Identification of Apoptosis-associated Proteins in a Human Burkitt Lymphoma Cell Line

Brockstedt, Ekkehard; Rickers, Anke; Kostka, Susanne; Laubersheimer, Andreas; Dörken, Bernd; Wittmann‐Liebold, Brigitte; Bommert, Kurt; Otto, Albrecht

doi:10.1074/jbc.273.43.28057

Cited by 173 publications

(130 citation statements)

References 44 publications

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“…On the ground of the SRB assay results, IC 50 values of 0.5 and 0.3 lM were determined for auranofin on the sensitive and resistant cell lines, respectively, after 72-h drug exposure. In turn, the measured IC 50 values for Auoxo6 were found to be perfectly consistent with those previously reported by Casini et al [5] (1.8 and 4.9 lM for A2780/S and A2780/R, respectively). We also observed that very limited cell death was evident, for both compounds, at 24 h, this rendering a classic proteomic approach well feasible.…”

Section: Resultssupporting

confidence: 91%

“…At the time point of the Auoxo6 and auranofin treatments studied, no increased apoptosis was observed. We observed that apoptosis occurs at a later time point and that the increase of heterogeneous nuclear ribonucleoprotein H levels just precedes this process [50].…”

Section: Functional Roles Of the Identified Proteinsmentioning

confidence: 65%

“…Briefly, the cells were seeded in tissue-culture plates at 5 9 10 4 cells/mL (total volume 30 mL) and incubated overnight, then exposed to concentrations of the study compounds equal to 72-h-exposure IC 50 values for 24 h. At the end of the incubation the cells were washed with phosphate-buffered saline, then were scraped in RIPA buffer [50 mM Tris-HCl pH 7.0, 1% NP-40, 150 mM NaCl, 2 mM ethylene glycol bis(2-aminoethyl ether)tetraacetic acid, 100 mM NaF] containing a cocktail of protease inhibitors (Sigma). The cells were sonicated (10 s) and protein extracts were clarified by centrifugation at 8,000g for 10 min.…”

Section: Sample Preparation and 2d Gel Electrophoresismentioning

confidence: 99%

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Exploring the biochemical mechanisms of cytotoxic gold compounds: a proteomic study

et al. 2010

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We have recently shown that a group of structurally diverse gold compounds are highly cytotoxic toward a panel of 36 human tumor cell lines through a variety of biochemical mechanisms. A classic proteomic approach is exploited here to gain deeper insight into those mechanisms. This investigation is focused on Auoxo6, a novel binuclear gold(III) complex, and auranofin, a clinically established gold(I) antiarthritic drug. First, the 72-h cytotoxicity profiles of Auoxo6 and auranofin were determined against A2780 human ovarian carcinoma cells. Subsequently, protein extraction from gold-treated A2780 cells sensitive to cisplatin and 2D gel electrophoresis separation were carried out according to established procedures. Notably, both metallodrugs caused relatively modest changes in protein expression in comparison with controls as only 11 out of approximately 1,300 monitored spots showed appreciable quantitative changes. Very remarkably, six altered proteins were in common between the two treatments. Eight altered proteins were identified by mass spectrometry; among them was ezrin, a protein associated with the cytoskeleton and involved in apoptosis. Interestingly, two altered proteins, i.e., peroxiredoxins 1 and 6, are known to play crucial roles in the cell redox metabolism. Increased cleavage of heterogeneous ribonucleoprotein H was also evidenced, consistent with caspase 3 activation. Overall, the results of the present proteomic study point out that the mode of action of Auoxo6 is strictly related to that of auranofin, that the induced changes in protein expression are limited and selective, that both gold compounds trigger caspase 3 activation and apoptosis, and that a few affected proteins are primarily involved in cell redox homeostasis.

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Section: Resultssupporting

confidence: 91%

Section: Functional Roles Of the Identified Proteinsmentioning

confidence: 65%

Section: Sample Preparation and 2d Gel Electrophoresismentioning

confidence: 99%

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Exploring the biochemical mechanisms of cytotoxic gold compounds: a proteomic study

et al. 2010

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“…Moreover, the modified S19 serves as a chemoattractant specific for macrophages (12). Two more reports suggest the structural modification of ribosomes during apoptosis: cleavage or at least modification of the 60S ribosome subunit protein PO (15) and destruction of polysomes (1). These findings indicate that ribosomal proteins and the ribosome complex are structurally modified in apoptotic cells, and suggest that some ribosomal proteins have extra-ribosomal functions.…”

mentioning

confidence: 95%

Structural Change of Ribosomes during Apoptosis: Degradation and Externalization of Ribosomal Proteins in Doxorubicin-Treated Jurkat Cells

