We present pulse sequences that satisfy the requirements and are easy to produce in the laboratory., Comment: 11 pages, 3 figures

Published
2013
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2. Experimental recovery of a qubit from partial collapse

Author

Sherman, J. A., Curtis, M. J., Szwer, D. J., Allcock, D. T. C., Imreh, G., Lucas, D. M., and Steane, A. M.

Subjects
Quantum Physics, Physics - Atomic Physics, Physics - Optics
Abstract

We describe and implement a method to restore the state of a single qubit, in principle perfectly, after it has partially collapsed. The method resembles the classical Hahn spin-echo, but works on a wider class of relaxation processes, in which the quantum state partially leaves the computational Hilbert space. It is not guaranteed to work every time, but successful outcomes are heralded. We demonstrate using a single trapped ion better performance from this recovery method than can be obtained employing projection and post-selection alone. The demonstration features a novel qubit implementation that permits both partial collapse and coherent manipulations with high fidelity., Comment: 5 pages, 3 figures

Published
2013
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3. Implementation of a symmetric surface electrode ion trap with field compensation using a modulated Raman effect

Author

Allcock, D. T. C., Sherman, J. A., Stacey, D. N., Burrell, A. H., Curtis, M. J., Imreh, G., Linke, N. M., Szwer, D. J., Webster, S. C., Steane, A. M., and Lucas, D. M.

Subjects
Quantum Physics, Physics - Atomic Physics
Abstract

We describe the fabrication and characterization of a new surface-electrode Paul ion trap designed for experiments in scalable quantum information processing with Ca+. A notable feature is a symmetric electrode pattern which allows rotation of the normal modes of ion motion, yielding efficient Doppler cooling with a single beam parallel to the planar surface. We propose and implement a technique for micromotion compensation in all directions using an infrared repumper laser beam directed into the trap plane. Finally, we employ an alternate repumping scheme that increases ion fluorescence and simplifies heating rate measurements obtained by time-resolved ion fluorescence during Doppler cooling., Comment: 9 pages, 14 figures; Rewritten section IB and added authors

Published
2009
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4. High-fidelity readout of trapped-ion qubits

Author

Myerson, A., Szwer, D., Webster, S., Allcock, D., Curtis, M., Imreh, G., Sherman, J., Stacey, D., Steane, A., and Lucas, D.

Subjects
Quantum Physics
Abstract

We demonstrate single-shot qubit readout with fidelity sufficient for fault-tolerant quantum computation, for two types of qubit stored in single trapped calcium ions. For an optical qubit stored in the (4S_1/2, 3D_5/2) levels of 40Ca+ we achieve 99.991(1)% average readout fidelity in one million trials, using time-resolved photon counting. An adaptive measurement technique allows 99.99% fidelity to be reached in 145us average detection time. For a hyperfine qubit stored in the long-lived 4S_1/2 (F=3, F=4) sub-levels of 43Ca+ we propose and implement a simple and robust optical pumping scheme to transfer the hyperfine qubit to the optical qubit, capable of a theoretical fidelity 99.95% in 10us. Experimentally we achieve 99.77(3)% net readout fidelity, inferring at least 99.87(4)% fidelity for the transfer operation., Comment: 4 pages, 3 figures; improved readout fidelity (numerical results changed)

Published
2008
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5. A long-lived memory qubit on a low-decoherence quantum bus

Author

Lucas, D. M., Keitch, B. C., Home, J. P., Imreh, G., McDonnell, M. J., Stacey, D. N., Szwer, D. J., and Steane, A. M.

Subjects
Quantum Physics
Abstract

We demonstrate long-lived coherence in internal hyperfine states of a single \Ca{43} trapped-ion qubit $[T_2=1.2(2)\s]$, and in external motional states of a single \Ca{40} trapped-ion qubit $[T_2'=0.18(4)\s]$, in the same apparatus. The motional decoherence rate is consistent with the heating rate, which was measured to be 3(1) quanta/sec. Long coherence times in the external motional states are essential for performing high-fidelity quantum logic gates between trapped-ion qubits. The internal-state $T_2$ time that we observe in \Ca{43}, which has not previously been used as a trapped-ion qubit, is about one thousand times longer than that of physical qubits based on \Ca{40} ions. Using a single spin-echo pulse to ``re-phase'' the internal state, we can detect no decoherence after 1\s, implying an effective coherence time $T_2^{\mbox{\tiny SE}} \gtish 45\s$. This compares with timescales in this trap for single-qubit operations of \ish 1\us, and for two-qubit operations of \ish 10\us., Comment: 4 pages, 4 figures

Published
2007

6. Long-lived mesoscopic entanglement outside the Lamb-Dicke regime

Author

McDonnell, M. J., Home, J. P., Lucas, D. M., Imreh, G., Keitch, B. C., Szwer, D. J., Thomas, N. R., Webster, S. C., Stacey, D. N., and Steane, A. M.

Subjects
Quantum Physics
Abstract

We create entangled states of the spin and motion of a single $^{40}$Ca$^+$ ion in a linear ion trap. The motional part consists of coherent states of large separation and long coherence time. The states are created by driving the motion using counterpropagating laser beams. We theoretically study and experimentally observe the behaviour outside the Lamb-Dicke regime, where the trajectory in phase space is modified and the coherent states become squeezed. We directly observe the modification of the return time of the trajectory, and infer the squeezing. The mesoscopic entanglement is observed up to $\Delta \alpha = 5.1$ with coherence time 170 microseconds and mean phonon excitation $\nbar = 16$., Comment: 5 pages, 3 figures. Revised version after editor comments

Published
2006
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7. Deterministic entanglement and tomography of ion spin qubits

Author

Home, J. P., McDonnell, M. J., Lucas, D. M., Imreh, G., Keitch, B. C., Szwer, D. J., Thomas, N. R., Webster, S. C., Stacey, D. N., and Steane, A. M.

