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17. A measurement of the direction of the polarization produced in the scattering of 135 MeV protons

Author

Brinkworth, M. and Rose, B.

Abstract

The 135 MeV polarized proton beam, obtained from the Harwell cyclotron by scattering to the left from carbon, has been slowed down to give protons of energy less than 10 MeV, and these protons have then been scattered by helium. The ratio of the intensities scattered at the same angle to left and right of the incident beam has been measured with photographic plates. This ratio, together with a phase shift calculation of the polarization produced in proton-helium scattering, gives the direction of the polarization produced in the first scattering. -The observed direction agrees with that predicted theoretically on the assumption that the spin-orbit interaction in high energy nuclear scattering is the same as in the shell model of the nucleus. Il fascio polarizzato di protoni ottenuto dal ciclotrone di Harwell per mezzo di scattering a sinistra su carbonio è stato rallentato per ottenere protoni di energia inferiore a 10 MeV e a questi protoni si fa subire uno scattering su elio. Il rapporto delle intensità diffuse sotto lo stesso angolo a destra o a sinistra del fascio incidente è stato misurato con lastre fotografiche. Tale rapporto in unione ad un calcolo in sfasamento della polarizzazione prodotta nello scattering dei protoni su elio dà la direzione della polarizzazione prodotta nel primo scattering. La direzione osservata si accorda con quella prevista dalla teoria facendo l’ipotesi che l’interazione spin-orbita nello scattering nucleare delle alte energie sia la stessa che nel modello a shell.

Published
1902
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23. Effects of Radiofrequency Electromagnetic Field (RF-EMF) exposure on male fertility and pregnancy and birth outcomes: Protocols for a systematic review of experimental studies in non-human mammals and in human sperm exposed in vitro

Author

Carmela Marino, James P. McNamee, Rob B. M. de Vries, Patrizia Eleuteri, Maurizio Sciortino, Francesca Pacchierotti, Martin H. Brinkworth, Carlijn R. Hooijmans, Claudia Consales, Andrew William Wood, Lucia Ardoino, Barbara Benassi, Guangdi Chen, Eugenia Cordelli, Pacchierotti, F., Ardoino, L., Benassi, B., Consales, C., Cordelli, E., Eleuteri, P., Marino, C., Sciortino, M., Brinkworth, M. H., Chen, G., Mcnamee, J. P., Wood, A. W., Hooijmans, C. R., and de Vries, R. B. M.

Subjects
Male, animal structures, Radio Waves, Human sperm, Scopus, Radiofrequency electromagnetic fields, Article, World health, Emf exposure, Cancer development and immune defence Radboud Institute for Health Sciences [Radboudumc 2], Electromagnetic Fields, Pregnancy, Environmental health, Animals, Humans, Medicine, GE1-350, Internal validity, Adverse effect, General Environmental Science, Mammals, Male infertility, business.industry, medicine.disease, Spermatozoa, Animal studies, Environmental sciences, Reconstructive and regenerative medicine Radboud Institute for Health Sciences [Radboudumc 10], Fertility, Health assessment, Adverse pregnancy outcomes, Male fertility, Systematic review, Female, business, Systematic Reviews as Topic
Abstract

Highlights • Male infertility and adverse pregnancy outcomes are relevant human health problems. • Radiofrequency electromagnetic fields are widespread in the human environment. • A link between radiofrequency and adverse reproductive outcomes is controversial. • This is the protocol of WHO-funded systematic review and meta-analysis on this issue., Background Radiofrequency Electromagnetic Fields (RF-EMF) at environmental level have been reported to induce adverse effects on the male reproductive system and developing embryos. However, despite the number of experiments conducted since the 1970s, the diversity of testing approaches and exposure conditions, inconsistencies among results, and dosimetric flaws have not yet permitted a solid assessment of the relationship between RF-EMF exposure and such effects, warranting a more systematic and methodologically rigorous approach to the evaluation of available data. Objectives This study aims at evaluating the effects of RF-EMF exposure on male fertility and pregnancy outcomes by a systematic review (SR) of experimental studies, conducted in compliance with international guidelines. The evidence will be organized into three streams: 1) Studies evaluating the impact of RF-EMF on the male reproductive system of experimental mammals; 2) studies evaluating the impact of RF-EMF on human sperm exposed in vitro; 3) studies evaluating the impact of RF-EMF on adverse pregnancy, birth outcomes and delayed effects in experimental mammals exposed in utero. Study eligibility and criteria Eligible studies will include peer-reviewed articles reporting of original results about effects of controlled exposures to RF-EMF in the frequency range 100 kHz–300 GHz on the selected outcomes without any language or year-of-publication restrictions. Eligible studies will be retrieved by calibrated search strings applied to three electronic databases, PubMed, Scopus and EMF Portal and by manual search of the list of references of included papers and published reviews. Study appraisal and synthesis method The internal validity of the studies will be evaluated using the Risk of Bias (RoB) Rating Tool developed by National Toxicology Program/Office of Health Assessment and Translation (NTP/OHAT) integrated with input from the SYRCLE RoB tool. Given sufficient commensurate data, meta-analyses will be performed, otherwise narrative syntheses will be produced. Finally, the certainty of the effects of RF-EMF exposure on male fertility and pregnancy and birth outcomes will be established following GRADE. Funding The study is financially supported by the World Health Organization. Registration OSF Registration DOI https://doi.org/10.17605/OSF.IO/7MUS3; PROSPERO CRD42021227729, CRD42021227746.

Published
2021

24. Genetic damage in oligozoospermic patients detected by fluorescence in-situ hybridization, inverse restriction site mutation assay, sperm chromatin structure assay and the Comet assay

Author

Heiner Bollwein, Thomas E. Schmid, Eberhard Nieschlag, Martin H. Brinkworth, Axel Kamischke, University of Zurich, and Brinkworth, M H

Subjects
Infertility, Adult, Male, Restriction Mapping, Semen, Biology, Gene mutation, Pregnancy, medicine, Humans, In Situ Hybridization, Fluorescence, medicine.diagnostic_test, 630 Agriculture, Rehabilitation, Obstetrics and Gynecology, 2729 Obstetrics and Gynecology, Oligospermia, 2743 Reproductive Medicine, medicine.disease, Aneuploidy, Molecular biology, Sperm, Spermatozoa, Chromatin, Comet assay, 10187 Department of Farm Animals, Reproductive Medicine, 570 Life sciences, biology, Female, Comet Assay, Spermatogenesis, Fluorescence in situ hybridization, DNA Damage
Abstract

BACKGROUND: The possibility that oligozoospermic men may have elevated levels of genetic damage in their sperm is of particular concern as they could transmit defects to their offspring. METHODS: Sperm samples were obtained from 12 infertile, oligozoospermic patients and 12 healthy normozoospermic volunteers. Fluorescence in-situ hybridization (FISH) was used to determine aneuploidy rates in sperm and inverse restriction site mutation (iRSM) assay to determine gene mutations; defective chromatin packaging was quantified by sperm chromatin structure assay (SCSA) and DNA strand breaks by the Comet assay. RESULTS: FISH analysis showed a significant increase in gonosomal X,Y,18 (P < 0.01) disomy and diploid sperm with X,Y,18,18 (P < 0.05) in the infertility patients compared with the controls. A significant increase (P < 0.01) in disturbed sperm chromatin was found in the infertility patients compared with the control group using the SCSA assay. In the Comet assay, a significant increase (P < 0.01) in the tail moment was found in the infertility patients compared with the control group, indicating significantly high levels of DNA strand breaks. There was no significant increase in point mutations detected by iRSM assay. CONCLUSIONS: The data indicate that infertile oligozoospermic men have an elevated level of XY aneuploidy and XY diploidy in the germ-line, as well as elevated levels of sperm chromatin disturbances and sperm DNA strand breaks. These data demonstrate that oligozoospermic infertility patients show several different types of genetic damage in their sperm. Thus, such men appear to have defects at a variety of levels of spermatogenesis and their infertility may not just be a result of the oligozoospermia.

