Progesterone and CatSper dependency

International journal of andrology Pub Date : 2012-09-12 DOI:10.1111/j.1365-2605.2012.01294.x

Martin Blomberg Jensen, Stephen J. Publicover

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A breakthrough came from two recent studies (Lishko et al., 2011; Strunker et al., 2011) which showed that progesterone causes activation of the Ca2+-permeable CatSper channel in human spermatozoa, suggesting that CatSper or an associated protein serves as the long sought binding site for progesterone in human spermatozoa.Progesterone not only raises [Ca2+]i in human spermatozoa, it also activates a complex series of signalling events and cell activities. In this issue of the International Journal of Andrology, Sagare-Patil et al. (2012) report that some of these progesterone-mediated effects have characteristics that suggest they are activated by mechanisms independent of CatSper. Sagare-Patil and colleagues used a classical approach to investigate the concentration and time-dependent effects of progesterone. They report clear differences in dose dependence between different responses to progesterone. Motility stimulation, hyperactivation, tyrosine kinase activity, ERK1/2 phosphorylation and P90RSK phosphorylation all showed dose-dependence over 0.01–1 μm, consistent with the action of progesterone on CatSper. Acrosome reaction, tyrosine phosphorylation (analysed from immunofluorescence), P38MAPK phosphorylation, JNK phosphorylation and AKT phosphorylation were dose-dependently induced over the range 1–10 μm progesterone, indicating involvement of a lower affinity binding site for progesterone. These findings are in line with a previous report that progesterone binding and Ca2+ mobilization in human spermatozoa occur at nm progesterone (consistent with CatSper), but that a second low-affinity phase requires ≥5 μm progesterone (Luconi et al., 1998).CatSper is the only identified calcium-permeable channel that has been detected by patch clamp of human spermatozoa (Kirichok & Lishko, 2011). T-type channel blockers NNC 55–0396 (2 μm) and mibefradil (30 μm) abolish CatSper currents in patch clamped human spermatozoa (Lishko et al., 2011; Strunker et al., 2011). These compounds also significantly inhibited the progesterone-induced Ca2+ response, but the signal was not abolished (Strunker et al., 2011). Sagare-Patil et al. (2012) also found that mibefradil (40 μm) was unable to abrogate the calcium increase induced by progesterone (∼80% reduction). In addition, mibefradil only partially inhibited the induction by progesterone of tyrosine phosphorylation and acrosome reaction. Likewise, tyrosine phosphorylation and the acrosome reaction are not diminished in CatSper knockout mouse spermatozoa and a late phase of the ZP-induced Ca2+ increase persists, although at lower frequency, in these cells (Ren & Xia, 2010). These data suggest that an as yet unidentified Ca2+-permeable channel exists in spermatozoa or that significant Ca2+ increases can originate from intracellular calcium stores. Ca2+ storage organelles are present at the sperm neck (Ho & Suarez, 2003; Costello et al., 2009) and thus a second site of progesterone-induced Ca2+ mobilization may occur here. Activated vitamin D (1,25(OH)2D3) appears to work by directly mobilizing stored Ca2+ at the sperm neck. This effect of 1,25(OH)2D3 on [Ca2+]i is smaller than the effect of progesterone but has significant effects on sperm motility and acrosome reaction (Aquila et al.,2009; Blomberg Jensen et al., 2011). 1,25(OH)2D3 differs from progesterone and other activators of CatSper, as the response is mediated by the vitamin D receptor, depends solely on stored intracellular calcium and does not influence the responsiveness to progesterone (Blomberg Jensen et al., 2011). Whether progesterone can directly activate Ca2+ release here remains unclear. Kinetics of the [Ca2+]i rise in response to progesterone are similar throughout the cell (Blomberg Jensen & Dissing, 2012; Blomberg Jensen et al., 2012; Servin-Vences et al., 2012), which is not consistent with a single site of Ca2+ influx in the flagellum. However, rapid buffering of extracellular Ca2+ by application of BAPTA simultaneously with progesterone (to avoid depletion of Ca2+ stores) completely abolished the progesterone-induced Ca2+ signal (Strunker et al., 2011).In conclusion, the findings published by Sagare-Patil et al. (2012) emphasize that the action of progesterone on human spermatozoa is complex and suggest that some of the progesterone-activated effects may not be CatSper dependent. Thus, progesterone signalling may occur by two diverse mechanisms and sites of action: a high affinity binding through CatSper in the tail and possibly a second low-affinity binding site that may be elsewhere in the spermatozoa – the neck/head region being a possibility. There is also a possibility that some progesterone-induced events in human spermatozoa are fully calcium independent. 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引用次数: 3

Abstract

Progesterone is present in high concentrations (μm) in the vicinity of the cumulus-oophorous complex and considered a key signalling factor for human spermatozoa. Progesterone induces an instant increase in intracellular calcium concentration [Ca²⁺]_i despite the absence of the classical progesterone receptor in human spermatozoa. Progesterone causes changes in beating of the flagellum but can also induce acrosome reaction in human spermatozoa. Both these effects are mediated by increased intracellular Ca²⁺ but they are exerted at opposite ends of this highly polarized cell. A breakthrough came from two recent studies (Lishko et al., 2011; Strunker et al., 2011) which showed that progesterone causes activation of the Ca²⁺-permeable CatSper channel in human spermatozoa, suggesting that CatSper or an associated protein serves as the long sought binding site for progesterone in human spermatozoa.