Subjects
Quantum Physics
Abstract

We have implemented a universal quantum logic gate between qubits stored in the spin state of a pair of trapped calcium 40 ions. An initial product state was driven to a maximally entangled state deterministically, with 83% fidelity. We present a general approach to quantum state tomography which achieves good robustness to experimental noise and drift, and use it to measure the spin state of the ions. We find the entanglement of formation is 0.54., Comment: 3 figures, 4 pages, footnotes fixed

Published
2006
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9. Implementing segmented ion trap designs for quantum computing

Author

Imreh, G and Steane, A

Subjects
Quantum computer, Quantum computing, Atomic physics
Abstract

With all the key elements of quantum computing in ion traps demonstrated by the research community, the focus is now placed on building more sophisticated traps with larger numbers of ions to allow practical scale information processing. One promising avenue is to store ions in and shuttle them between many independent traps which serve as potential interaction sites. The core of the work described in this thesis is the experimental evaluation of a microfabricated segmented ion trap, built by Sandia National Laboratories ("Sandia trap"). These experiments required construction of a wholly new optical setup including laser and detection systems, a vacuum system and control electronics. Among our experimental achievements were: successful loading of single and pairs of ions in the microscale trap, measurement of ion storage lifetime, measurement of the motional heating rate with a time-resolved Doppler-cooling method — which showed above than average heating, and implemented a single-ion shuttling method — which reliably transferred the ion through a distance of 360 μm (two DC electrode widths away) and back. These results have been used to improve the next version of the Sandia trap design. We also used computer modelling to study several aspects of ion traps: a mesoscopic ion trap designed for fast ion separation, simulated ion loading to quantify requirements for successful trapping in small and shallow traps, and analyzed a precise shuttling method — where the time dependence of the trapping potential is engineered such that there is minimal motional heating. The results show that ion trap arrays at the 100 μm distance scale are feasible and suggests that such multiple trap designs merit further study.

Published
2018

11. Deterministic entanglement and tomography of trapped ion-spin qubits

Author

Home, Jonathan, McDonnell, M.J., Lucas, D.M., Imreh, G., Keitch, Ben C., Szwer, D.J., Thomas, Nathaniel R., Webster, Simon C., Stacey, Derek N., and Steane, Andrew M.

Subjects
Quantum Physics
Abstract

We have implemented a universal quantum logic gate between qubits stored in the spin state of a pair of trapped 40Ca ions. An initial product state was driven to a maximally entangled state deterministically, with 83% fidelity. We present a general approach to quantum state tomography which achieves good robustness to experimental noise and drift, and use it to measure the spin state of the ions. We find the entanglement of formation is 0.54., New Journal of Physics, 8, ISSN:1367-2630

Published
2006
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15. High-Fidelity Readout of Trapped-Ion Qubits

Author

Myerson, A. H., primary, Szwer, D. J., additional, Webster, S. C., additional, Allcock, D. T. C., additional, Curtis, M. J., additional, Imreh, G., additional, Sherman, J. A., additional, Stacey, D. N., additional, Steane, A. M., additional, and Lucas, D. M., additional

Published
2008
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19. Practicing Perfection: Piano Performance as Expert Memory.

Author

Chaffin, R. and Imreh, G.

Subjects
*MEMORY, *PIANO playing
Abstract

A concert pianist recorded her practice as she learned the third movement, Presto, of J.S. Bach's Italian Concerto. She also described the formal structure of the piece and reported her decisions about basic features (e.g., fingering), interpretive features (e.g., phrasing), and cues to attend to during performance (performance cues). These descriptions were used to identify which locations, features, and cues she practiced most, which caused hesitations when she first played from memory, and which affected her recall 2 years later. Effects of the formal structure and performance cues on all three activities indicated that the pianist used the formal structure as a retrieval scheme and performance cues as retrieval cues. Like expert memorists in other domains, she engaged in extended retrieval practice, going to great lengths to ensure that retrieval was as rapid and automatic from conceptual (declarative) memory as from motor and auditory memory. [ABSTRACT FROM AUTHOR]

Published
2002
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20. Zur Verbreitung des Strontiums in tertiären Kalken

Author

Imreh, J., Imreh, G., and Mihálka, St.

Abstract

The Sr-contents of some tertiary limestones in the northwestern part of Rumania are investigated. Samples were taken at different horizons of one and the same limestone layer. Thereby the geochemical distribution of Sr is determined in a vertical profile. Special reference is made to the relative abundance of Sr in the limestone outcrop of Cheia. The migration of Sr within the limestone strata is discussed.

Published
1965
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25. Improving light microscopy training routines with evidence-based education.