Published
2003

27. Effects of radiofrequency electromagnetic field (RF-EMF) exposure on male fertility: A systematic review of experimental studies on non-human mammals and human sperm in vitro.

Author

Cordelli E, Ardoino L, Benassi B, Consales C, Eleuteri P, Marino C, Sciortino M, Villani P, H Brinkworth M, Chen G, P McNamee J, Wood AW, Belackova L, Verbeek J, and Pacchierotti F

Subjects
Animals, Humans, Male, Mammals, Radio Waves adverse effects, Reproduction, Electromagnetic Fields adverse effects, Semen radiation effects, Infertility, Male etiology
Abstract

Background: The World Health Organization is coordinating an international project aimed at systematically reviewing the evidence regarding the association between radiofrequency electromagnetic field (RF-EMF) exposure and adverse health effects. Reproductive health outcomes have been identified among the priority topics to be addressed., Objectives: To evaluate the effect of RF-EMF exposure on male fertility of experimental mammals and on human sperm exposed in vitro., Methods: Three electronic databases (PubMed, Scopus and EMF Portal) were last searched on September 17, 2022. Two independent reviewers screened the studies, which were considered eligible if met the following criteria: 1) Peer-reviewed publications of sham controlled experimental studies, 2) Non-human male mammals exposed at any stage of development or human sperm exposed in vitro, 3) RF-EMF exposure within the frequency range of 100 kHz-300 GHz, including electromagnetic pulses (EMP), 4) one of the following indicators of reproductive system impairment:Two reviewers extracted study characteristics and outcome data. We assessed risk of bias (RoB) using the Office of Health Assessment and Translation (OHAT) guidelines. We categorized studies into 3 levels of overall RoB: low, some or high concern. We pooled study results in a random effects meta-analysis comparing average exposure to no-exposure and in a dose-response meta-analysis using all exposure doses. For experimental animal studies, we conducted subgroup analyses for species, Specific Absorption Rate (SAR) and temperature increase. We grouped studies on human sperm exposed in vitro by the fertility status of sample donors and SAR. We assessed the certainty of the evidence using the GRADE approach after excluding studies that were rated as "high concern" for RoB., Results: One-hundred and seventeen papers on animal studies and 10 papers on human sperm exposed in vitro were included in this review. Only few studies were rated as "low concern" because most studies were at RoB for exposure and/or outcome assessment. Subgrouping the experimental animal studies by species, SAR, and temperature increase partly accounted for the heterogeneity of individual studies in about one third of the meta-analyses. In no case was it possible to conduct a subgroup analysis of the few human sperm in vitro studies because there were always 1 or more groups including less than 3 studies. Among all the considered endpoints, the meta-analyses of animal studies provided evidence of adverse effects of RF-EMF exposure in all cases but the rate of infertile males and the size of the sired litters. The assessment of certainty according to the GRADE methodology assigned a moderate certainty to the reduction of pregnancy rate and to the evidence of no-effect on litter size, a low certainty to the reduction of sperm count, and a very low certainty to all the other meta-analysis results. Studies on human sperm exposed in vitro indicated a small detrimental effect of RF-EMF exposure on vitality and no-effect on DNA/chromatin alterations. According to GRADE, a very low certainty was attributed to these results. The few studies that used EMP exposure did not show effects on the outcomes. A low to very low certainty was attributed to these results., Discussion: Many of the studies examined suffered of severe limitations that led to the attribution of uncertainty to the results of the meta-analyses and did not allow to draw firm conclusions on most of the endpoints. Nevertheless, the associations between RF-EMF exposure and decrease of pregnancy rate and sperm count, to which moderate and low certainty were attributed, are not negligible, also in view of the indications that in Western countries human male fertility potential seems to be progressively declining. It was beyond the scope of our systematic review to determine the shape of the dose-response relationship or to identify a minimum effective exposure level. The subgroup and the dose-response fitting analyses did not show a consistent relationship between the exposure levels and the observed effects. Notably, most studies evaluated RF-EMF exposure levels that were higher than the levels to which human populations are typically exposed, and the limits set in international guidelines. For these reasons we cannot provide suggestions to confirm or reconsider current human exposure limits. Considering the outcomes of this systematic review and taking into account the limitations found in several of the studies, we suggest that further investigations with better characterization of exposure and dosimetry including several exposure levels and blinded outcome assessment were conducted., Protocol Registration: Protocols for the systematic reviews of animal studies and of human sperm in vitro studies were published in Pacchierotti et al., 2021. The former was also registered in PROSPERO (CRD42021227729 https://www.crd.york.ac.uk/prospero/display&#95;record.php?RecordID = 227729) and the latter in Open Science Framework (OSF Registration DOI https://doi.org/10.17605/OSF.IO/7MUS3)., Competing Interests: Declaration of competing interest AWW previously directed a research group, which included two technical associates who are telecommunications company employees. AWW has been member of the ICNIRP Scientific Expert Group (SEG) from 2013 until 2021 and collaborates with the Australian Radiation Protection and Nuclear Safety Agency. JPMN was a member for IARC Monograph 102 Working Group assessing the carcinogenicity of RF-EMF (Mechanistic Studies sub-group), a co-author of Canada’s Safety Code 6 (which are the de facto national human exposure limits applied in Canada) and a member of the WHO EMF Project International Advisory Committee (Canadian representative). Health Canada financially contributed to the WHO EMF Project to support the completion of the systematic reviews on RF-EMF. CM has been member of Technical Consultation on the WHO RF Research Agenda (2010), member of ICNIRP main commission since May 2012, confirmed in 2016 and 2020, Italian delegate for the European Cost Actions BM0704 and BM1309 “EMF-MED”. All other authors declare that they have no known conflicts of interest., (Copyright © 2024 The Authors. Published by Elsevier Ltd.. All rights reserved.)

Published
2024
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28. Responses to genotoxicity in mouse testicular germ cells and epididymal spermatozoa are affected by increased age.