Progesterone not only raises [Ca²⁺]_i in human spermatozoa, it also activates a complex series of signalling events and cell activities. In this issue of the International Journal of Andrology, Sagare-Patil et al. (2012) report that some of these progesterone-mediated effects have characteristics that suggest they are activated by mechanisms independent of CatSper. Sagare-Patil and colleagues used a classical approach to investigate the concentration and time-dependent effects of progesterone. They report clear differences in dose dependence between different responses to progesterone. Motility stimulation, hyperactivation, tyrosine kinase activity, ERK1/2 phosphorylation and P90RSK phosphorylation all showed dose-dependence over 0.01–1 μm, consistent with the action of progesterone on CatSper. Acrosome reaction, tyrosine phosphorylation (analysed from immunofluorescence), P38MAPK phosphorylation, JNK phosphorylation and AKT phosphorylation were dose-dependently induced over the range 1–10 μm progesterone, indicating involvement of a lower affinity binding site for progesterone. These findings are in line with a previous report that progesterone binding and Ca²⁺ mobilization in human spermatozoa occur at nm progesterone (consistent with CatSper), but that a second low-affinity phase requires ≥5 μm progesterone (Luconi et al., 1998).

CatSper is the only identified calcium-permeable channel that has been detected by patch clamp of human spermatozoa (Kirichok & Lishko, 2011). T-type channel blockers NNC 55–0396 (2 μm) and mibefradil (30 μm) abolish CatSper currents in patch clamped human spermatozoa (Lishko et al., 2011; Strunker et al., 2011). These compounds also significantly inhibited the progesterone-induced Ca²⁺ response, but the signal was not abolished (Strunker et al., 2011). Sagare-Patil et al. (2012) also found that mibefradil (40 μm) was unable to abrogate the calcium increase induced by progesterone (∼80% reduction). In addition, mibefradil only partially inhibited the induction by progesterone of tyrosine phosphorylation and acrosome reaction. Likewise, tyrosine phosphorylation and the acrosome reaction are not diminished in CatSper knockout mouse spermatozoa and a late phase of the ZP-induced Ca²⁺ increase persists, although at lower frequency, in these cells (Ren & Xia, 2010). These data suggest that an as yet unidentified Ca²⁺-permeable channel exists in spermatozoa or that significant Ca²⁺ increases can originate from intracellular calcium stores. Ca²⁺ storage organelles are present at the sperm neck (Ho & Suarez, 2003; Costello et al., 2009) and thus a second site of progesterone-induced Ca²⁺ mobilization may occur here. Activated vitamin D (1,25(OH)₂D₃) appears to work by directly mobilizing stored Ca²⁺ at the sperm neck. This effect of 1,25(OH)₂D₃ on [Ca²⁺]_i is smaller than the effect of progesterone but has significant effects on sperm motility and acrosome reaction (Aquila et al.,2009; Blomberg Jensen et al., 2011). 1,25(OH)₂D₃ differs from progesterone and other activators of CatSper, as the response is mediated by the vitamin D receptor, depends solely on stored intracellular calcium and does not influence the responsiveness to progesterone (Blomberg Jensen et al., 2011). Whether progesterone can directly activate Ca²⁺ release here remains unclear. Kinetics of the [Ca²⁺]_i rise in response to progesterone are similar throughout the cell (Blomberg Jensen & Dissing, 2012; Blomberg Jensen et al., 2012; Servin-Vences et al., 2012), which is not consistent with a single site of Ca²⁺ influx in the flagellum. However, rapid buffering of extracellular Ca²⁺ by application of BAPTA simultaneously with progesterone (to avoid depletion of Ca²⁺ stores) completely abolished the progesterone-induced Ca²⁺ signal (Strunker et al., 2011).

In conclusion, the findings published by Sagare-Patil et al. (2012) emphasize that the action of progesterone on human spermatozoa is complex and suggest that some of the progesterone-activated effects may not be CatSper dependent. Thus, progesterone signalling may occur by two diverse mechanisms and sites of action: a high affinity binding through CatSper in the tail and possibly a second low-affinity binding site that may be elsewhere in the spermatozoa – the neck/head region being a possibility. There is also a possibility that some progesterone-induced events in human spermatozoa are fully calcium independent. We encourage future studies to focus on the spatial organization of signalling in human spermatozoa and to determine whether there exists another binding site/channel besides CatSper for progesterone, while we await development of specific inhibitors of CatSper.

