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与公羊精子获能和顶体酶外排相关的钙调蛋白免疫细胞化学定位变化。

Changes in calmodulin immunocytochemical localization associated with capacitation and acrosomal exocytosis of ram spermatozoa.

作者信息

Colás C, Grasa P, Casao A, Gallego M, Abecia J A, Forcada F, Cebrián-Pérez J A, Muiño-Blanco T

机构信息

Department of Biochemistry and Molecular and Cell Biology, University of Zaragoza, Miguel Servet, 177, 50013 Zaragoza, Spain.

出版信息

Theriogenology. 2009 Mar 15;71(5):789-800. doi: 10.1016/j.theriogenology.2008.10.003. Epub 2008 Dec 9.

Abstract

The aim of this study was to determine the localization of calmodulin (CaM) in ram sperm and the possible changes during in vitro capacitation (CA) and the ionophore-induced acrosome reaction (AR). Likewise, changes in intracellular calcium levels (Ca(2+)) were also analysed by using flow cytometry. CA was induced in vitro in a medium containing BSA, CaCl(2), NaHCO(3), and AR by the addition of the calcium ionophore A23187. The acrosomal status was assessed by the chlortetracycline-fluorescence (CTC) assay. Flow cytometry (FC) analyses were performed by loading samples with Fluo-3 AM, that emits fluorescence at a high Ca(2+), combined with propidium iodide (PI) that allowed us to discriminate sperm with/without an integral plasma membrane both with high/low Ca(2+). Immunocytochemistry localized CaM to the flagellum, and some sperm also contained CaM in the head (equatorial and post-acrosomal regions). CA and AR resulted in a slight increase in the post-acrosomal labelling. The treatment of sperm with increasing concentrations of two CaM antagonists, W7 and calmidazolium (CZ), accounted for an increase in capacitated and acrosome-reacted CTC-sperm patterns. CZ induced a significant reduction in the content of three protein tyrosine-phosphorylated bands of approximately of 30, 40 and 45kDa. However, W7 showed no significant effect at any of the studied concentrations. Neither of them significantly influenced protein serine and threonine phosphorylation. FC analysis revealed that the main subpopulation in the control samples contained 70% of the total sperm with integral plasma membrane and a medium Ca(2+). After CA, 67.1% of the sperm preserved an integral membrane with a higher Ca(2+). After AR, only 7.2% of the total sperm preserved intact membranes with a very high Ca(2+). These results imply that CaM appears to be involved in ram sperm capacitation, and both treatments increased its localization in the post-acrosomal region.

摘要

本研究的目的是确定钙调蛋白(CaM)在公羊精子中的定位以及体外获能(CA)和离子载体诱导的顶体反应(AR)过程中可能发生的变化。同样,还通过流式细胞术分析了细胞内钙水平([Ca(2+)]i)的变化。在含有牛血清白蛋白(BSA)、氯化钙(CaCl2)、碳酸氢钠(NaHCO3)的培养基中体外诱导CA,并通过添加钙离子载体A23187诱导AR。通过金霉素荧光(CTC)测定评估顶体状态。通过用Fluo-3 AM加载样品进行流式细胞术(FC)分析,Fluo-3 AM在高[Ca(2+)]i时发出荧光,结合碘化丙啶(PI),使我们能够区分具有完整质膜且[Ca(2+)]i高/低的精子。免疫细胞化学将CaM定位到鞭毛,一些精子的头部(赤道和顶体后区域)也含有CaM。CA和AR导致顶体后标记略有增加。用两种CaM拮抗剂W7和氯米帕明(CZ)的浓度增加处理精子,导致获能和顶体反应的CTC精子模式增加。CZ诱导约30、40和45kDa的三条蛋白质酪氨酸磷酸化带的含量显著降低。然而,W7在任何研究浓度下均未显示出显著影响。它们都没有显著影响蛋白质丝氨酸和苏氨酸的磷酸化。FC分析显示,对照样品中的主要亚群包含70%具有完整质膜且[Ca(2+)]i中等的总精子。CA后,67.1%的精子保留了完整的膜且[Ca(2+)]i较高。AR后,仅7.2%的总精子保留了完整的膜且[Ca(

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