Author

Taylor JD, Baumgartner A, Schmid TE, and Brinkworth MH

Subjects
Age Factors, Animals, Apoptosis drug effects, Chromatin Assembly and Disassembly drug effects, Comet Assay, DNA Damage, Epididymis metabolism, Epididymis pathology, In Situ Nick-End Labeling, Male, Mice, Inbred C3H, Risk Assessment, Spermatozoa metabolism, Spermatozoa pathology, Testis metabolism, Testis pathology, Cyclophosphamide toxicity, Epididymis drug effects, Spermatogenesis drug effects, Spermatozoa drug effects, Testis drug effects
Abstract

The increased number of cell divisions undergone by spermatogonia of older fathers cannot fully account for the observed increase in germline genetic damage. Studies have shown that the mechanisms induced in germ cells in response to oxidative damage varies with age, that DNA repair efficiency declines, and both sperm DNA damage and spontaneous mutations increase. However, it is not known whether the altered response with age is a cause, or consequence, of an age-associated change in cell susceptibility to genetic damage. Following a single 150 mg/kg dose of cyclophosphamide (CP), young (8-weeks old) and aged (17-month old) male mice were examined 24 h later for induced genetic damage in epididymal spermatozoa using the alkaline comet and sperm chromatin stability assays. Apoptosis among testicular cells was examined on tissue cross-sections using the TUNEL assay. Sperm showed no significant increase in DNA strand breaks with age (detected by the comet assay) and no change in sperm chromatin stability (detected by the SCSA assay). Following CP treatment, there was no effect on DNA-strand breakage but sperm chromatin instability was significantly higher. Furthermore, it was also significantly elevated in old treated, compared with young treated, animals suggesting that increased age affects the sensitivity of epididymal sperm to chromatin damage. There was no difference in apoptosis in testicular germ cells from either young or old control animals, while CP administration resulted in a significant increase in apoptosis among young animals but not old animals. Following genotoxin exposure, an increase in chromatin instability in the spermatozoa of old animals and a decrease in the ability of their testicular germ cells undergo apoptosis suggests an age-related decrease in genome protection mechanisms. Since those germ cells are only transiently present in the testis, it is likely that this age-related deterioration originates in the spermatogonial stem cells. The findings are also evidence that the safety evaluation of reproductive genotoxins should consider young and old individuals separately., (Copyright © 2019 Elsevier B.V. All rights reserved.)

Published
2019
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29. Detection of phase specificity of in vivo germ cell mutagens in an in vitro germ cell system.

Author

Habas K, Anderson D, and Brinkworth M

Subjects
Animals, Comet Assay, Dose-Response Relationship, Drug, In Situ Nick-End Labeling, Male, Mutagenicity Tests, Mutagens administration & dosage, Rats, Rats, Sprague-Dawley, Spermatocytes drug effects, Spermatogenesis drug effects, DNA Damage drug effects, Meiosis drug effects, Mutagens toxicity, Spermatogonia drug effects, Spermatozoa drug effects
Abstract

In vivo tests for male reproductive genotoxicity are time consuming, resource-intensive and their use should be minimised according to the principles of the 3Rs. Accordingly, we investigated the effects in vitro, of a variety of known, phase-specific germ cell mutagens, i.e., pre-meiotic, meiotic, and post-meiotic genotoxins, on rat spermatogenic cell types separated using Staput unit-gravity velocity sedimentation, evaluating DNA damage using the Comet assay. N-ethyl-N-nitrosourea (ENU), N-methyl-N-nitrosourea (MNU) (spermatogenic phase), 6-mercaptopurine (6-MP) and 5-bromo-2'-deoxy-uridine (5-BrdU) (meiotic phase), methyl methanesulphonate (MMS) and ethyl methanesulphonate (EMS) (post-meiotic phase) were selected for use as they are potent male rodent, germ cell mutagens in vivo. DNA damage was detected directly using the Comet assay and indirectly using the TUNEL assay. Treatment of the isolated cells with ENU and MNU produced the greatest concentration-related increase in DNA damage in spermatogonia. Spermatocytes were most sensitive to 6-MP and 5-BrdU while spermatids were particularly susceptible to MMS and EMS. Increases were found when measuring both Olive tail moment (OTM) and% tail DNA, but the greatest changes were in OTM. Parallel results were found with the TUNEL assay, which showed highly significant, concentration dependent effects of all these genotoxins on spermatogonia, spermatocytes and spermatids in the same way as for DNA damage. The specific effects of these chemicals on different germ cell types matches those produced in vivo. This approach therefore shows potential for use in the detection of male germ cell genotoxicity and could contribute to the reduction of the use of animals in such toxicity assays., (Copyright © 2016. Published by Elsevier Ireland Ltd.)

Published
2016
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30. Development of an in vitro test system for assessment of male, reproductive toxicity.

Author

Habas K, Anderson D, and Brinkworth M

Subjects
Animals, Biomarkers metabolism, Cell Separation, Cells, Cultured, Dose-Response Relationship, Drug, Immunohistochemistry, Male, Mice, Spermatids drug effects, Spermatids pathology, Spermatocytes drug effects, Spermatocytes pathology, Spermatogonia drug effects, Spermatogonia pathology, Spermatozoa metabolism, Spermatozoa pathology, Testis metabolism, Testis pathology, Apoptosis drug effects, Hydrogen Peroxide toxicity, In Situ Nick-End Labeling, Reproduction drug effects, Spermatozoa drug effects, Testis drug effects, Toxicity Tests methods
Abstract

There is a need for improved reproductive toxicology assays that do not require large numbers of animals but are sensitive and informative. Therefore, Staput velocity-sedimentation separation followed by culture of specific mouse testicular cells was used as such a system. The specificity of separation was assessed using immunocytochemistry to identify spermatids, spermatocytes and spermatogonia. The efficacy of the system to detect toxicity was then evaluated by analysing the effects of hydrogen peroxide (H2O2) by the terminal uridine-deoxynucleotide end-labelling (TUNEL) assay to show the rate of apoptosis induced among the different types of germ cells. We found that 2 h of treatment at both 1 and 10 μM induced increases of over ∼10-fold in the percentage of apoptotic cells (p≤0.001), confirming that testicular germ cells are prone to apoptosis at very low concentrations of H2O2. It was also demonstrated for the first time for this compound that spermatogonia are significantly more susceptible than spermatocytes, which are more affected than spermatids. This reflects the proportion of actively dividing cells in these cell types, suggesting a mechanism for the differential sensitivity. The approach should thus form the basis of a useful test system for reproductive and genetic toxicology in the future., (Copyright © 2013 Elsevier Ireland Ltd. All rights reserved.)

Published
2014
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31. Moderating effects of teacher-student relationship in adolescent trajectories of emotional and behavioral adjustment.