Author

Imreh G, Hu J, and Le Guyader S

Subjects
Humans, Research Personnel education, Reproducibility of Results, Teaching, Microscopy methods
Abstract

The low reproducibility of scientific data published in articles has recently become a cause of concern in many scientific fields. Data involving light microscopy is no exception. The low awareness of researchers of the technologies they use in their research has been identified as one of the main causes of the problem. Potential solutions have hinted at the need to improve technological and methodological education within research. Despite the pivotal role of microscopy core facilities in the education of researchers being well documented, facility staff (FS) often learn their trade on the job, without receiving themselves any structured education about the technology they teach others to use. Additionally, despite endorsing an important role at the highest level of education, most FS never receive any training in pedagogy, the field of research on teaching and learning methods. In this article, we argue that the low level of awareness that researchers have of microscopy stems from a knowledge gap formed between them and microscopy FS during training routines. On the one hand, FS consider that their teaching task is to explain what is needed to produce reliable data. On the other, despite understanding what is being taught, researchers fail to learn the most challenging aspects of microscopy, those involving their judgement and reasoning. We suggest that the misunderstanding between FS and researchers is due to FS not being educated in pedagogy and thus often confusing understanding and learning. To bridge this knowledge gap and improve the quality of the microscopy education available to researchers, we propose a paradigm shift where training staff at technological core facilities be acknowledged as full-fledged teachers and offered structured education not only in the technology they teach but also in pedagogy. We then suggest that training routines at facilities be upgraded to follow the principles of the Constructive Alignment pedagogical method. We give an example of how this can be applied to existing microscopy training routines. We also describe a model to define where the responsibility of FS in training researchers begins and ends. This involves a major structural change where university staff involved in teaching research technologies themselves receive appropriate education. For this to be achieved, we advocate that funding agencies, universities, microscopy and core facility organisations mobilise resources of time and funding. Such changes may involve funding the creation and development of 'Train-the-trainer' type of courses and giving incentives for FS to upgrade their technological and pedagogical knowledge, for example by including them in career paths. We believe that this paradigm shift is necessary to improve the level of microscopy education and ultimately the reproducibility of published data., (© 2023 The Authors. Journal of Microscopy published by John Wiley & Sons Ltd on behalf of Royal Microscopical Society.)

Published
2024
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27. An overview of the National COVID-19 Chest Imaging Database: data quality and cohort analysis.

Author

Cushnan D, Bennett O, Berka R, Bertolli O, Chopra A, Dorgham S, Favaro A, Ganepola T, Halling-Brown M, Imreh G, Jacob J, Jefferson E, Lemarchand F, Schofield D, and Wyatt JC

Subjects
Cohort Studies, Data Accuracy, Humans, Pandemics, SARS-CoV-2, Tomography, X-Ray Computed, COVID-19
Abstract

Background: The National COVID-19 Chest Imaging Database (NCCID) is a centralized database containing mainly chest X-rays and computed tomography scans from patients across the UK. The objective of the initiative is to support a better understanding of the coronavirus SARS-CoV-2 disease (COVID-19) and the development of machine learning technologies that will improve care for patients hospitalized with a severe COVID-19 infection. This article introduces the training dataset, including a snapshot analysis covering the completeness of clinical data, and availability of image data for the various use-cases (diagnosis, prognosis, longitudinal risk). An additional cohort analysis measures how well the NCCID represents the wider COVID-19-affected UK population in terms of geographic, demographic, and temporal coverage., Findings: The NCCID offers high-quality DICOM images acquired across a variety of imaging machinery; multiple time points including historical images are available for a subset of patients. This volume and variety make the database well suited to development of diagnostic/prognostic models for COVID-associated respiratory conditions. Historical images and clinical data may aid long-term risk stratification, particularly as availability of comorbidity data increases through linkage to other resources. The cohort analysis revealed good alignment to general UK COVID-19 statistics for some categories, e.g., sex, whilst identifying areas for improvements to data collection methods, particularly geographic coverage., Conclusion: The NCCID is a growing resource that provides researchers with a large, high-quality database that can be leveraged both to support the response to the COVID-19 pandemic and as a test bed for building clinically viable medical imaging models., (© The Author(s) 2021. Published by Oxford University Press GigaScience.)

Published
2021
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28. Towards nationally curated data archives for clinical radiology image analysis at scale: Learnings from national data collection in response to a pandemic.

Author

Cushnan D, Berka R, Bertolli O, Williams P, Schofield D, Joshi I, Favaro A, Halling-Brown M, Imreh G, Jefferson E, Sebire NJ, Reilly G, Rodrigues JCL, Robinson G, Copley S, Malik R, Bloomfield C, Gleeson F, Crotty M, Denton E, Dickson J, Leeming G, Hardwick HE, Baillie K, Openshaw PJ, Semple MG, Rubin C, Howlett A, Rockall AG, Bhayat A, Fascia D, Sudlow C, and Jacob J

Abstract

The prevalence of the coronavirus SARS-CoV-2 disease has resulted in the unprecedented collection of health data to support research. Historically, coordinating the collation of such datasets on a national scale has been challenging to execute for several reasons, including issues with data privacy, the lack of data reporting standards, interoperable technologies, and distribution methods. The coronavirus SARS-CoV-2 disease pandemic has highlighted the importance of collaboration between government bodies, healthcare institutions, academic researchers and commercial companies in overcoming these issues during times of urgency. The National COVID-19 Chest Imaging Database, led by NHSX, British Society of Thoracic Imaging, Royal Surrey NHS Foundation Trust and Faculty, is an example of such a national initiative. Here, we summarise the experiences and challenges of setting up the National COVID-19 Chest Imaging Database, and the implications for future ambitions of national data curation in medical imaging to advance the safe adoption of artificial intelligence in healthcare., (© The Author(s) 2021.)

Published
2021
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29. Involvement of autophagy in the outcome of mitotic catastrophe.

