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首页> 外文期刊>Andrologia >Evaluation of sperm DNA fragmentation and chromatin structure in infertile men with immotile short‐tail sperm defect
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Evaluation of sperm DNA fragmentation and chromatin structure in infertile men with immotile short‐tail sperm defect

机译:具有Inmotile短尾精子缺损的不育男性精子DNA碎片和染色质结构的评价

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Abstract Teratozoospermia is characterised by the presence of spermatozoa with abnormal morphology. One of the morphological disorders that lead to male infertility is immotile short‐tail sperm (ISTS) defect. In this study, we evaluated the levels of chromatin packing and DNA fragmentation in patients with immotile short‐tail sperm defect. Semen samples were obtained from 31 infertile men with ISTS as case group and 31 normozoospermic men as a control group. Protamine status was evaluated using chromomycin A3 (CMA3) staining and sperm DNA fragmentation assessed by sperm chromatin structure assay (SCSA) and terminal deoxynucleotidyl transferase‐mediated deoxyuridine triphosphate biotin nick‐end labelling (TUNEL). The percentage of positive CMA3 spermatozoa was significantly higher in patients’ samples (22.6?±?6.9) compared with controls (16.3?±?4.2) ( p ??.05) and also mean (± SD ) of sperm DNA fragmentation was significantly higher in patients compared with controls, as measured by TUNEL assay (10.45?±?4.60 vs. 7.03?±?2.86, p ??.05) and SCSA (24.80?±?13.1 vs. 15.2?±?7.2, p ??.05). According to our study, sperm DNA fragmentation and chromatin packing abnormality are significantly higher in the ISTS samples compared with normal samples. A possible explanation for this relationship is that sperm chromatin condensation and sperm flagellum formation occur during the same phase of spermatogenesis.
机译:摘要Teratozoospermia的特征在于具有异常形态的精子存在。导致男性不孕症的形态疾病之一是Incoxile短尾精子(ISTS)缺陷。在这项研究中,我们评估了Incoxile短尾精子缺损患者染色质包装和DNA碎片的水平。从31种因病例组和31种常规组织为对照组的患者获得精液样品。使用色素染色质结构测定(SCSA)和末端脱氧核苷酸转移酶介导的脱氧核苷酸三磷酸生物素位点标记(TUNEL)评估protamycin A3(CMA3)染色和精子DNA片段化评估和精子DNA碎片。与对照组(16.3〜±4.2)(P 1 4.α.4.2)(P 1 4.±4.2)相比,阳性CMA3精子的百分比显着高(22.6?±6.9)患者与对照相比显着较高,如Tunel Assay测量的(10.45?±4.60与7.03?±2.86,P?& 05)和SCSA(24.80?±13.1与15.2?±? 7.2,p?&lt ;? 05)。根据我们的研究,与正常样品相比,ISTS样品中的精子DNA碎片和染色质包装异常显着高。对这种关系的可能解释是在相同的精子发生期间发生精子染色质缩合和精子鞭毛形成。

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