Author

Wang MT, Brinkworth M, and Eccles J

Subjects
Adolescent, Adolescent Behavior, Child, Child Behavior Disorders, Female, Humans, Linear Models, Longitudinal Studies, Male, Sex Factors, Temperament, Urban Population, Adaptation, Psychological, Depression, Faculty, Interpersonal Relations, Parent-Child Relations, Students psychology
Abstract

This study examined relations between effortful control, parent-adolescent conflict, and teacher-student relationships and the concurrent and longitudinal impact of these factors on adolescent depression and misconduct. In particular, we examined whether the risks of low effortful control and parent-adolescent conflict could be buffered by positive teacher-student relationships characterized by warmth and trust. Data were collected on 1,400 urban youths (52% female, 51% Black, 44% White) who reported on their effortful control at age 13 years and on their depressive symptoms and misconduct from ages 13-18. Teacher-student relationship data were collected from teacher-report at age 13 and parent-adolescent conflict data from parent-report at age 13. As hypothesized, regardless of gender, both early poor effortful control and conflictive parent-adolescent relationship were general risks for adolescents' depression and misconduct. Positive teacher-student relationships protected adolescents against depression and misconduct throughout ages 13-18. In addition, positive teacher-student relationships moderated the negative influences of adolescents' early poor effortful control and conflictive parent-adolescent relationships on misconduct and helped such at-risk adolescents to attain less behaviorally delinquent developmental trajectories over time., ((PsycINFO Database Record (c) 2013 APA, all rights reserved).)

Published
2013
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32. Key gene regulatory sequences with distinctive ontological signatures associate with differentially endonuclease-accessible mouse sperm chromatin.

Author

Saida M, Iles D, Elnefati A, Brinkworth M, and Miller D

Subjects
Animals, Binding Sites, CCCTC-Binding Factor, Cell Nucleus metabolism, Cell Nucleus ultrastructure, Comparative Genomic Hybridization, DNA Methylation, Data Mining, Epididymis cytology, Histones metabolism, Hydrolysis, In Situ Hybridization, Fluorescence, Male, Mice, Nucleosomes chemistry, Nucleosomes metabolism, Polynucleotides chemistry, Polynucleotides metabolism, Solubility, Spermatozoa metabolism, Bacterial Proteins metabolism, Chromatin chemistry, Chromatin metabolism, Micrococcal Nuclease metabolism, Promoter Regions, Genetic, Repressor Proteins metabolism, Spermatozoa ultrastructure
Abstract

Using a well-established endonuclease-based chromatin dissection procedure in conjunction with both experimental comparative genome hybridisation (CGH) array profiling and in silico data mining, we show that mouse spermatozoa contain chromatin that is sensitive and resistant to digestion with micrococcal nuclease (MNase). Sequences represented in the micrococcal nuclease digestion solubilised (MNDS) but not the MND insoluble (MNDI) chromatin are strongly enriched in chromosomal regions of high gene density. Furthermore, by fluorescence in situ hybridisation (FISH) analysis, we show that MNDS and MNDI DNAs occupy distinct domains of decondensed mouse sperm nuclei that may also retain abundant histones. More detailed in silico analysis of CGH probe location in relation to known promoters and sequences recognised by CCCTC binding factor (CTCF) shows a significant excess of both in MNDS chromatin. A functional analysis of gene promoters reveals strong ontological signatures for ion transport on methylated promoters associated with CTCF binding sequences in MNDS chromatin. Sensory perception is the only strong ontological signature present in MNDI chromatin, driven by promoters that are not associated with CTCF regardless of their methylation status.

Published
2011
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33. Paternal DNA packaging in spermatozoa: more than the sum of its parts? DNA, histones, protamines and epigenetics.

Author

Miller D, Brinkworth M, and Iles D

Subjects
Animals, DNA Methylation, Female, Gene Expression Regulation, Developmental, Genetic Code, Genomic Imprinting, Humans, Male, Paternity, Sperm-Ovum Interactions, Spermatogenesis, Chromatin Assembly and Disassembly, DNA metabolism, Epigenesis, Genetic, Histones metabolism, Nucleosomes metabolism, Protamines metabolism, Spermatozoa metabolism
Abstract

Haploid male germ cells package their DNA into a volume that is typically 10% or less that of a somatic cell nucleus. To achieve this remarkable level of compaction, spermatozoa replace most of their histones with smaller, highly basic arginine and (in eutherians) cysteine rich protamines. One reason for such a high level of compaction is that it may help optimise nuclear shape and hence support the gametes' swimming ability for the long journey across the female reproductive tract to the oocyte. Super-compaction of the genome may confer additional protection from the effects of genotoxic factors. However, many species including the human retain a fraction of their chromatin in the more relaxed nucleosomal configuration that appears to run counter to the ergonomic, toroidal and repackaging of sperm DNA. Recent research suggests that the composition of this 'residual' nucleosomal compartment, a generally overlooked feature of the male gamete, is far more significant and important than previously thought. In this respect, the transport and incorporation of modified paternal histones by the spermatozoon to the zygote has been demonstrated and indicates another potential paternal effect in the epigenetic reprogramming of the zygote following fertilisation that is independent of imprinting status. In this review, the most recent research into mammalian spermatozoal chromatin composition is discussed alongside evidence for conserved, non-randomly located nucleosomal domains in spermatozoal nuclei, all supporting the hypothesis that the spermatozoon delivers a novel epigenetic signature to the egg that may be crucial for normal development. We also provide some thoughts on why this signature may be required in early embryogenesis.

Published
2010
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34. Endonuclease-sensitive regions of human spermatozoal chromatin are highly enriched in promoter and CTCF binding sequences.

Author

Arpanahi A, Brinkworth M, Iles D, Krawetz SA, Paradowska A, Platts AE, Saida M, Steger K, Tedder P, and Miller D

Subjects
Acetylation, Animals, Base Sequence, Binding Sites genetics, CCCTC-Binding Factor, Chromatin metabolism, Chromatin Immunoprecipitation, Comparative Genomic Hybridization, DNA genetics, DNA metabolism, Electrophoresis, Agar Gel, Genome-Wide Association Study, Histones metabolism, Humans, Lysine metabolism, Male, Mice, Protein Binding, Regulatory Sequences, Nucleic Acid genetics, Chromatin genetics, Endonucleases metabolism, Promoter Regions, Genetic genetics, Repressor Proteins metabolism, Spermatozoa metabolism
Abstract

During the haploid phase of mammalian spermatogenesis, nucleosomal chromatin is ultimately repackaged by small, highly basic protamines to generate an extremely compact, toroidal chromatin architecture that is critical to normal spermatozoal function. In common with several species, however, the human spermatozoon retains a small proportion of its chromatin packaged in nucleosomes. As nucleosomal chromatin in spermatozoa is structurally more open than protamine-packaged chromatin, we considered it likely to be more accessible to exogenously applied endonucleases. Accordingly, we have used this premise to identify a population of endonuclease-sensitive DNA sequences in human and murine spermatozoa. Our results show unequivocally that, in contrast to the endonuclease-resistant sperm chromatin packaged by protamines, regions of increased endonuclease sensitivity are closely associated with gene regulatory regions, including many promoter sequences and sequences recognized by CCCTC-binding factor (CTCF). Similar differential packaging of promoters is observed in the spermatozoal chromatin of both mouse and man. These observations imply the existence of epigenetic marks that distinguish gene regulatory regions in male germ cells and prevent their repackaging by protamines during spermiogenesis. The ontology of genes under the control of endonuclease-sensitive regulatory regions implies a role for this phenomenon in subsequent embryonic development.