Nishida

Shiratsuchi

Nadano

et al. 2002

Journal of Biochemistry

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Changes in the amount and localization of human ribosomal proteins during apoptosis were determined. When total lysates of Jurkat cells undergoing apoptosis induced by doxorubicin were analyzed by Western blotting, degradation of three ribosomal proteins, S18, L5, and L14, was detected at 48 h after the induction of apoptosis. Decreases in the amounts of these three ribosomal proteins were also observed in ribosome-enriched fractions. These changes were partly abolished by the addition of the pan-caspase inhibitor z-VAD-fmk. Moreover, formation of the 80S ribosome complex appeared to be inhibited at 48 h after apoptosis induction. On the other hand, the rate of protein synthesis, assessed by measuring the incorporation of [ 38 S]Met into bulk proteins, decreased as early as 12 h after the addition of doxorubicin. These results indicate that changes in the amount of ribosomal proteins and the overall structure of ribosomes in apoptosing cells occur after protein synthesis declines. Finally, analyses by flow cytometry, immunofluorescence, and Western blotting showed that six ribosomal proteins, S15, PO, L5, L6, L36a, and L41, were relocalized and expressed at the cell surface during apoptosis. The above results collectively indicate that ribosomes are structurally altered in apoptotic cells following inactivation of protein synthesis.Key words: apoptosis, protein degradation, protein synthesis, ribosomal protein, ribosome.Degradation of chromosomal DNA at the last stage in the though the precise function of individual ribosomal proteins process of apoptosis should result in the complete cessation and RNA has not yet been clarified, it is reasonable to of gene expression in cells fated to die. However, the rate of expect that the inhibition of protein synthesis in apoptotic protein synthesis decreases even before chromosomal DNA cells is the consequence of structural modification of these is degraded (1^1), suggesting the presence of an active molecules. In fact, the 28S ribosomal RNA is selectively mechanism that inhibits gene expression at the level of degraded in apoptotic cells (3,(5)(6)(7). This event occurs at relprotein synthesis in apoptotic cells. The molecular basis for atively early stages of apoptosis via both caspase-depenthis event, however, is not fully understood. dent and -independent mechanisms. It is, however, not A variety of proteins and nucleic acids are involved in clear whether degradation of the 28S RNA leads to strucprotein synthesis. The ribosome stands at the center of the tural changes of ribosomes or the inhibition of protein syntranslational machinery, and the eukaryotic 80S ribosome thesis. On the other hand, factors that are closely related to complex consists of two subunits, 40S and 60S, each of the translation reaction have been shown to undergo degrawhich contains a large number of proteins and RNA. Al-dation in apoptotic cells: eukaryotic translation initiation factors eIF2, eIF3, eIF4B, and eIF4G are degraded in a 1 This study was supported by Grante-in-Aid for Scientific Rese...

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“…Apoptosis studies on Burkitt lymphoma BL60 cells revealed various apoptosis-associated proteins not known in this process so far [117,118]. They gave clues about the apoptosis pathway, the caspases cascade and specific cleavage sites [119,120].…”

Section: Examples Of Successful Application Of Proteomicsmentioning

confidence: 99%

Two‐dimensional gel electrophoresis as tool for proteomics studies in combination with protein identification by mass spectrometry

2006

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The proteome analysis by 2-DE is one of the most potent methods of analyzing the complete proteome of cells, cell lines, organs and tissues in proteomics studies. It allows a fast overview of changes in cell processes by analysis of the entire protein extracts in any biological and medical research projects. New instrumentation and advanced technologies provide proteomics studies in a wide variety of biological and biomedical questions. Proteomics work is being applied to study antibiotics-resistant strains and human tissues of various brain, lung, and heart diseases. It cumulated in the identification of antigens for the design of new vaccines. These advances in proteomics have been possible through the development of advanced high-resolution 2-DE systems allowing resolution of up to 10 000 protein spots of entire cell lysates in combination with protein identification by new highly sensitive mass spectrometric techniques. The present technological achievements are suited for a high throughput screening of different cell situations. Proteomics may be used to investigate the health effects of radiation and electromagnetic field to clarify possible dangerous alterations in human beings.

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Identification of Apoptosis-associated Proteins in a Human Burkitt Lymphoma Cell Line

Cited by 173 publications

References 44 publications

Exploring the biochemical mechanisms of cytotoxic gold compounds: a proteomic study

Exploring the biochemical mechanisms of cytotoxic gold compounds: a proteomic study

Structural Change of Ribosomes during Apoptosis: Degradation and Externalization of Ribosomal Proteins in Doxorubicin-Treated Jurkat Cells

Two‐dimensional gel electrophoresis as tool for proteomics studies in combination with protein identification by mass spectrometry

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