Author

Sorokina IV, Denisenko TV, Imreh G, Tyurin-Kuzmin PA, Kaminskyy VO, Gogvadze V, and Zhivotovsky B

Subjects
Apoptosis, Carcinoma, Non-Small-Cell Lung physiopathology, Cell Death physiology, Cell Line, Tumor, Colorectal Neoplasms physiopathology, HCT116 Cells, Humans, Lung Neoplasms physiopathology, Myeloid Cell Leukemia Sequence 1 Protein metabolism, bcl-X Protein metabolism, Autophagy physiology, Mitosis
Abstract

Evading cell death is a major driving force for tumor progression that is one of the main problems in current cancer research. Mitotic catastrophe (MC) represents attractive platform compromising tumor resistance to current therapeutic modalities. MC appeared as onco-suppressive mechanism and is defined as a stage driving the cell to an irreversible destiny, i.e. cell death via apoptosis or necrosis. Our study highlights that MC induction in colorectal carcinoma cell lines ultimately leads to the autophagy followed by apoptosis. We show that autophagy suppression in Atg 13 knockout non-small cell lung carcinoma cells lead to the dramatic decrease of MC rate. Furthermore, mitochondria-linked anti-apoptotic proteins Mcl-1 and Bcl-xL play a crucial role in the duration of MC and a cross-talk between autophagy and apoptosis. Thus, the suppression of apoptosis by overexpression of Mcl-1 or Bcl-xL affected MC and lead to a significant induction of autophagy in HCT116 wt and HCT116 14-3-3σ -/- cells. Our data demonstrate that MC induction is a critical stage, in which a cell decides how to die, while mitochondria are responsible for the maintaining the balance between MC - autophagy - apoptosis.

Published
2017
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31. Molecular basis for the dual subcellular distribution of microsomal glutathione transferase 1.

Author

Shimoji M, Figueroa RA, Neve E, Maksel D, Imreh G, Morgenstern R, and Hallberg E

Subjects
Amino Acid Sequence, Animals, COS Cells, Cell Line, Chlorocebus aethiops, Endoplasmic Reticulum metabolism, Mitochondria metabolism, Mitochondrial Membranes metabolism, Oxidative Stress physiology, Glutathione Transferase metabolism, Microsomes, Liver metabolism
Abstract

Microsomal glutathione transferase 1 (MGST1) is a membrane bound enzyme involved in the detoxification of reactive electrophiles and protection of membranes from oxidative stress. The enzyme displays an unusual and broad subcellular distribution with especially high levels in the endoplasmic reticulum (ER) and outer mitochondrial membrane (OMM). Here we examined the molecular basis for this dual distribution. We hypothesized that the amphipathic properties of the first transmembrane segment (TMS), that contains a positively charged lysine (K25), is a central feature guiding dual targeting. The lysine-25 was substituted to alanine by site directed mutagenesis. We also increased the amphipathic character of the helix by inserting an additional lysine either one turn above or below K25. Expressing these constructs in simian COS cells, and analyzing subcellular distribution by immunocytochemistry, we observed an increased ER targeting of K25A-MGST1. In contrast I22K-MGST1 and F28K-MGST1 displayed pronounced mitochondrial targeting. By using in vitro transcription-translation we examined whether insertion of WT-MGST1 into ER is co- or post-translational and provide evidence for the former. In the same experimental set-up, mitochondrial insertion was shown to depend on the positive charge. Together these results show that removing the positive charge of lysine-25 promotes ER incorporation, but counteracts mitochondrial insertion. In contrast, introducing an extra lysine in the first TMS of MGST1 had opposite effects. The amphipathic character of the first TMS thus constitutes a molecular determinant for the dual targeting of MGST1. Broad subcellular distribution is consistent with a physiological role in protection from reactive intermediates and oxidative stress., (Copyright © 2016 Elsevier B.V. All rights reserved.)

Published
2017
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32. Reactive oxygen species regulate a balance between mitotic catastrophe and apoptosis.

Author

Sorokina IV, Denisenko TV, Imreh G, Gogvadze V, and Zhivotovsky B

Subjects
Doxorubicin pharmacology, HCT116 Cells, Humans, Mitochondria drug effects, Mitochondria metabolism, Apoptosis drug effects, Mitosis drug effects, Reactive Oxygen Species metabolism
Abstract

Mitotic catastrophe (MC) is a sequence of events resulting from premature or inappropriate entry of cells into mitosis that can be caused by chemical or physical stresses. There are several observations permitting to define MC as an oncosuppressive mechanism. MC can end up in apoptosis, necrosis or senescence. Here we show that the anticancer drug doxorubicin triggers DNA damage and MC independently of ROS production. In contrast, doxorubicin-induced apoptosis was found to be ROS-dependent. Antioxidants NAC or Trolox suppressed apoptosis, but facilitated MC development. Our data demonstrate that evasion of apoptosis and subsequent stimulation of MC can contribute to tumor cell elimination improving anticancer therapy., (Copyright © 2016 Elsevier Ltd. All rights reserved.)

Published
2016
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34. The scaffold protein WRAP53β orchestrates the ubiquitin response critical for DNA double-strand break repair.

