A single, mild, transient scrotal heat stress causes DNA damage, subfertility and impairs formation of blastocysts in mice

Paul, Catriona; Murray, Alison; Spears, Norah; Saunders, Philippa T. K.

doi:10.1530/rep-08-0036

Cited by 222 publications

(190 citation statements)

References 72 publications

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“…In general, the major deleterious effects of the TNP in affected tubules were the occurrence of intraepithelial vacuoles of varying size, slouging and seminiferous tubule atrophy. The vacuoles we observed within the seminiferous epithelium resembled those described following a variety of testicular insults including exposure to toxicants, hypophysectomy, transient scrotal heat stress and acute withdrawal of androgens following destruction of Leydig cells with ethane dimethane sulphonate [39][40][41][42][43]. Sloughing is caused by the effects of the chemical on microtubules and intermediate filaments of the Sertoli cell.…”

Section: Discussionsupporting

confidence: 62%

Effect of beta-carotene on titanium oxide nanoparticles-induced testicular toxicity in mice

Orazizadeh

Khorsandi

Absalan

et al. 2014

J Assist Reprod Genet

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Objective This study evaluated the protective effect of betacarotene (BC) on titanium oxide nanoparticle (TNP) induced spermatogenesis defects in mice. Materials and methods Thirty-two NMRI mice were randomly divided into four groups. BC group received 10 mg/kg of BC for 35 days. TNP group received 300 mg/kg TNP for 35 days. TNP+BC group initially received 10 mg/kg BC for 10 days and was followed by concomitant administration of 300 mg/kg TNP for 35 days. Control group received only normal saline for 35 days. Epididymal sperm parameters, testicular histopathology, spermatogenesis assessments and testosterone assay were performed for evaluation of the TNP and BC effects on testis. Results Serum testosterone levels were markedly decreased in TNP-intoxicated mice. Epididymal sperm parameters including sperm number, motility and percentage of abnormality were significantly changed in TNP-intoxicated mice (p < 0.01). Histopathological criteria such as epithelial vacuolization, sloughing of germ cells and detachment were significantly increased in TNP-intoxicated mice (p<0.001). BC+TNP treatment significantly prevented these changes (p<0.05). BC also significantly elevates testosterone levels in BC+TNP group compared to TNP-treated mice (p<0.01). Discussion and conclusion The results of this study demonstrated that BC improved the spermatogenesis defects in TNPtreated mice. BC had a potent protective effect against the testicular toxicity and might be clinically useful.

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Section: Discussionsupporting

confidence: 62%

Effect of beta-carotene on titanium oxide nanoparticles-induced testicular toxicity in mice

Orazizadeh

Khorsandi

Absalan

et al. 2014

J Assist Reprod Genet

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“…Incubation of spermatozoa at 398C for 24 h before fertilisation has been reported to decrease blastocyst developmental competence (Lechniak et al 2003), which we confirmed in the present study using spermatozoa incubated at 418C for 4 h. It is conceivable that the quality of blastocysts produced after fertilisation of oocytes with heatstressed spermatozoa is compromised because of the increased level of sperm DNA damage. Similarly, several studies have reported that mice exposed to scrotal heat stress have an increased percentage of spermatozoa with high levels of DNA damage and, as such, insemination using these spermatozoa ultimately resulted in impaired blastocyst formation (Jannes et al 1998;Paul et al 2008;2009). Further in vitro studies in cattle have confirmed these findings: Walters et al (2005aWalters et al ( , 2005b observed less blastocyst development with higher ACR after fertilisation of oocytes with semen collected from scrotalinsulated bulls.…”

