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v-Src activates a unique phospholipase D activity that can be distinguished from the phospholipase D activity activated by phorbol esters.

机译：v-Src激活独特的磷脂酶D活性可将其与佛波酯所激活的磷脂酶D活性区分开。

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Phospholipase D (PLD) activity, as measured by the transphosphatidylation of cellular phospholipids, is elevated in BALB/c 3T3 cells transformed by v-Src. Phorbol esters that activate protein kinase C (PKC) also increase PLC activity in BALB/c 3T3 cells. v-Src-induced PLD activity could be distinguished from phorbol ester-induced PLD activity by differential radiolabelling of phospholipids, which are the substrates of PLD. Both v-Src- and phorbol ester-induced PLD activity could be detected when phospholipids were prelabelled with either radiolabelled myristate or palmitate; however, only phorbol ester-induced PLD activity could be detected when either arachidonate or 1-O-alkyl-sn-glyceryl-3-phosphorylcholine (alkyl-lysoPC) was used to prelabel the phospholipids. The increased PLD activity in v-Src-transformed cells was not detected when the cells were prelabelled with either arachidonic acid or alkyl-lysoPC, which contains an ether linkage at sn-1 of the glycerol backbone. As both arachidonic acid and alkyl-lysoPC are incorporated into phosphatidylcholine (PC), the substrate for v-Src-induced PLD activity, these data suggest that the PLD activated by v-Src can distinguish PCs lacking arachidonic acid and ether linkages. Consistent with v-Src activating a PLD activity that is distinct from that activated by phorbol esters that activate PKC directly, neither depleting cells of PKC nor treatment with the protein kinase inhibitor, staurosporine, had any effect on v-Src-induced PLD activity, whereas both PKC depletion and staurosporine inhibited phorbol ester-induced PLD activity. Taken together, these data suggest that v-Src activates a PKC-independent PLD activity that is specific for a subpopulation of PC and distinct from the PLD activity induced by PKC activity induced by phorbol esters. The diacylglycerol produced from PC by the action of the v-Src-induced PLD may therefore be responsible for the activation of PKC by v-Src.

机译：通过细胞磷脂的转磷脂酰化测量的磷脂酶D（PLD）活性在被v-Src转化的BALB / c 3T3细胞中升高。激活蛋白激酶C（PKC）的酚酯也可以增加BALB / c 3T3细胞中的PLC活性。 v-Src诱导的PLD活性可通过佛波酯诱导的PLD活性通过磷脂的差异放射性标记来区分，磷脂是PLD的底物。当用放射性标记的肉豆蔻酸酯或棕榈酸酯预先标记磷脂时，可以检测到v-Src-和佛波酯诱导的PLD活性。然而，当使用花生四烯酸酯或1-O-烷基-sn-甘油-3-磷酸胆碱（烷基-lysoPC）预标记磷脂时，仅能检测到佛波酯诱导的PLD活性。当用花生四烯酸或烷基-lysoPC（在甘油骨架的sn-1处含有醚键）进行预标记时，未检测到v-Src转化细胞中PLD活性的增加。由于花生四烯酸和烷基-lysoPC都被掺入了磷脂酰胆碱（PC），这是v-Src诱导的PLD活性的底物，这些数据表明被v-Src激活的PLD可以区分缺乏花生四烯酸和醚键的PC。与v-Src激活PLD活性不同，v-Src激活与直接激活PKC的佛波酯激活的活性不同，消耗PKC的细胞或用蛋白激酶抑制剂星形孢菌素处理均不会对v-Src诱导的PLD活性产生任何影响，而PKC耗竭和星形孢菌素均抑制佛波酯诱导的PLD活性。综上所述，这些数据表明，v-Src激活了不依赖于PKC的PLD活性，该活性对PC亚群具有特异性，并且不同于由佛波酯诱导的PKC活性诱导的PLD活性。因此，通过v-Src诱导的PLD的作用从PC产生的二酰基甘油可能是v-Src激活PKC的原因。

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期刊名称 Biochemical Journal
作者
J Song; D A Foster;
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年(卷),期 1993(294),Pt 3
年度 1993
页码 711–717
总页数 7
原文格式 PDF
正文语种
中图分类分子生物学;
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专利

1. v-Src activates a unique phospholipase D activity that can be distinguished from the phospholipase D activity activated by phorbol esters [J] . D A Foster, J Song The biochemical journal . 1993,第3期

机译：v-Src激活独特的磷脂酶D活性，可将其与佛波酯激活的磷脂酶D活性区分开
2. Phorbol ester treatment of intact rabbit platelets greatly enhances both the basal and guanosine 5′-[γ-thio]triphosphate-stimulated phospholipase D activities of isolated platelet membranes. Physiological activation of phospholipase D may be secondary to activation of phospholipase C [J] . J Van der Meulen, R J Haslam The biochemical journal . 1990,第3期

机译：完整的兔血小板的佛波酯处理可大大增强离体血小板膜的基础和鸟苷5'-[γ-硫]三磷酸刺激的磷脂酶D的活性。磷脂酶D的生理活化可能是继磷脂酶C活化之后的
3. Expression of a peptide binding to receptor for activated C-kinase (RACK1) inhibits phorbol myristoyl acetate-stimulated phospholipase D activity in C3H/10T1/2 cells: dissociation of phospholipase D-mediated phosphatidylcholine breakdown from its syn [J] . Vidar A. T. Thorsen, Bodil Bjorndal, Gary Nolan, Biochimica et Biophysica Acta. Molecular and cell biology of Lipids . 2000,第2a3期

机译：表达与活化C激酶（RACK1）受体结合的肽抑制C3H / 10T1 / 2细胞中佛波醇乙酸肉豆蔻酸酯刺激的磷脂酶D的活性：磷脂酶D介导的磷脂酰胆碱从其syn上解离
4. Secretory Phospholipase A2 as a Site Specific Trigger for Tumor Activation of a Novel Class of Liposomal Prodrug Lipids [C] . Controlled Release Society annual meeting . 2004

机译：分泌磷脂酶A2作为一种肿瘤活化的位点特异性触发，用于一种新型脂质体前药脂质的肿瘤活化
5. Signal regulation of protease-activated receptor-2 and structural determinants of Galpha(q)-dependent activation and deactivation of phospholipase C-beta. [D] . Ricks, Tiffany Kristal. 2010

机译：蛋白酶激活的受体2的信号调节和Galpha（q）依赖性磷脂酶C-β激活和失活的结构决定因素。
6. Phorbol ester treatment of intact rabbit platelets greatly enhances both the basal and guanosine 5-gamma-thiotriphosphate-stimulated phospholipase D activities of isolated platelet membranes. Physiological activation of phospholipase D may be secondary to activation of phospholipase C. [O] . J Van der Meulen, R J Haslam 1990

机译：完整的兔血小板的佛波酯处理极大地增强了分离的血小板膜的基础和鸟苷5-γ-硫代三磷酸刺激的磷脂酶D的活性。磷脂酶D的生理活化可能是继磷脂酶C活化之后的。
7. v-Src activates a unique phospholipase D activity that can be distinguished from the phospholipase D activity activated by phorbol esters. [O] . Song, J, Foster, D A 1993

机译：v-Src激活独特的磷脂酶D活性，可将其与佛波酯所激活的磷脂酶D活性区分开。

v-Src activates a unique phospholipase D activity that can be distinguished from the phospholipase D activity activated by phorbol esters.

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