Author

Henriksson S, Rassoolzadeh H, Hedström E, Coucoravas C, Julner A, Goldstein M, Imreh G, Zhivotovsky B, Kastan MB, Helleday T, and Farnebo M

Subjects
Adaptor Proteins, Signal Transducing, Ataxia Telangiectasia Mutated Proteins metabolism, Cell Cycle Proteins, Cell Line, Tumor, Cells, Cultured, DNA Breaks, Double-Stranded, DNA Repair genetics, DNA-Binding Proteins metabolism, HeLa Cells, Histones metabolism, Humans, Molecular Chaperones, Nuclear Proteins metabolism, Phosphorylation, Protein Binding, Protein Structure, Tertiary, Telomerase genetics, Trans-Activators metabolism, Ubiquitin-Protein Ligases, DNA Repair physiology, Telomerase metabolism, Ubiquitin metabolism
Abstract

The WD40 domain-containing protein WRAP53β (WD40 encoding RNA antisense to p53; also referred to as WDR79/TCAB1) controls trafficking of splicing factors and the telomerase enzyme to Cajal bodies, and its functional loss has been linked to carcinogenesis, premature aging, and neurodegeneration. Here, we identify WRAP53β as an essential regulator of DNA double-strand break (DSB) repair. WRAP53β rapidly localizes to DSBs in an ATM-, H2AX-, and MDC1-dependent manner. We show that WRAP53β targets the E3 ligase RNF8 to DNA lesions by facilitating the interaction between RNF8 and its upstream partner, MDC1, in response to DNA damage. Simultaneous binding of MDC1 and RNF8 to the highly conserved WD40 scaffold domain of WRAP53β facilitates their interaction and accumulation of RNF8 at DSBs. In this manner, WRAP53β controls proper ubiquitylation at DNA damage sites and the downstream assembly of 53BP1, BRCA1, and RAD51. Furthermore, we reveal that knockdown of WRAP53β impairs DSB repair by both homologous recombination (HR) and nonhomologous end-joining (NHEJ), causes accumulation of spontaneous DNA breaks, and delays recovery from radiation-induced cell cycle arrest. Our findings establish WRAP53β as a novel regulator of DSB repair by providing a scaffold for DNA repair factors., (© 2014 Henriksson et al.; Published by Cold Spring Harbor Laboratory Press.)

Published
2014
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35. Chromosomal breaks during mitotic catastrophe trigger γH2AX-ATM-p53-mediated apoptosis.

Author

Imreh G, Norberg HV, Imreh S, and Zhivotovsky B

Subjects
14-3-3 Proteins deficiency, 14-3-3 Proteins genetics, Ataxia Telangiectasia Mutated Proteins, Biomarkers, Tumor deficiency, Biomarkers, Tumor genetics, Caspases metabolism, Cell Cycle Proteins genetics, Chromatids drug effects, Chromatids genetics, Chromosome Aberrations chemically induced, DNA Damage, DNA-Binding Proteins genetics, Doxorubicin pharmacology, Exonucleases deficiency, Exonucleases genetics, Exoribonucleases, G1 Phase genetics, Gene Knockout Techniques, Genomic Instability, HCT116 Cells, Histones genetics, Humans, Phosphorylation, Protein Serine-Threonine Kinases genetics, S Phase genetics, Signal Transduction, Tumor Suppressor Protein p53 genetics, Tumor Suppressor Proteins genetics, Apoptosis genetics, Cell Cycle Proteins metabolism, Chromosome Breakage, DNA-Binding Proteins metabolism, Histones metabolism, Mitosis genetics, Protein Serine-Threonine Kinases metabolism, Tumor Suppressor Protein p53 metabolism, Tumor Suppressor Proteins metabolism
Abstract

Although the cause and outcome of mitotic catastrophe (MC) has been thoroughly investigated, precisely how the ensuing lethality is regulated during or following this process and what signals are involved remain unknown. Moreover, the mechanism of the decision of cell death modalities following MC is still not well characterised. We demonstrate here a crucial role of the γH2AX-ATM-p53 pathway in the regulation of the apoptotic outcome of MC resulting from cells entering mitosis with damaged DNA. In addition to p53 deficiency, the depletion of ATM (ataxia telangiectasia mutated), but not ATR (ataxia telangiectasia and Rad3-related protein), protected against apoptosis and shifted cell death towards necrosis. Activation of this pathway is triggered by the augmented chromosomal damage acquired during anaphase in doxorubicin-treated cells lacking 14-3-3σ (also known as epithelial cell marker protein-1 or stratifin). Moreover, cells that enter mitosis with damaged DNA encounter segregation problems because of their abnormal chromosomes, leading to defects in mitotic exit, and they therefore accumulate in G1 phase. These multi- or micronucleated cells are prevented from cycling again in a p53- and p21-dependent manner, and subsequently die. Because increased chromosomal damage resulting in extensive H2AX phosphorylation appears to be a direct cause of catastrophic mitosis, our results describe a mechanism that involves generation of additional DNA damage during MC to eliminate chromosomally unstable cells.

Published
2011
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36. Transthyretin constitutes a functional component in pancreatic beta-cell stimulus-secretion coupling.

