突触小泡膜蛋白与神经递质释放的局部调节

突触小泡膜蛋白及其在神经递质释放过程中的作用已取得若干研究进展.突触素I、SY蛋白、SO蛋白、SB蛋白、SG蛋白等都是突触小泡膜的重要蛋白质,这些蛋白质在突触小泡的贴靠、膜融合及胞吐作用中起着局部自主性调节作用.     

甲基紫精对水稻幼苗根细胞膜微囊Ca2+-ATP酶活性的影响

10μmool/L甲基紫精(MV)预处理水稻幼苗可明显提高其抗冷力,但这种功效可被钙的螯合剂EGTA(10 mmol/L)和钙调素(CaM)的抑制剂氯丙嗪(CPZ,0.5 mmol/L)所抑制.MV预处理提高了幼苗质膜、液泡膜Ca2+-ATP酶活性,同时也有提高质膜Fe(CN)3-6还原速率和这些活性的冷适应性,但这些效果均可被EGTA和CPZ所抑制.离体条件下,膜微囊的Ca2+-ATP酶活性对H2O2、O-2、-OH敏感.结果显示,MV预处理提高幼苗的抗冷力可能是通过钙信使介导起作用的,钙信使或CaM可能刺激了质膜、液泡膜Ca2+-ATP酶活性;而该预处理有增加质膜、液泡膜Ca2+-ATP酶的冷稳定性则可能与该处理有提高细胞抗氧化能力、稳定冷胁迫下细胞膜系统结构有关.     

Cadmium impairs ion homeostasis by altering K+ and Ca2+ channel activities in rice root hair cells

Cadmium (Cd²⁺) interferes with the uptake, transport and utilization of several macro‐ and micronutrients, which accounts, at least in part, for Cd²⁺ toxicity in plants. However, the mechanisms underlying Cd²⁺ interference of ionic homeostasis is not understood. Using biophysical techniques including membrane potential measurements, scanning ion‐selective electrode technique for non‐invasive ion flux assays and patch clamp, we monitored the effect of Cd²⁺ on calcium (Ca²⁺) and potassium (K⁺) transport in root hair cells of rice. Our results showed that K⁺ and Ca²⁺ contents in both roots and shoots were significantly reduced when treated with exogenous Cd²⁺. Further studies revealed that three cellular processes may be affected by Cd²⁺, leading to changes in ionic homeostasis. First, Cd²⁺‐induced depolarization of the membrane potential was observed in root hair cells, attenuating the driving force for cation uptake. Second, the inward conductance of Ca²⁺ and K⁺ was partially blocked by Cd²⁺, decreasing uptake of K⁺ and Ca²⁺. Third, the outward K⁺ conductance was Cd²⁺‐inducible, decreasing the net content of K⁺ in roots. These results provide direct evidence that Cd²⁺ impairs uptake of Ca²⁺ and K⁺, thereby disturbing ion homeostasis in plants.     

Ca2+ and Calmodulin-Dependent Phosphorylation of Endogenous Synaptic Vesicle Tubulin by a Vesicle-Bound Calmodulin Kinase System

Endogenous synaptic vesicle alpha- and beta-tubulin were shown to be the major substrates for a Ca2+-calmodulin-regulated protein kinase system in enriched synaptic vesicle preparations from rat cortex as determined by two-dimensional gel electrophoresis and peptide mapping. The activation of this endogenous tubulin kinase system was dependent on Ca2+ and the Ca2+ binding protein, calmodulin. Under maximally stimulated conditions, approximately 40% of the tubulin present in enriched synaptic vesicles was phosphorylated within less than 50 s by the vesicle Ca2+-calmodulin kinase. Evidence is presented indicating that the Ca2+-calmodulin tubulin kinase is an enzyme system distinct from previously described cyclic AMP protein kinases. alpha-Tubulin and beta-tubulin were identified as major components of previously designated vesicle phosphorylation bands DPH-L and DPH-M. The Ca2+-calmodulin tubulin kinase is very labile and specialized isolation procedures were necessary to retain activity. Ca2+-activated synaptic vesicle tubulin phosphorylation correlated with vesicle neurotransmitter release. Depolarization-dependent Ca2+ uptake in intact synaptosomes simultaneously stimulated the release of neurotransmitters and the phosphorylation of synaptic vesicle alpha- and beta-tubulin. The results indicate that regulation of the synaptic vesicle tubulin kinase by Ca2+ and calmodulin may play a role in the functional utilization of synaptic vesicle tubulin and may mediate some of the effects of Ca2+ on vesicle function and neurosecretion.     

