Differential Expression of Genes Encoding Constitutive and Inducible 20S Proteasomal Core Subunits in the Testis and Epididymis of Theophylline- or 1,3-Dinitrobenzene-Exposed Rats1

Tengowski, Mark W.; Feng, Dongyan; Sutovsky, Miriam; Šutovský, Peter

doi:10.1095/biolreprod.106.053173

Cited by 28 publications

(20 citation statements)

References 35 publications

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“…Another important consideration regarding the results of this study that was initially discussed in previous work is how relatively few proteins were identified as targets of oxidative carbonylation when compared to the overall number of proteins present in a DI TNC1 cell’s proteome; an observation made apparent by simply comparing an immunoblot with its corresponding 2D gel. This consistent finding might be explained by one of multiple reasons that include how only the most oxidationsensitive proteins are carbonylated at the toxicant concentrations used, that carbonylation stimulates proteasomal degradation of oxidized proteins, or that protein carbonyl formation may be dependent on molecular weight given that the majority of the carbonylated proteins identified in the current study were distributed among a mass range of 50–70 kDa (Floor and Wetzel 1998; Ceccarini et al, 2007; Tengowski et al, 2007). A recent study surveying current methods of detecting carbonylated proteins using immunoblotting discussed how derivatizing proteins with DNPH after electrophoresis resulted in the detection of more carbonyl-modified proteins than if one were to derivatize proteins prior to electrophoresis (Linares et al, 2011).…”

Section: Discussionsupporting

confidence: 60%

A comparative study of protein carbonylation and mitochondrial dysfunction using the neurotoxicants 1,3-dinitrobenzene, 3-nitropropionic acid, and 3-chloropropanediol

Steiner¹,

Milton²,

Philbert³

2013

NeuroToxicology

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Section: Discussionsupporting

confidence: 60%

A comparative study of protein carbonylation and mitochondrial dysfunction using the neurotoxicants 1,3-dinitrobenzene, 3-nitropropionic acid, and 3-chloropropanediol

Steiner¹,

Milton²,

Philbert³

2013

NeuroToxicology

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“…Proteasomes are tethered to acrosomal membranes and the acrosome surface (Morales et al 2004, Sutovsky et al 2004, Yi et al 2009b, most likely inserted there during acrosomal biogenesis in the spermatid (Mochida et al 2000). We have detected various proteasomal subunits and components of the UPS in the acrosomal granule and cap of rat spermatids (Tengowski et al 2007) but have only incomplete data from livestock species. A possible candidate for proteasome anchoring molecule in the acrosomal membranes is immunophilin FKBP38, shown to tether proteasomes to mitochondrial membranes (Nakagawa et al 2007).…”

Section: Genetic Evidencementioning

confidence: 73%

Sperm proteasome and fertilization

Šutovský

2011

Reproduction

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117

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The omnipresent ubiquitin-proteasome system (UPS) is an ATP-dependent enzymatic machinery that targets substrate proteins for degradation by the 26S proteasome by tagging them with an isopeptide chain composed of covalently linked molecules of ubiquitin, a small chaperone protein. The current knowledge of UPS involvement in the process of sperm penetration through vitelline coat (VC) during human and animal fertilization is reviewed in this study, with attention also being given to sperm capacitation and acrosome reaction/exocytosis. In ascidians, spermatozoa release ubiquitin-activating and conjugating enzymes, proteasomes, and unconjugated ubiquitin to first ubiquitinate and then degrade the sperm receptor on the VC; in echinoderms and mammals, the VC (zona pellucida/ZP in mammals) is ubiquitinated during oogenesis and the sperm receptor degraded during fertilization. Various proteasomal subunits and associated enzymes have been detected in spermatozoa and localized to sperm acrosome and other sperm structures. By using specific fluorometric substrates, proteasome-specific proteolytic and deubiquitinating activities can be measured in live, intact spermatozoa and in sperm protein extracts. The requirement of proteasomal proteolysis during fertilization has been documented by the application of various proteasome-specific inhibitors and antibodies. A similar effect was achieved by depletion of sperm-surface ATP. Degradation of VC/ZP-associated sperm receptor proteins by sperm-borne proteasomes has been demonstrated in ascidians and sea urchins. On the applied side, polyspermy has been ameliorated by modulating sperm-associated deubiquitinating enzymes. Diagnostic and therapeutic applications could emerge in human reproductive medicine. Altogether, the studies on sperm proteasome indicate that animal fertilization is controlled in part by a unique, gamete associated, extracellular UPS.

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“…The standard coefficient was then acquired from dividing the β-Actin value from each patient by the average of the 30 patients. This dosage was called relative because we measured the control expression in relation to the standard test [4][5][6][7] . In the statistical analysis, among the measures of interest, we used parametric and non-parametric tests, with statistical significance level fixed at 5% and a confidence interval at a minimum of 80% and a maximum of 95%.…”

Section: Methodsmentioning

confidence: 99%

Análise de citocinas pela RT-PCR em pacientes com rinite alérgica

Silva

Guimarães²,

Nascimento³

et al. 2009

Rev. Bras. Otorrinolaringol.

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Al lergic rhinitis is an inflammatory reaction of the nasal mucosa, in consequence of an IgE mediated hypersensitive reaction to inhaling allergens, involving different mediators and cytokine cells. Aim: The purpose of this study was to evaluate the transcriptions for IL-4, IL-5, IL-8 and IFNgama, particularly important in the nasal allergy process, especially IL-4 and IL-5. For this study we decided to evaluate atopic patients who were free from allergic crises, with the purpose of knowing the cytokine expressions during this period. Materials and Methods: Another prospective and transversal study was carried out, selecting 30 patients, 13 of these patients were pauci-symptomatic and 17 were non atopic. The groups were selected by means of a medical interview, an otolaryngologic clinical exam and allergy skin tests -Prick Test. The cytokines were investigated in fragments of the nasal mucosa, using RT-PCR -chosen because it has good reproducibility and specificity. Results: IL-5, IL-8, IFNgama cytokine values were kept homogeneous in relation to the control group. Only IL-4 presented significant statistic differences. Conclusion: Asymptomatic patients with allergic rhinitis presented with normalization of cytokine expression in the nasal mucosa, with exception of IL-4.

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Differential Expression of Genes Encoding Constitutive and Inducible 20S Proteasomal Core Subunits in the Testis and Epididymis of Theophylline- or 1,3-Dinitrobenzene-Exposed Rats1

Cited by 28 publications

References 35 publications

A comparative study of protein carbonylation and mitochondrial dysfunction using the neurotoxicants 1,3-dinitrobenzene, 3-nitropropionic acid, and 3-chloropropanediol

A comparative study of protein carbonylation and mitochondrial dysfunction using the neurotoxicants 1,3-dinitrobenzene, 3-nitropropionic acid, and 3-chloropropanediol

Sperm proteasome and fertilization

Análise de citocinas pela RT-PCR em pacientes com rinite alérgica

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