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向顶端膜和细胞旁途径发出信号:伊蚊马氏管胞质蛋白质组的变化。

Signaling to the apical membrane and to the paracellular pathway: changes in the cytosolic proteome of Aedes Malpighian tubules.

作者信息

Beyenbach Klaus W, Baumgart Sabine, Lau Kenneth, Piermarini Peter M, Zhang Sheng

机构信息

Department of Biomedical Sciences, Cornell University, Ithaca, NY 14853, USA.

出版信息

J Exp Biol. 2009 Feb;212(Pt 3):329-40. doi: 10.1242/jeb.024646.

Abstract

Using a proteomics approach, we examined the post-translational changes in cytosolic proteins when isolated Malpighian tubules of Aedes aegypti were stimulated for 1 min with the diuretic peptide aedeskinin-III (AK-III, 10(-7) mol l(-1)). The cytosols of control (C) and aedeskinin-treated (T) tubules were extracted from several thousand Malpighian tubules, subjected to 2-D electrophoresis and stained for total proteins and phosphoproteins. The comparison of C and T gels was performed by gel image analysis for the change of normalized spot volumes. Spots with volumes equal to or exceeding C/T ratios of +/-1.5 were robotically picked for in-gel digestion with trypsin and submitted for protein identification by nanoLC/MS/MS analysis. Identified proteins covered a wide range of biological activity. As kinin peptides are known to rapidly stimulate transepithelial secretion of electrolytes and water by Malpighian tubules, we focused on those proteins that might mediate the increase in transepithelial secretion. We found that AK-III reduces the cytosolic presence of subunits A and B of the V-type H(+) ATPase, endoplasmin, calreticulin, annexin, type II regulatory subunit of protein kinase A (PKA) and rab GDP dissociation inhibitor and increases the cytosolic presence of adducin, actin, Ca(2+)-binding protein regucalcin/SMP30 and actin-depolymerizing factor. Supporting the putative role of PKA in the AK-III-induced activation of the V-type H(+) ATPase is the effect of H89, an inhibitor of PKA, on fluid secretion. H89 reverses the stimulatory effect of AK-III on transepithelial fluid secretion in isolated Malpighian tubules. However, AK-III does not raise intracellular levels of cAMP, the usual activator of PKA, suggesting a cAMP-independent activation of PKA that removes subunits A and B from the cytoplasm in the assembly and activation of the V-type H(+) ATPase. Alternatively, protein kinase C could also mediate the activation of the proton pump. Ca(2+) remains the primary intracellular messenger of the aedeskinins that signals the remodeling of the paracellular complex apparently through protein kinase C, thereby increasing transepithelial anion secretion. The effects of AK-III on active transcellular and passive paracellular transport are additive, if not synergistic, to bring about the rapid diuresis.

摘要

我们采用蛋白质组学方法,研究了用利尿肽埃及伊蚊激肽-III(AK-III,10⁻⁷ mol l⁻¹)刺激埃及伊蚊分离的马氏管1分钟后,胞质蛋白的翻译后变化。对照(C)和经埃及伊蚊激肽处理(T)的马氏管的胞质溶胶是从数千条马氏管中提取的,进行二维电泳,并对总蛋白和磷酸化蛋白进行染色。通过凝胶图像分析对C和T凝胶进行比较,以观察标准化斑点体积的变化。体积等于或超过C/T比值±1.5的斑点用胰蛋白酶进行胶内消化,并通过纳升液相色谱/串联质谱分析进行蛋白质鉴定。鉴定出的蛋白质涵盖了广泛的生物活性。由于已知激肽肽能迅速刺激马氏管的跨上皮电解质和水分泌,我们重点关注那些可能介导跨上皮分泌增加的蛋白质。我们发现,AK-III降低了V型H⁺ATP酶亚基A和B、内质网素、钙网蛋白、膜联蛋白、蛋白激酶A(PKA)II型调节亚基以及rab GDP解离抑制剂的胞质含量,并增加了内收蛋白、肌动蛋白、Ca²⁺结合蛋白调钙蛋白/SMP30和肌动蛋白解聚因子的胞质含量。PKA抑制剂H89对液体分泌的影响支持了PKA在AK-III诱导的V型H⁺ATP酶激活中的假定作用。H89可逆转AK-III对分离的马氏管跨上皮液体分泌的刺激作用。然而,AK-III不会提高细胞内cAMP水平(PKA的常见激活剂),这表明PKA的激活不依赖cAMP,在V型H⁺ATP酶的组装和激活过程中,PKA将亚基A和B从细胞质中移除。或者,蛋白激酶C也可能介导质子泵的激活。Ca²⁺仍然是埃及伊蚊激肽的主要细胞内信使,显然通过蛋白激酶C发出信号,促使细胞旁复合体重塑,从而增加跨上皮阴离子分泌。AK-III对主动跨细胞和被动细胞旁转运的影响即使不是协同的,也是相加的,从而实现快速利尿。

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