Published
2009
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35. Detection of structural and numerical chromosomal abnormalities by ACM-FISH analysis in sperm of oligozoospermic infertility patients.

Author

Schmid TE, Brinkworth MH, Hill F, Sloter E, Kamischke A, Marchetti F, Nieschlag E, and Wyrobek AJ

Subjects
Adult, Color, Gene Deletion, Genes, Duplicate, Humans, Infertility, Male pathology, Infertility, Male physiopathology, Male, Oligospermia pathology, Oligospermia physiopathology, Sperm Count, Sperm Motility, Chromosome Aberrations, In Situ Hybridization, Fluorescence methods, Infertility, Male genetics, Oligospermia genetics, Spermatozoa ultrastructure
Abstract

Background: Modern reproductive technologies are enabling the treatment of infertile men with severe disturbances of spermatogenesis. The possibility of elevated frequencies of genetically and chromosomally defective sperm has become an issue of concern with the increased usage of ICSI, which can enable men with severely impaired sperm production to father children. Several papers have been published reporting aneuploidy in oligozoospermic patients, but relatively little is known about chromosome structural aberrations in the sperm of these patients., Methods: We examined sperm from infertile, oligozoospermic individuals for structural and numerical chromosomal abnormalities using a multicolour ACM fluorescence in situ hybridization (FISH) assay that utilizes DNA probes specific for three regions of chromosome 1 to detect human sperm that carry numerical chromosomal abnormalities plus two categories of structural aberrations: duplications and deletions of 1pter and 1cen, and chromosomal breaks within the 1cen-1q12 region., Results: There was a significant increase in the average frequencies of sperm with duplications and deletions in the infertility patients compared with the healthy concurrent controls. There was also a significantly elevated level of breaks within the 1cen-1q12 region. There was no evidence for an increase in chromosome 1 disomy, or in diploidy., Conclusions: Our data reveal that oligozoospermia is associated with chromosomal structural abnormalities, suggesting that oligozoospermic men carry a higher burden of transmissible, chromosome damage. The findings raise the possibility of elevated levels of transmissible chromosomal defects following ICSI treatment.

Published
2004
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36. Effect of age on testicular germ cell apoptosis and sperm aneuploidy in MF-1 mice.

Author

Brinkworth MH and Schmid TE

Subjects
Animals, Chromosome Aberrations, DNA Probes, In Situ Hybridization, Fluorescence, In Situ Nick-End Labeling, Male, Mice, Mice, Mutant Strains, Aging physiology, Aneuploidy, Apoptosis physiology, Spermatozoa physiology, Testis physiology
Abstract

The spontaneous mutation rate in the male germ-line increases with age. The reason for this is unknown, but presumably involves an age-related degeneration in the efficacy of cellular processes. To investigate the possibility that rates of apoptosis and genetic damage (represented by aneuploidy) might vary with age in mice, the testes and sperm of 2- and 12-month-old male MF-1 mice were examined by a modified TUNEL technique and 3-colour sperm-FISH assay, respectively. Sperm were labeled with probes to chromosomes 8, X and Y and 20,000 sperm scored from each of 5 animals per group. A significant increase in gonosomal disomy was found in the aged mice, especially X-X-8. This suggests that advanced paternal age is associated primarily with meiosis II rather than meiosis I disjunction errors. Neither diploidy nor autosomal disomy was affected in the older group. The rate of germ cell apoptosis (apoptotic cells per seminiferous tubule cross-section per animal per group) was higher in the old mice than controls, but not significantly. Considerable inter-animal variability was observed in the older group. The finding of an increase in levels of sperm aneuploidy is novel for 1-year-old mice and confirms the genotoxic effect of ageing in mice. Since apoptosis is assumed to eliminate cells with unrepaired damage, it may be that the apoptotic response in older mice is compromised, resulting in the higher levels of aneuploidy in sperm. However, given the inter-animal variability in testicular germ cell apoptosis, this awaits confirmation., (Copyright 2003 Wiley-Liss, Inc.)

Published
2003
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37. Paternal transmission of genetic damage: findings in animals and humans.

Author

Brinkworth MH

Subjects
Animals, Female, Humans, Male, Germ-Line Mutation, Mutagens toxicity, Paternity
Abstract

The concept that mutations can be induced in the male germ-line and result in adverse effects in the offspring has achieved only limited acceptance despite considerable theoretical appeal. This is partly because fetal malformations are generally perceived to be induced solely as a result of maternally mediated events during gestation and partly because the low incidence of the end-points concerned make experimental approaches costly and time-consuming. Nonetheless, a substantial body of work relating to the hypothesis has accumulated in the last 20 years, which has never been reviewed in its entirety. A consideration of the available evidence indicates that preconceptional paternal exposure to mutagens (particularly radiation, cyclophosphamide and ethylnitrosourea) can indeed, under certain conditions, have adverse effects on offspring. The results suggest two principal mechanisms by which such effects may be induced: the induction of germ-line genomic instability or the suppression of germ cell apoptosis.

Published
2000
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38. Examination of ras oncoproteins in human plasma from healthy controls and workers exposed to petroleum emissions, including benzene-related compounds.

Author

Anderson D, Hughes JA, Brinkworth MH, Cebulska-Wasilewska A, Nizankowska E, Graca B, Veidebaum T, Peltonen K, and Sorsa M

Subjects
Blotting, Western, Chemical Industry, Electrophoresis, Polyacrylamide Gel, Environmental Monitoring methods, Estonia, Humans, Petroleum, Poland, Seasons, Air Pollutants, Occupational blood, Benzene analysis, Benzene Derivatives analysis, Biomarkers blood, Occupational Exposure analysis, Proto-Oncogene Proteins p21(ras) blood
Abstract

Ras oncoproteins in blood plasma from workers exposed to petroleum emissions and unexposed controls were examined from Polish and Estonian samples. Twenty-four workers and 35 unexposed controls were examined from Poland and 97 exposed and 40 unexposed controls from Estonia. Of the Estonian workers, 50 were exposed to benzene in a benzene production plant and 47 to polyaromatic hydrocarbons and benzene in a cokery. Blood plasma proteins were separated by gel electrophoresis, transferred to a nitrocellulose membrane by Western blotting and detected by chemiluminescence using a monoclonal antibody as the primary antibody. There were no statistically significant differences between the exposed and the control groups in either the Polish or the Estonian samples.

Published
1999
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39. Direct analysis by small-pool PCR of MS205 minisatellite mutation rates in sperm after mutagenic therapies.

