局部钙的变化调节生长锥丝状足的长度。

Su Cheng, Matthew S. Geddis, V. Rehder
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引用次数: 42

摘要

已有研究表明,生长球果细胞内游离钙浓度([Ca(2+)](i))可作为生长球果行为的重要调节因子。在这里,我们研究了[Ca(2+)](i)与生长锥行为的一个特定方面(即生长锥丝状足的调节)之间是否存在时空相关性。钙从笼化化合物NP-EGTA(邻硝基苯EGTA四钾盐)中释放出来,以模拟[Ca(2+)]瞬间增加的信号事件(i)。在三种不同的实验范式中,我们释放钙的方式有三种,一种是全局释放(在整个生长锥内),一种是局部释放(在片叶基的一小块区域内),另一种是局部释放(在单个丝足内)。我们证明了生长锥内NP-EGTA的整体光解导致整个生长锥内[Ca(2+)](i)的短暂增加,并引发了随后的丝状延伸,这种延伸仅限于受刺激的生长锥。钙调素或钙(2+)依赖性磷酸酶(钙调磷酸酶)钙调磷酸酶(钙调磷酸酶)的药理阻断抑制了钙的释放作用,这表明这些酶在钙的下游起作用。片叶基局部脱钙引起[Ca(2+)](i)的局部增加,但引起整个生长锥的丝状延伸。单个丝足内[Ca(2+)](i)的局部升高只导致受刺激的丝足伸长。这些发现表明,[Ca(2+)](i)的升高对丝状行为的影响取决于钙信号的空间分布。特别是,丝状伪足内的钙信号可以引起丝状伪足长度的变化,这可能是在体内寻路过程中看到的定向丝状伪足转向事件的第一步。
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Local calcium changes regulate the length of growth cone filopodia.
Previous studies have demonstrated that the free intracellular calcium concentration ([Ca(2+)](i)) in growth cones can act as an important regulator of growth cone behavior. Here we investigated whether there is a spatial and temporal correlation between [Ca(2+)](i) and one particular aspect of growth cone behavior, namely the regulation of growth cone filopodia. Calcium was released from the caged compound NP-EGTA (o-nitrophenyl EGTA tetrapotassium salt) to simulate a signaling event in the form of a transient increase in [Ca(2+)](i). In three different experimental paradigms, we released calcium either globally (within an entire growth cone), regionally (within a small area of the lamellipodium), or locally (within a single filopodium). We demonstrate that global photolysis of NP-EGTA in growth cones caused a transient increase in [Ca(2+)](i) throughout the growth cone and elicited subsequent filopodial elongation that was restricted to the stimulated growth cone. Pharmacological blockage of either calmodulin or the Ca(2+)-dependent phosphatase, calcineurin, inhibited the effect of uncaging calcium, suggesting that these enzymes are acting downstream of calcium. Regional uncaging of calcium in the lamellipodium caused a regional increase in [Ca(2+)](i), but induced filopodial elongation on the entire growth cone. Elevation of [Ca(2+)](i) locally within an individual filopodium resulted in the elongation of only the stimulated filopodium. These findings suggest that the effect of an elevation of [Ca(2+)](i) on filopodial behavior depends on the spatial distribution of the calcium signal. In particular, calcium signals within filopodia can cause filopodial length changes that are likely a first step towards directed filopodial steering events seen during pathfinding in vivo.
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