Author

Refai E, Dekki N, Yang SN, Imreh G, Cabrera O, Yu L, Yang G, Norgren S, Rössner SM, Inverardi L, Ricordi C, Olivecrona G, Andersson M, Jörnvall H, Berggren PO, and Juntti-Berggren L

Subjects
Animals, Calcium physiology, Glucose physiology, Humans, Membrane Potentials physiology, Mice, Mice, Obese, Patch-Clamp Techniques, Potassium Chloride, Insulin-Secreting Cells physiology, Prealbumin physiology
Abstract

Transthyretin (TTR) is a transport protein for thyroxine and, in association with retinol-binding protein, for retinol, mainly existing as a tetramer in vivo. We now demonstrate that TTR tetramer has a positive role in pancreatic beta-cell stimulus-secretion coupling. TTR promoted glucose-induced increases in cytoplasmic free Ca(2+) concentration ([Ca(2+)](i)) and insulin release. This resulted from a direct effect on glucose-induced electrical activity and voltage-gated Ca(2+) channels. TTR also protected against beta-cell apoptosis. The concentration of TTR tetramer was decreased, whereas that of a monomeric form was increased in sera from patients with type 1 diabetes. The monomer was without effect on glucose-induced insulin release and apoptosis. Thus, TTR tetramer constitutes a component in normal beta-cell function. Conversion of TTR tetramer to monomer may be involved in the development of beta-cell failure/destruction in type 1 diabetes.

Published
2005
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37. Apolipoprotein CIII promotes Ca2+-dependent beta cell death in type 1 diabetes.

Author

Juntti-Berggren L, Refai E, Appelskog I, Andersson M, Imreh G, Dekki N, Uhles S, Yu L, Griffiths WJ, Zaitsev S, Leibiger I, Yang SN, Olivecrona G, Jörnvall H, and Berggren PO

Subjects
Adult, Animals, Apolipoprotein C-III, Calcium Channels, L-Type physiology, Diabetes Mellitus, Type 1 blood, Female, Humans, Male, Mice, Apolipoproteins C physiology, Apoptosis, Calcium physiology, Diabetes Mellitus, Type 1 pathology, Islets of Langerhans pathology
Abstract

In type 1 diabetes (T1D), there is a specific destruction of the insulin secreting pancreatic beta cell. Although the exact molecular mechanisms underlying beta cell destruction are not known, sera from T1D patients have been shown to promote Ca(2+)-induced apoptosis. We now demonstrate that apolipoprotein CIII (apoCIII) is increased in serum from T1D patients and that this serum factor both induces increased cytoplasmic free intracellular Ca(2+) concentration ([Ca(2+)](i)) and beta cell death. The apoCIII-induced increase in [Ca(2+)](i) reflects an activation of the voltage-gated L-type Ca(2+) channel. Both the effects of T1D sera and apoCIII on the beta cell are abolished in the presence of antibody against apoCIII. Increased serum levels of apoCIII can thus account for the increase in beta cell [Ca(2+)](i) and thereby beta cell apoptosis associated with T1D.

Published
2004
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38. On-line monitoring of apoptosis in insulin-secreting cells.

Author

Köhler M, Zaitsev SV, Zaitseva II, Leibiger B, Leibiger IB, Turunen M, Kapelioukh IL, Bakkman L, Appelskog IB, de Monvel JB, Imreh G, and Berggren PO

Subjects
Animals, Bacterial Proteins, Caspase 3, Caspases metabolism, Cells, Cultured, Enzyme Precursors metabolism, Fluorescence Resonance Energy Transfer, Fluorometry, Green Fluorescent Proteins, Indicators and Reagents, Insulin Secretion, Luminescent Proteins, Mice, Microscopy, Confocal, Obesity genetics, Obesity metabolism, Photons, Apoptosis, Insulin metabolism, Internet, Islets of Langerhans metabolism, Monitoring, Physiologic, Obesity physiopathology
Abstract

Apoptosis was monitored in intact insulin-producing cells both with microfluorometry and with two-photon laser scanning microscopy (TPLSM), using a fluorescent protein based on fluorescence resonance energy transfer (FRET). TPLSM offers three-dimensional spatial information that can be obtained relatively deep in tissues. This provides a potential for future in vivo studies of apoptosis. The cells expressed a fluorescent protein (C-DEVD-Y) consisting of two fluorophores, enhanced cyan fluorescent protein (ECFP) and enhanced yellow fluorescent protein (EYFP), linked by the amino acid sequence DEVD selectively cleaved by caspase-3-like proteases. FRET between ECFP and EYFP in C-DEVD-Y could therefore be monitored on-line as a sensor of caspase-3 activation. The relevance of using caspase-3 activation to indicate beta-cell apoptosis was demonstrated by inhibiting caspase-3-like proteases with Z-DEVD-fmk and thereby showing that caspase-3 activation was needed for high-glucose-and cytokine-induced apoptosis in the beta-cell and for staurosporine-induced apoptosis in RINm5F cells. In intact RINm5F cells expressing C-DEVD-Y and in MIN6 cells expressing the variant C-DEVD-Y2, FRET was lost at 155 +/- 23 min (n = 9) and 257 +/- 59 min (n = 4; mean +/- SE) after activation of apoptosis with staurosporine (6 micromol/l), showing that this method worked in insulin-producing cells.

Published
2003
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41. Sequential degradation of proteins from the nuclear envelope during apoptosis.