Author

Armour JA, Brinkworth MH, and Kamischke A

Subjects
DNA drug effects, DNA genetics, Drug-Related Side Effects and Adverse Reactions, Humans, Male, Minisatellite Repeats genetics, Mutagenesis, Polymerase Chain Reaction, Semen cytology, Semen drug effects, Semen metabolism, Sperm Count drug effects, Sperm Motility drug effects, Spermatozoa metabolism, Germ-Line Mutation, Minisatellite Repeats drug effects, Spermatozoa drug effects
Abstract

We have used small-pool PCR to analyse mutation in samples of sperm taken from men after mutagenic therapy. Small-pool PCR uses direct analysis of germline DNA at a highly unstable tandem-repeated "minisatellite" locus to measure rates of length-change mutation in individual sperm samples. The advantages of this approach are that the normal mutation rate is extremely high (about 0.4% per gamete at the locus analysed here), so that relatively small increases in mutation rate can be detectable in individual samples. It is known from work on sperm from untreated individuals that different alleles at this locus have different mutation rates. For this reason, we have analysed the germline mutation rates in sperm samples from two men, in each case comparing a post-treatment sample with a pre-treatment sample from the same individual. We find no evidence for altered mutation in the post-treatment sample, suggesting that the repopulation of the germ-cell compartment after treatment may be subject to stringent mechanisms for the detection and elimination of germ-cell damage.

Published
1999
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40. An investigation of male-mediated F1 effects in mice treated acutely and sub-chronically with urethane.

Author

Edwards AJ, Anderson D, Brinkworth MH, Myers B, and Parry JM

Subjects
Animals, Body Weight, Carcinogens metabolism, DNA Mutational Analysis, Female, Infertility, Karyotyping, Male, Mice, Polymorphism, Restriction Fragment Length, Pregnancy, Urethane administration & dosage, Urethane metabolism, Abnormalities, Drug-Induced etiology, Carcinogens toxicity, Neoplasms chemically induced, Paternal Exposure, Urethane toxicity
Abstract

In order to investigate the alleged potential of paternally administered urethane to cause foetal abnormalities and heritable tumours, male CD-1 mice were treated with urethane, either acutely by intraperitoneal injection at doses of 1.25 and 1.75 g/kg bodyweight (bwt) or sub-chronically in the drinking water at 1.25 for 10 weeks, and 3.75 mg/ml for 9 weeks or vehicle for the control groups. They were mated to untreated females 1 week later. Uterine contents of half the pregnant females were examined just before full term, while the remaining females were allowed to deliver their litters. The resulting F1 offspring were observed for approximately 18 months and 12 months for acute and sub-chronic exposures respectively and subjected to necropsy examination. Some of the mice treated acutely with 1.75 g/kg bwt exhibited partial infertility but none of those treated with 1.25 g/kg bwt had an adverse effect on their reproductive ability. There was no genetic effect of acute urethane treatment on male germ cells as indicated by dominant lethality. After birth, there was an increase (P < 0.05) in post-implantation deaths possibly due to perinatal mortality. There was an increased incidence and earlier onset of liver tumours induced in F1 male offspring from F0 males treated with 1.75 g/kg bwt, (20.7% vs. 10.1%, P = 0.026) but not in the female offspring. F1 males from both treatment groups had mean bodyweights significantly higher than controls (P < 0.01). Some males from each dose group of the acute study were examined using the restriction site mutation assay involving analysis of exon sequences. No mutations were identified in testes, liver or spleen of DNA isolated from the urethane-treated animals. No reproductive or genetic effects were seen with sub-chronic treatment at either 1.25 or 3.75 mg/ml urethane nor was there any predisposition of F1 animals to tumours although observation times were shorter.

Published
1999

41. Commentary: paternal legacies.

Author

Anderson D, Jenkinson PC, Edwards AJ, Hughes JA, and Brinkworth MH

Subjects
Abnormalities, Drug-Induced, Animals, Male, Mice, Rats, Teratogens pharmacology, Butadienes administration & dosage, Butadienes pharmacology, Cyclophosphamide administration & dosage, Cyclophosphamide pharmacology, Paternal Exposure, Urethane administration & dosage, Urethane pharmacology
Published
1999

42. Modulation of ras p21 oncoprotein levels and DNA strand breakage in human cells with chemotherapeutic agents and/or deferoxamine.

Author

Anderson D, Yardley-Jones A, Yu TW, Hughes JA, and Brinkworth MH

Subjects
Caco-2 Cells, Free Radicals, Humans, Antineoplastic Agents toxicity, DNA radiation effects, DNA Damage, Deferoxamine pharmacology, Doxorubicin toxicity, Mitomycin toxicity, Proto-Oncogene Proteins p21(ras) analysis
Abstract

Oncogenes are involved with the regulation of cellular proliferation. Ras oncogenes can be activated by chemical treatment and any increased activity could be modulated by further chemical treatment. In the present study, therefore, ras p21 protein expression was examined in in vitro cultures of human lymphocytes treated with mitomycin C and in the human colon adenocarcinoma Caco-2 cell line treated with doxorubicin with and without deferoxamine. Both chemotherapeutic agents act partially through oxygen radical mechanisms. Increases in p21 protein levels were seen with mitomycin C but no clear response was seen with doxorubicin. However, deferoxamine, with and without doxorubicin, altered p21 expression. Deferoxamine is an iron chelator so these results support the hypothesis that oxygen radicals were responsible for the altered p21 protein levels. Modulating responses were confirmed by measuring DNA strand-breakage in the Comet assay after treatment with doxorubicin and deferoxamine. Alterations of ras p21 protein expression in vitro might prove a suitable system for examining modulating effects on chemical carcinogens.

Published
1998

43. Expression of mitotic cyclin B1 is not confined to proliferating cells in the rat testis.

Author

Gromoll J, Wessels J, Rosiepen G, Brinkworth MH, and Weinbauer GF

Subjects
Amino Acid Sequence, Animals, Blotting, Northern, Cloning, Molecular, Cyclin B chemistry, Cyclin B1, Gene Expression Regulation, Humans, Immunohistochemistry, In Situ Hybridization, Male, Molecular Sequence Data, RNA, Messenger analysis, Rats, Rats, Sprague-Dawley, Sequence Homology, Spermatogenesis, Cell Division, Cyclin B genetics, Gene Expression, Mitosis, Testis cytology
Abstract

Spermatogenesis is a precisely controlled and timed process comprising mitotic divisions of spermatogonia, meiotic divisions of spermatocytes, and the maturation and differentiation of haploid spermatids. Cell proliferation is controlled by genes involved in the regulation of the cell cycle. Among the principal regulatory proteins are cyclins, which are categorized according to their appearance during the cell cycle. B-type cyclins are mitotic cyclins and function at the G2/M transition of the cell cycle. We have investigated the expression and regulation of cyclin B1 during rat spermatogenesis. Rat cyclin B1 was isolated from a testis cDNA library and further used as a probe to detect mRNA expression. Northern blot hybridization of testis mRNA revealed the presence of a single 1.7-kilobase transcript. In situ hybridization showed stage-specific expression during spermatogenesis with highest expression found in late pachytene spermatocytes and early round spermatids. This pattern was confirmed in fractions of isolated germ cells. Immunocytochemistry displayed highest protein levels in round spermatids. Depletion of gonadotropins did not change the quantitative and qualitative expression pattern of cyclin B1. Therefore, the signals triggering the onset of cyclin B1 expression seem not to originate from the pituitary-gonadal endocrine axis and might therefore be paracrine factors originating within the germinal epithelium. Our observations suggest that cyclin B1 plays a hitherto unknown role in spermatid maturation in addition to its known function in dividing cells.