咖啡因和茶碱对大鼠皂素蜕膜心肌肌钙蛋白Ca~(2 )敏感性和肌浆网Ca~(2 )释放的影响

在低浓度皂素（50μg／ml）制备的浆膜蜕变（通透性增高）而肌浆网（SR）膜无损的蜕膜心肌标本上,以其收缩的幅度作为SRCa(2 )释放的半定量指标;高浓度皂素（500μg／ml）制备的浆膜和SR膜均蜕变的蜕膜心肌标本,以其张力-PCa关系曲线以及产生50％最大张力所需的Ch(2 )浓度（PCa50）分别作为肌钙蛋白（TN）Ca(2 )敏感性的定性和定量指标。结果观察到：（1）在低浓度皂素蜕膜心肌标本上,5和10mmol／L咖啡因分别引起约89．2±12．7和142．5±17mg（n＝4,P＜0．05）张力的强直收缩,而5mmol／L茶碱未能引起明显的强直收缩;（2）在高浓度皂素蜕膜心肌标本上,5和10mmol／L咖啡因及5mmol／L茶碱均使张力-pCa关系曲线左移;PCa50较对照分别增加了0．261,0．274和0．212PCa单位（P均小于0．001）。上述结果提示：咖啡因和茶碱均能增高TNCa(2 )敏感性;此外,咖啡因尚有促使SR释放Ca(2 )的作用。     

产前应激对子代大鼠海马CA3区神经元Ca2+和K+通道的影响

本研究的目的在于探讨产前应激对子代大鼠海马CA3神经元高电压激活(HVA)钙通道、延迟整流钾电流(delayedrectifierpotassiumcurrents,IKD)的影响。产前应激(prenatalstress,PNS)组孕鼠孕晚期给予束缚应激,应用全细胞膜片钳技术进行研究。结果显示产前应激增加了子代海马CA3神经元HVA钙通道峰电流幅值,对照组和产前应激组子代CA3神经元平均最大HVA钙电流峰值分别为-576.52±7.03pA和-702.05±6.82pA(P<0.01)。同时未改变其电导-电压关系,也未改变延迟整流钾通道电流-电压关系、电导-电压关系。结果提示,在胎儿发育的关键时期,给予母体产前应激,引起子代海马神经元HVA钙电流增加,其机制一方面PNS导致皮质酮升高,从而可能增加HVA钙通道mRNA表达;另一方面PNS所致反应性氧化产物(reactiveoxygenspecies,ROS)增多,后者可能通过磷酸化HVACa2 通道亚单位,从而提高HVA钙电流幅值。     

Conserved biophysical features of the CaV2 presynaptic Ca2+ channel homologue from the early-diverging animal Trichoplax adhaerens

The dominant role of Ca_V2 voltage-gated calcium channels for driving neurotransmitter release is broadly conserved. Given the overlapping functional properties of Ca_V2 and Ca_V1 channels, and less so Ca_V3 channels, it is unclear why there have not been major shifts toward dependence on other Ca_V channels for synaptic transmission. Here, we provide a structural and functional profile of the Ca_V2 channel cloned from the early-diverging animal Trichoplax adhaerens, which lacks a nervous system but possesses single gene homologues for Ca_V1–Ca_V3 channels. Remarkably, the highly divergent channel possesses similar features as human Ca_V2.1 and other Ca_V2 channels, including high voltage–activated currents that are larger in external Ba²⁺ than in Ca²⁺; voltage-dependent kinetics of activation, inactivation, and deactivation; and bimodal recovery from inactivation. Altogether, the functional profile of Trichoplax Ca_V2 suggests that the core features of presynaptic Ca_V2 channels were established early during animal evolution, after Ca_V1 and Ca_V2 channels emerged via proposed gene duplication from an ancestral Ca_V1/2 type channel. The Trichoplax channel was relatively insensitive to mammalian Ca_V2 channel blockers ω-agatoxin-IVA and ω-conotoxin-GVIA and to metal cation blockers Cd²⁺ and Ni²⁺. Also absent was the capacity for voltage-dependent G-protein inhibition by co-expressed Trichoplax Gβγ subunits, which nevertheless inhibited the human Ca_V2.1 channel, suggesting that this modulatory capacity evolved via changes in channel sequence/structure, and not G proteins. Last, the Trichoplax channel was immunolocalized in cells that express an endomorphin-like peptide implicated in cell signaling and locomotive behavior and other likely secretory cells, suggesting contributions to regulated exocytosis.     

Munc13-1 is a Ca2+-phospholipid-dependent vesicle priming hub that shapes synaptic short-term plasticity and enables sustained neurotransmission

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