Section: Discussionmentioning

confidence: 83%

“…Studies indicate that the contribution of a spermatozoon to the oocyte is more than delivering the paternal genome, and that the centriole (for a review, see Sutovsky and Schatten 1999), RNA (Ostermeier et al 2004) and proper epigenetic marks in the form of DNA methylation (for a review, see Miller et al 2010;Steger et al 2011) are almost equally important for successful fertilisation and embryo development. Hence, in addition to causing sperm DNA damage (Paul et al 2008(Paul et al , 2009, it is also possible that heat stress damages the sperm centriole and/or causes aberrant DNA methylation in the male pronucleus that subsequently leads to a delay in fertilisation or fertilisation failure; this would be an interesting area for future research. Incubation of spermatozoa at 398C for 24 h before fertilisation has been reported to decrease blastocyst developmental competence (Lechniak et al 2003), which we confirmed in the present study using spermatozoa incubated at 418C for 4 h. It is conceivable that the quality of blastocysts produced after fertilisation of oocytes with heatstressed spermatozoa is compromised because of the increased level of sperm DNA damage.…”

Section: Discussionmentioning

confidence: 99%

Bovine spermatozoa react to in vitro heat stress by activating the mitogen-activated protein kinase 14 signalling pathway

Rahman

Vandaele²,

Rijsselaere

et al. 2014

Reprod. Fertil. Dev.

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Abstract. Heat stress has long been recognised as a cause of subfertility in farm animals. The objectives of the present study were to elucidate the effect of heat stress on sperm function and involvement of the mitogen-activated protein kinase (MAPK) 14 signalling pathway. Spermatozoa incubated for 4 h at a physiological temperature (38.58C) exhibited significantly (P , 0.05) reduced motility, plasma membrane integrity and mitochondrial potential compared with nonincubated spermatozoa; the reductions in these parameters were more severe following incubation at a hyperthermic (418C) temperature (P , 0.01). Percentages of fertilisation and embryo development were highly affected in spermatozoa incubated at 418C compared with non-incubated spermatozoa (P , 0.01). Similarly, embryo quality was adversely affected by sperm incubation at 418C, as indicated by a higher apoptotic cell ratio in Day 7 blastocysts compared with that in the non-incubated control group (14.6% vs 6.7%, respectively; P , 0.01). Using SB203580 (10 mg mL À1 ), a specific inhibitor of the p38 MAPK pathway, during sperm hyperthermia reduced MAPK14 activation (24.9% vs 35.6%), increased sperm motility (45.8% vs 26.5%) and reduced DNA fragmentation (16.9% vs 23.4%) compared with the untreated control group, but did not improve subsequent fertilisation and embryo development. In conclusion, heat stress significantly affects the potential of spermatozoa to penetrate oocytes, as well as subsequent embryo development and quality. Notably, the data show that the MAPK14 signalling pathway is largely involved in heat-induced sperm damage. However, further research is needed to elucidate other signalling pathways possibly involved in heat-induced sperm damage.Additional keywords: functional parameters, mitogen-activated protein kinase 14 phosphorylation, terminal deoxyribonucleotidyl transferase-mediated dUTP-digoxigenin nick end-labelling.

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“…To study the effects of TXLNA ablation on testicular phagocytic activity, we treated mice with a single, mild, transient scrotal heat stress (HS). 16 At post-HS 24 h or 14 d, testes were harvested and subjected to apoptotic analyses. These two time points were chosen because HS-induced apoptosis increases to the maximum level at about 24 h, and then disappears by 14 d. 17 Histological examinations revealed a significant increase in the apoptotic GCs at post-treatment 24 h (black arrows in Supplementary Figure 1).…”

Section: Resultsmentioning

confidence: 99%

Unexpected requirement for a binding partner of the syntaxin family in phagocytosis by murine testicular Sertoli cells

Hou

et al. 2015

Cell Death Differ

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A single, mild, transient scrotal heat stress causes DNA damage, subfertility and impairs formation of blastocysts in mice

Cited by 222 publications

References 72 publications

Effect of beta-carotene on titanium oxide nanoparticles-induced testicular toxicity in mice

Effect of beta-carotene on titanium oxide nanoparticles-induced testicular toxicity in mice

Bovine spermatozoa react to in vitro heat stress by activating the mitogen-activated protein kinase 14 signalling pathway

Unexpected requirement for a binding partner of the syntaxin family in phagocytosis by murine testicular Sertoli cells

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