Published
1997
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44. Somatic and germ cell effects in rats and mice after treatment with 1,3-butadiene and its metabolites, 1,2-epoxybutene and 1,2,3,4-diepoxybutane.

Author

Anderson D, Dobrzyńka MM, Jackson LI, Yu TW, and Brinkworth MH

Subjects
Administration, Inhalation, Animals, Bone Marrow drug effects, Butadienes administration & dosage, Butadienes metabolism, DNA biosynthesis, DNA drug effects, Dose-Response Relationship, Drug, Electrophoresis methods, Epoxy Compounds administration & dosage, Liver drug effects, Male, Mice, Mice, Inbred Strains, Micronucleus Tests, Mutagenicity Tests methods, Mutagens toxicity, Rats, Rats, Sprague-Dawley, Species Specificity, Testis drug effects, Butadienes toxicity, Epoxy Compounds toxicity, Spermatozoa drug effects
Abstract

1,3-Butadiene is produced in large quantities for use in the manufacture of synthetic rubber. It is also an environmental pollutant. There is concern about exposure to 1,3-butadiene as it has been shown to produce tumours in rats, mice and an increased risk of leukaemia in humans. It has also been shown to produce germ cell effects in mice. Differences in responses to 1,3-butadiene have been reported in rats and mice, possibly due to different metabolic capabilities. The present study thus investigated somatic and germ cell effects of 1,3-butadiene in mice and its metabolites in both rats and mice to help determine species differences using different endpoints for genotoxic effects. These included DNA strand breakage as measured in the single cell gel electrophoresis (Comet assay) in bone marrow and testicular cells, and micronuclei in bone marrow cells using both the acridine orange and Giemsa staining methods. Unscheduled DNA synthesis (UDS) was also measured in the testes of mice. CD-1 mice were exposed to 1,3-butadiene by inhalation for 6 h/day for 4 weeks, and CD-1 mice and Sprague-Dawley rats to the metabolites after i.p. injection. 1,3-Butadiene did not affect liver, bone marrow and testicular cells in mice as measured in the Comet assay. After treatment with 1,2-epoxybutene in the Comet assay, there was a response in the testes in mice but not in rats and there was little or no effect in the bone marrow assay in mice but there was in rats. After treatment with 1,2,3,4-diepoxybutane in the Comet assay in mice, there was a response in the bone marrow cells but not in the testicular cells, and in rats there was also a response only in bone marrow cells. There was an increase in micronuclei in both rats and mice with both metabolites, but clastogenicity was stronger with 1,2,3,4-diepoxybutane, occurring at lower doses, than with 1,2-epoxybutene. In the UDS assay in the testes of mice, there was an increase in response with 1,2,3,4-diepoxybutane treatment but not with 1,2-epoxybutene. These studies would appear to confirm a species difference of CD-1 mice and Sprague-Dawley rats, where mice were sensitive at lower doses than rats.

Published
1997
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45. Male-mediated F1 effects in mice exposed to 1,3-butadiene.

Author

Anderson D, Edwards AJ, Brinkworth MH, and Hughes JA

Subjects
Animals, Female, Male, Mice, Abnormalities, Drug-Induced, Butadienes toxicity, Carcinogens toxicity, Fetus drug effects, Mutagens toxicity, Paternal Exposure
Abstract

We examined the effects on dominant lethality, the incidence of fetal abnormalities and tumour incidence in surviving offspring of acute and subchronic exposure of male mice by inhalation to the industrial monomer, 1,3-butadiene. In the acute study, CD-1 mice were exposed to atmospheres containing 0 (n = 25), 1250 (n = 25) or 6250 ppm (n = 50) for 6 h, and each male was caged 5 days later for 1 week with two untreated virgin females. One of the females was killed humanely on day 17 of gestation. The other was allowed to deliver and rear her litter and the litters were monitored throughout adulthood. The killed female was examined for the number of live foetuses, the number of post implantation deaths (early and late) and the number and type of any gross malformations. In the subchronic study, males were exposed to 0 (n = 25), 12.5 (n = 25) or 1250 (n = 50) for 6 h per day on 5 days per week for 10 weeks and then mated the next morning. Mating and observation details were as for the acute study. Acute exposure to butadiene resulted in only a small decrease in implantations; after 10 weeks' subchronic exposure with either the high or low concentration, however, a wide variety of statistically significant effects was seen. At 1250' ppm, the number of implantations was reduced, dominant lethal mutations were induced, and the incidences of early and late deaths were increased; some of the live foetuses were malformed. The low dose also increased the frequency of malformations and late deaths but it did not affect the number of early deaths. Skeletal examination of malformed foetuses, randomly selected normal litter mates and controls confirmed the abnormalities seen at necropsy in malformed foetuses. However, karyotypic analysis of foetal liver from malformed foetuses, randomly selected normal litter mates and controls showed no karyotypic abnormalities. The number of gross suspected tumours in the F1 adults did not appear to reveal an increase over control values. Thus, butadiene is mutagenic in the germ cells of male mice, as shown by the induction of dominant lethality at 1250 ppm, and the frequencies of late deaths and congenital malformations appear to be increased at the subchronic level of 12.5 ppm and skeletal examination of malformed foetuses confirmed the macroscopic abnormalities.

Published
1996
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46. Ubiquitous expression of the androgen receptor and testis-specific expression of the FSH receptor in the cynomolgus monkey (Macaca fascicularis) revealed by a ribonuclease protection assay.

Author

Dankbar B, Brinkworth MH, Schlatt S, Weinbauer GF, Nieschlag E, and Gromoll J

Subjects
Animals, Blotting, Northern methods, Macaca fascicularis, Male, Orchiectomy, Organ Specificity, Receptors, Androgen analysis, Ribonucleases, Gene Expression, RNA, Messenger analysis, Receptors, Androgen genetics, Receptors, FSH genetics, Testis chemistry
Abstract

Androgens are known to exert a variety of effects on an organism while follicle-stimulating hormone (FSH) seems to act specifically on the gonads. To investigate whether these effects are reflected by the expression pattern of the androgen receptor (AR) or the FSH receptor (FSHR) we screened 38 different tissues and organs of one intact and one castrated male non-human primate (Macaca fascicularis). By means of a highly sensitive ribonuclease protection assay (RPA) we demonstrated AR mRNA expression in all tissues of the intact monkey investigated. Immunohistochemistry of selected organs from this monkey revealed a good correlation between AR mRNA and protein expression. In the castrated monkey, the overall AR mRNA expression was markedly lower compared with the intact monkey, although higher expression was present in the pituitary, thyroid and prostate glands. FSHR mRNA was only detected in testicular tissue. This study has revealed, for the first time, ubiquitious expression of the AR mRNA in a non-human primate. The testis-specific expression of the FSHR highlights the importance of FSH for spermatogenesis with the testis being apparently the only target organ.

