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鉴定首个人工饲养蜜蜂 Ca²⁺通道亚基揭示了两种新型的、物种特异性和剪接特异性调节通道失活的模式。

Characterization of the first honeybee Ca²⁺ channel subunit reveals two novel species- and splicing-specific modes of regulation of channel inactivation.

机构信息

CRBM, UMR 5237, CNRS, Université de Montpellier I&II, Montpellier, France.

出版信息

Pflugers Arch. 2013 Jul;465(7):985-96. doi: 10.1007/s00424-013-1223-2. Epub 2013 Apr 16.

DOI:10.1007/s00424-013-1223-2
PMID:23588376
Abstract

The honeybee is a model system to study learning and memory, and Ca(2+) signals play a key role in these processes. We have cloned, expressed, and characterized the first honeybee Ca(2+) channel subunit. We identified two splice variants of the Apis CaVβ Ca(2+) channel subunit (Am-CaVβ) and demonstrated expression in muscle and neurons. Although AmCaVβ shares with vertebrate CaVβ subunits the SH3 and GK domains, it beholds a unique N terminus that is alternatively spliced in the first exon to produce a long (a) and short (b) variant. When expressed with the CaV2 channels both, AmCaVβa and AmCaVβb, increase current amplitude, shift the voltage-sensitivity of the channel, and slow channel inactivation as the vertebrate CaVβ2a subunit does. However, as opposed to CaVβ2a, slow inactivation induced by Am-CaVβa was insensitive to palmitoylation but displayed a unique PI3K sensitivity. Inactivation produced by the b variant was PI3K-insensitive but staurosporine/H89-sensitive. Deletion of the first exon suppressed the sensitivity to PI3K inhibitors, staurosporine, or H89. Recording of Ba(2+) currents in Apis neurons or muscle cells evidenced a sensitivity to PI3K inhibitors and H89, suggesting that both AmCaVβ variants may be important to couple cell signaling to Ca(2+) entry in vivo. Functional interactions with phospho-inositide and identification of phosphorylation sites in AmCaVβa and AmCaVβb N termini, respectively, suggest that AmCaVβ splicing promoted two novel and alternative modes of regulation of channel activity with specific signaling pathways. This is the first description of a splicing-dependent kinase switch in the regulation of Ca(2+) channel activity by CaVβ subunit.

摘要

蜜蜂是研究学习和记忆的模式生物,钙离子信号在这些过程中起着关键作用。我们已经克隆、表达和鉴定了第一个蜜蜂 Ca2+通道亚基。我们鉴定了两种 Apis CaVβ Ca2+通道亚基(Am-CaVβ)的剪接变体,并证明其在肌肉和神经元中有表达。尽管 AmCaVβ与脊椎动物的 CaVβ 亚基共享 SH3 和 GK 结构域,但它具有独特的 N 端,可在第一外显子中进行选择性剪接,产生长(a)和短(b)变体。当与 CaV2 通道一起表达时,AmCaVβa 和 AmCaVβb 均增加电流幅度、改变通道的电压敏感性,并像脊椎动物的 CaVβ2a 亚基一样减缓通道失活。然而,与 CaVβ2a 不同,Am-CaVβa 诱导的缓慢失活对棕榈酰化不敏感,但表现出独特的 PI3K 敏感性。b 变体诱导的失活对 PI3K 抑制剂、staurosporine/H89 不敏感。删除第一个外显子会抑制对 PI3K 抑制剂、staurosporine 或 H89 的敏感性。在 Apis 神经元或肌肉细胞中记录的 Ba2+电流表明对 PI3K 抑制剂和 H89 敏感,这表明两种 AmCaVβ 变体都可能在体内将细胞信号与 Ca2+内流偶联。AmCaVβa 和 AmCaVβb N 端的磷酸肌醇相互作用和磷酸化位点的鉴定表明,AmCaVβ 的剪接促进了两种新的、替代的调节通道活性的模式,具有特定的信号通路。这是第一个描述 CaVβ 亚基调节 Ca2+通道活性的剪接依赖性激酶开关的例子。

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