Author

Kihlmark M, Imreh G, and Hallberg E

Subjects
Animals, Apoptosis radiation effects, Cells, Cultured, Enzyme Inhibitors pharmacology, Fluorescent Dyes metabolism, Green Fluorescent Proteins, Hepatocytes cytology, Hepatocytes drug effects, Hepatocytes physiology, Lamin Type B, Lamins, Luminescent Proteins metabolism, Microscopy, Confocal, Rats, Rats, Inbred BUF, Recombinant Fusion Proteins metabolism, Staurosporine pharmacology, Transfection, Tumor Cells, Cultured, Apoptosis physiology, Membrane Proteins metabolism, Nuclear Envelope metabolism, Nuclear Pore Complex Proteins metabolism, Nuclear Proteins metabolism
Abstract

We have produced new antibodies specific for the integral pore membrane protein POM121. Using these antibodies we show that during apoptosis POM121 becomes proteolytically degraded in a caspase-dependent manner. The POM121 antibodies and antibodies specific for other proteins of the nuclear envelope were used in a comparative study of nuclear apoptosis in staurosporine-treated buffalo rat liver cells. Nuclei from these cells were classified in three different stages of apoptotic progression: stage I, moderately condensed chromatin surrounded by a smooth nuclear periphery; stage II, compact patches of condensed chromatin collapsing against a smooth nuclear periphery; stage III, round compact chromatin bodies surrounded by grape-shaped nuclear periphery. We have performed double labeling immunofluorescence microscopy of individual apoptotic cells and quantitative immunoblotting analysis of total proteins from apoptotic cell cultures. The results showed that degradation of nuclear envelope marker proteins occurred in a specific order. POM121 degradation occurred surprisingly early and was initiated before nucleosomal DNA degradation could be detected using TUNEL assay and completed before clustering of the nuclear pores. POM121 was eliminated significantly more rapid compared with NUP153 (a peripheral protein located in the nucleoplasmic basket of the nuclear pore complex) and lamin B (a component of the nuclear lamina). Disappearance of NUP153 and lamin B was coincident with onset of DNA fragmentation and clustering of nuclear pores. By contrast, the peripheral NPC protein p62 was degraded much later. The results suggest that degradation of POM121 may be an important early step in propagation of nuclear apoptosis.

Published
2001
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42. Nuclear pore complexes form immobile networks and have a very low turnover in live mammalian cells.

Author

Daigle N, Beaudouin J, Hartnell L, Imreh G, Hallberg E, Lippincott-Schwartz J, and Ellenberg J

Subjects
Animals, COS Cells, Cells, Cultured, DNA metabolism, Green Fluorescent Proteins, HeLa Cells, Humans, Lamins, Luminescent Proteins metabolism, Membrane Proteins metabolism, Microscopy, Confocal, Microscopy, Electron, Microscopy, Fluorescence, Mitosis, Protein Binding, Rats, Recombinant Fusion Proteins metabolism, Time Factors, Xenopus, Lamin Type B, Nuclear Pore chemistry, Nuclear Pore metabolism, Nuclear Pore Complex Proteins, Nuclear Proteins metabolism
Abstract

The nuclear pore complex (NPC) and its relationship to the nuclear envelope (NE) was characterized in living cells using POM121-green fluorescent protein (GFP) and GFP-Nup153, and GFP-lamin B1. No independent movement of single pore complexes was found within the plane of the NE in interphase. Only large arrays of NPCs moved slowly and synchronously during global changes in nuclear shape, strongly suggesting mechanical connections which form an NPC network. The nuclear lamina exhibited identical movements. NPC turnover measured by fluorescence recovery after photobleaching of POM121 was less than once per cell cycle. Nup153 association with NPCs was dynamic and turnover of this nucleoporin was three orders of magnitude faster. Overexpression of both nucleoporins induced the formation of annulate lamellae (AL) in the endoplasmic reticulum (ER). Turnover of AL pore complexes was much higher than in the NE (once every 2.5 min). During mitosis, POM121 and Nup153 were completely dispersed and mobile in the ER (POM121) or cytosol (Nup153) in metaphase, and rapidly redistributed to an immobilized pool around chromatin in late anaphase. Assembly and immobilization of both nucleoporins occurred before detectable recruitment of lamin B1, which is thus unlikely to mediate initiation of NPC assembly at the end of mitosis.

Published
2001
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43. An integral membrane protein from the nuclear pore complex is also present in the annulate lamellae: implications for annulate lamella formation.

Author

Imreh G and Hallberg E

Subjects
Animals, Antibodies, Antineoplastic Agents, Phytogenic pharmacology, COS Cells, Cricetinae, Cytoplasm ultrastructure, Gene Expression drug effects, Gene Expression physiology, Genes, Reporter, Green Fluorescent Proteins, Indicators and Reagents metabolism, Kidney cytology, Luminescent Proteins genetics, Membrane Proteins analysis, Membrane Proteins immunology, Membrane Proteins physiology, Plasmids, Transfection, Vinblastine pharmacology, Cytoplasm chemistry, Cytoplasm physiology, Membrane Proteins genetics, Nuclear Envelope chemistry, Nuclear Envelope physiology, Nuclear Proteins
Abstract