Published
1995
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47. Identification of male germ cells undergoing apoptosis in adult rats.

Author

Brinkworth MH, Weinbauer GF, Schlatt S, and Nieschlag E

Subjects
Animals, Follicle Stimulating Hormone blood, Gonadotropin-Releasing Hormone pharmacology, Male, Rats, Rats, Sprague-Dawley, Spermatogenesis, Spermatozoa cytology, Spermatozoa drug effects, Staining and Labeling, Testis anatomy & histology, Testis drug effects, Testosterone blood, Acetates pharmacology, Apoptosis drug effects, Gonadotropin-Releasing Hormone analogs & derivatives, Gonadotropin-Releasing Hormone antagonists & inhibitors, Spermatozoa physiology
Abstract

The possible role of apoptosis in spontaneous or induced germ cell death was investigated by treating adult male rats with either a GnRH antagonist (112.5 micrograms kg-1 day-1 for 14 days) or methoxyacetic acid (650 micrograms kg-1; single dose) or sham-treated with either of the vehicles (n = 3 per group). The antagonist virtually abolished gonadotrophin secretion, while methoxyacetic acid reduced serum testosterone concentrations and slightly increased those of FSH (neither significantly). Bands of low molecular mass characteristic of apoptotically degraded DNA were detected by electrophoresis in both treatment groups but not in the controls. Sectioned, Carnoy-fixed testes were screened for degenerating cells with periodic acid-Schiff's base and haemalaun or examined for apoptotic cells using a modified in situ end-labelling procedure. Periodic acid-Schiff's-stained dying cells were found in low numbers in control animals with a distribution and frequency that matched that of apoptotic cells. Degenerating germ cells identified by histology were present at certain stages of spermatogenesis after 2 weeks of antagonist treatment. A comparison of their distribution with that of end-labelled cells identified the cell death as apoptotic. Methoxyacetic acid caused a massive depletion of spermatocytes at stages IX-II, which was also found to be apoptotic. It is concluded that spontaneous germ cell death in adult rats is apoptotic and that both gonadotrophin ablation and administration of methoxyacetic acid can cause apoptosis in the germ cells of adult male rats, but via different routes.

Published
1995
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48. Male-mediated F1 effects in mice exposed to 1,3-butadiene.

Author

Anderson D, Edwards AJ, and Brinkworth MH

Subjects
Animals, Embryo Implantation drug effects, Female, Male, Mice, Mice, Inbred Strains, Abnormalities, Drug-Induced etiology, Butadienes toxicity, Fetal Death chemically induced, Mutagens toxicity, Spermatozoa drug effects
Abstract

We examined the effects on dominant lethality and the incidence of fetal abnormalities of acute and subchronic exposure of male mice by inhalation to the industrial monomer 1,3-butadiene. Investigation of the effect on tumour incidence in surviving offspring is still in progress. In the acute study, CD-1 mice were exposed to atmospheres containing 0 (n = 25), 1250 (n = 25) or 6250 ppm (n = 50) for 6 h, and each male was caged five days later for one week with two untreated virgin females. One of the females was killed humanely on day 17 of gestation. The other was allowed to deliver and rear her litter; the litters are being monitored for life. The killed female was examined for the number of live fetuses, the number of post-implantation deaths (early and late) and the number and type of any gross malformations. In the subchronic study, males were exposed to 0 (n = 25), 12.5 (n = 25) or 1250 ppm (n = 50) for 6 h per day on 5 days per week for 10 weeks and then mated immediately. Mating and observation were conducted as in the acute study. Acute exposure to butadiene resulted in only a small decrease in implantations; after 10 weeks' subchronic exposure to either the high or the low concentration, however, a wide variety of statistically significant effects was seen. At 1250 ppm, the number of implantations was reduced, dominant lethal mutations were induced, and the incidences of early and late deaths were increased; some of the live fetuses had abnormalities. The low dose also increased the frequency of abnormalities and late deaths, but it did not affect the number of early deaths. Thus, butadiene is mutagenic in the germ cells of male mice, as shown by the induction of dominant lethality at 1250 ppm, and the frequencies of late deaths and congenital abnormalities appear to be increased at the subchronic level of 12.5 ppm.

Published
1993

49. A comparison of smokers and nonsmokers with respect to oncogene products and cytogenetic parameters.

Author

Brinkworth MH, Yardley-Jones A, Edwards AJ, Hughes JA, and Anderson D

Subjects
Confounding Factors, Epidemiologic, Female, Humans, Male, Monitoring, Physiologic, Research Design, Chromosome Aberrations, Proto-Oncogene Proteins p21(ras) analysis, Sister Chromatid Exchange, Smoking genetics
Abstract

Human monitoring studies can be valuable tools for assessing the adverse effects of chemicals. Cytogenetic parameters have been frequently employed but are rarely related directly to possible adverse health effects. Recently, the measurement of oncoprotein levels in plasma has been proposed as a possible and more appropriate indicator of exposure and carcinogenic risk but, unlike chromosome damage, little is known about the effects of possible confounding factors. This study compared the effect of smoking on chromosome aberrations, sister chromatid exchange, and plasma ras oncoprotein levels, in forty humans not otherwise known to be exposed to any specific chemical hazard. No effect was found on any of these end points, with the exception of a moderate, statistically nonsignificant elevation of sister chromatid exchange levels. It is concluded that smoking is unlikely to be a confounding factor in human monitoring studies using oncoprotein levels as an end point.

Published
1992

50. Effects of dietary imbalances on spermatogenesis in CD-1 mice and CD rats.

Author

Brinkworth MH, Anderson D, and McLean AE

Subjects
Administration, Oral, Animals, Diet, Male, Mice, Rats, Species Specificity, Dietary Carbohydrates administration & dosage, Dietary Proteins administration & dosage, Spermatogenesis drug effects
Abstract

Nutritional toxicology is now a well established discipline for somatic cells, but no such approach is widely used yet in studies of reproductive toxicology. Reduced dietary intake in mice is known to impair spermatogenesis, and animals in toxicity studies frequently show reduced food intake after dosing. Furthermore, although many human groups have nutritionally inadequate diets, the impact of dietary imbalances on the reproductive system has not been systematically examined. A series of experiments was conducted to dissect the spermatogenic response to dietary alterations in mice and rats. It was found that in mice, the increase in abnormal sperm after such treatment was the result of a lack of calories, while the decrease in sperm counts may have been caused by a lack of protein. In rats, dietary restriction was found only to deplete sperm numbers, probably because of a lack of calories and/or non-energetic components of the diet. Additionally, it was shown that a protein-free diet causes a multiplicity of effects on germ cells, some of which are different in mice and rats. A low-fat diet had an adverse effect on sperm numbers and a similar, but much more pronounced effect was observed in both species fed a carbohydrate-free diet. These alterations of spermatogenic endpoints and the species differences observed, have considerable implications for reproductive toxicology.

Published
1992
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