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黄体酮和CatSper依赖性

孕酮在卵积云复合体附近以高浓度(μm)存在，被认为是人类精子的关键信号因子。尽管在人类精子中缺乏经典的孕酮受体，孕酮诱导细胞内钙浓度[Ca2+]i立即增加。黄体酮引起鞭毛跳动的变化，但也能引起人精子的顶体反应。这两种作用都是由增加的细胞内Ca2+介导的，但它们是在这个高度极化的细胞的两端施加的。最近的两项研究取得了突破(Lishko et al.， 2011;Strunker et al.， 2011)的研究表明，黄体酮会激活人类精子中Ca2+可渗透的CatSper通道，这表明CatSper或相关蛋白是人类精子中寻找已久的黄体酮结合位点。黄体酮不仅提高了人类精子中的[Ca2+]i，还激活了一系列复杂的信号事件和细胞活动。在这一期的《国际男科杂志》上，Sagare-Patil等人(2012)报道，其中一些黄体酮介导的效应具有一些特征，表明它们是由独立于CatSper的机制激活的。Sagare-Patil和他的同事使用了一种经典的方法来研究黄体酮的浓度和时间依赖性。他们报告了不同黄体酮反应之间剂量依赖性的明显差异。运动刺激、过度活化、酪氨酸激酶活性、ERK1/2磷酸化和P90RSK磷酸化均呈0.01-1 μm以上的剂量依赖性，与黄体酮对CatSper的作用一致。顶体反应、酪氨酸磷酸化(免疫荧光分析)、P38MAPK磷酸化、JNK磷酸化和AKT磷酸化在1-10 μm孕酮范围内呈剂量依赖性，表明孕酮参与了一个较低亲和力的结合位点。这些发现与先前的报告一致，即人类精子中的孕酮结合和Ca2+动员发生在nm孕酮(与CatSper一致)，但第二个低亲和期需要≥5 μm孕酮(Luconi et al.， 1998)。CatSper是唯一通过人类精子膜片钳检测到的钙渗透通道(Kirichok &Lishko, 2011)。t型通道阻滞剂NNC 55-0396 (2 μm)和mibefradil (30 μm)可消除贴片夹紧的人类精子中的CatSper电流(Lishko等，2011;Strunker et al.， 2011)。这些化合物也显著抑制黄体酮诱导的Ca2+反应，但信号并未被消除(Strunker et al.， 2011)。Sagare-Patil等人(2012)也发现，米贝弗拉迪(40 μm)无法消除黄体酮诱导的钙增加(减少约80%)。此外，米贝拉地尔仅部分抑制黄体酮诱导的酪氨酸磷酸化和顶体反应。同样，在敲除CatSper的小鼠精子中，酪氨酸磷酸化和顶体反应并没有减少，并且在这些细胞中，zp诱导的Ca2+增加的后期持续存在，尽管频率较低(Ren &夏,2010)。这些数据表明，精子中存在一个尚未确定的Ca2+可渗透通道，或者显著的Ca2+增加可能源于细胞内钙储存。Ca2+储存细胞器存在于精子颈部(Ho &苏亚雷斯,2003;Costello et al.， 2009)，因此黄体酮诱导的Ca2+动员的第二个位点可能发生在这里。活化的维生素D (1,25(OH)2D3)似乎通过直接动员储存在精子颈部的Ca2+起作用。1,25(OH)2D3对[Ca2+]i的影响比黄体酮的影响小，但对精子活力和顶体反应有显著影响(Aquila等，2009;bloomberg Jensen et al.， 2011)。1,25(OH)2D3不同于黄体酮和其他CatSper的激活剂，因为这种反应是由维生素D受体介导的，完全依赖于细胞内储存的钙，不影响对黄体酮的反应(Blomberg Jensen et al.， 2011)。黄体酮是否能直接激活Ca2+释放尚不清楚。[Ca2+]i升高响应孕酮的动力学在整个细胞中是相似的(Blomberg Jensen &对,2012;Blomberg Jensen et al.， 2012;Servin-Vences et al.， 2012)，这与鞭毛Ca2+内流的单一位点不一致。然而，通过与孕酮同时应用BAPTA快速缓冲细胞外Ca2+(以避免Ca2+存储的消耗)，完全消除了孕酮诱导的Ca2+信号(Strunker等，2011)。总之，Sagare-Patil等人(2012)发表的研究结果强调，黄体酮对人类精子的作用是复杂的，并且表明一些黄体酮激活的作用可能不依赖于CatSper。因此，孕激素信号可能通过两种不同的机制和作用位点发生:通过尾部CatSper的高亲和力结合，以及可能在精子其他地方的第二个低亲和力结合位点(可能是颈部/头部区域)。还有一种可能性是，人类精子中一些黄体酮诱导的事件是完全不依赖钙的。我们鼓励未来的研究将重点放在人类精子信号的空间组织上，并确定除了CatSper之外是否存在另一个孕酮结合位点/通道，同时等待CatSper特异性抑制剂的开发。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

International journal of andrology 医学-男科学

自引率

0.00%

发文量

200

审稿时长

6-12 weeks