Annulate lamellae (AL) are cytoplasmic arrays of stacked membrane cisternae containing densely packed pore complexes which are similar in structure to the nuclear pore complexes (NPCs) and thus referred to as annulate lamella pore complexes (ALPCs). We have recently shown that the integral nuclear pore membrane protein POM121 tagged with green fluorescent protein was correctly targeted to the nuclear pores (H. Söderqvist et al., 1997, Eur. J. Biochem. 250, 808-813). Here we have investigated if POM121 fused to three tandem molecules of yellow fluorescent protein (YFP) (POM121-YFP(3)) also was able to distribute in the extensive and well-characterized AL of RC37 and BMGE cells. Transfected RC37 or BMGE cells displayed YFP fluorescence around the nuclear envelope, as well as in the cytoplasmic AL structures. The YFP fluorescence colocalized perfectly with immunostaining using antibodies specific for different NPC proteins. The AL of both transfected and untransfected BMGE cells resisted extractions with Tx-100 and 250 mM NaCl, but were completely solubilized at 450 mM NaCl. Loss of YFP fluorescence and immunostaining for other NPC proteins correlated under all extraction conditions tested, suggesting that overexpressed POM121-YFP(3) had become an integrated part both of the NPCs and of the ALPCs. Furthermore, we have generated a stable BHK cell line expressing POM121-YFP(3) located exclusively at the nuclear pores. Treatment with vinblastine sulfate, which induces formation of AL in a variety of cells, resulted in distribution of POM121-YFP(3) into cytoplasmic foci colocalizing with immunostaining for peripheral NPC proteins. Taken together, the results show that YFP-tagged POM121 is able to distribute in drug-induced or naturally occurring AL, suggesting that POM121 is a natural constituent of ALPCs. In COS cells, which normally lack or have very little AL, YFP-tagged POM121 distributed in the nuclear pores when expressed at low levels. However, at high expression levels the YFP fluorescence also distributed in a number of brightly fluorescing cytoplasmic dots or foci, which were not present in untransfected cells. This was also true for untagged POM121. The cytoplasmic foci varied in size from 0. 1 to 2 microm and were distinctly located in the immediate vicinity of ER cisternae (without colocalizing) and also contained other nuclear pore proteins, indicating that they may represent cytoplasmic AL. This idea is supported by time-lapse studies of postmitotic assembly of these structures. This raises the question of the role of POM121 in ALPC and NPC biogenesis., (Copyright 2000 Academic Press.)

Published
2000
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45. Noninvasive monitoring of apoptosis versus necrosis in a neuroblastoma cell line expressing a nuclear pore protein tagged with the green fluorescent protein.

Author

Imreh G, Beckman M, Iverfeldt K, and Hallberg E

Subjects
Benzoquinones pharmacology, Biomarkers, Chromatin, Green Fluorescent Proteins, Humans, Luminescent Proteins genetics, Nuclear Envelope chemistry, Recombinant Fusion Proteins analysis, Staurosporine pharmacology, Transfection, Tumor Cells, Cultured, Apoptosis, DNA Fragmentation, Luminescent Proteins analysis, Membrane Proteins genetics, Necrosis, Neuroblastoma pathology, Nuclear Proteins
Abstract

A fusion chimera between the integral nuclear pore membrane protein POM121 and GFP (green fluorescent protein) has been shown to correctly target to the nuclear pores when transiently expressed in a number of mammalian cell types. POM121-GFP is therefore an excellent marker for the noninvasive studies of the nuclear pores in living cells using fluorescence microscopy. We have established a line of neuroblastoma cells stably expressing the POM121-GFP fusion protein. We also monitored the nuclear envelope in living cells after induction of apoptosis or necrosis using 1 microM staurosporine or 100 microM p-benzoquinone, respectively. Interestingly, the POM121-GFP fluorescence was weaker or missing in the apoptotic cells. The disappearance of the nuclear pore marker accompanied apoptotic progression as judged by the degree of chromatin condensation and DNA fragmentation as analyzed by DNA staining and TUNEL assay, respectively. In contrast, the intensity of the nuclear rim fluorescence was unaffected in necrotic cells displaying an abnormal morphology with tilted nuclei. Thus, it was possible to distinguish between apoptotic and necrotic development in living cells using fluorescence microscopy. This cell line provides a fast and convenient model for screening suspected toxic xenobiotics., (Copyright 1998 Academic Press.)

Published
1998
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46. Intracellular distribution of an integral nuclear pore membrane protein fused to green fluorescent protein--localization of a targeting domain.

Author

Söderqvist H, Imreh G, Kihlmark M, Linnman C, Ringertz N, and Hallberg E

Subjects
Animals, Blotting, Western, CHO Cells, Cricetinae, Green Fluorescent Proteins, Immunohistochemistry, Luminescent Proteins genetics, Membrane Proteins chemistry, Membrane Proteins genetics, Microscopy, Fluorescence, Nuclear Proteins analysis, Peptide Fragments analysis, Recombinant Fusion Proteins analysis, Recombinant Fusion Proteins genetics, Transfection genetics, Tumor Cells, Cultured, Luminescent Proteins analysis, Membrane Proteins analysis
Abstract

The 121-kDa pore membrane protein (POM121) is a bitopic integral membrane protein specifically located in the pore membrane domain of the nuclear envelope with its short N-terminal tail exposed on the luminal side and its major C-terminal portion adjoining the nuclear pore complex. In order to locate a signal for targeting of POM121 to the nuclear pores, we overexpressed selected regions of POM121 alone or fused to the green fluorescent protein (GFP) in transiently transfected COS-1 cells or in a stably transfected neuroblastoma cell line. Microscopic analysis of the GFP fluorescence or immunostaining was used to determine the intracellular distribution of the overexpressed proteins. The endofluorescent GFP tag had no effect on the distribution of POM121, since the chimerical POM121-GFP fusion protein was correctly targeted to the nuclear pores of both COS-1 cells and neuroblastoma cells. Based on the differentiated intracellular sorting of the POM121 variants, we conclude that the first 128 amino acids of POM121 contains signals for targeting to the continuous endoplasmic reticulum/nuclear envelope membrane system but not specifically to the nuclear pores and that a specific nuclear pore targeting signal is located between amino acids 129 and 618 in the endoplasmically exposed portion of POM121.

Published
1997
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