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Protein kinase C regulates FLT1 abundance and stimulates its cleavage in vascular endothelial cells with the release of a soluble PlGF/VEGF antagonist

机译:蛋白激酶C调节FLT1的丰度并通过释放可溶性PlGF / VEGF拮抗剂刺激其在血管内皮细胞中的裂解

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摘要

FLT1 and its soluble form (sFLT1) arise as alternate transcripts from the same gene and sFLT1 can antagonize the effect of vascular endothelial growth factor (VEGF) on its cognate receptors. We investigated the effect of VEGF and protein kinase C (PKC) activation on sFLT1 abundance. We demonstrated that VEGF stimulates sFLT1 and FLT1 mRNA and protein levels in vascular endothelial cells via VEGFR2 and PKC. Using an FLT1 expression vector with N and C-terminal epitope tags, we show that PKC activation increases the cleavage of FLT1 into an N-terminal extracellular fragment and a C-terminal intracellular fragment with the cleavage occurring adjacent to the transmembrane domain. The trafficking and glycosylation inhibitors brefeldin, monensin and tunicamycin substantially reduced cleavage and release of the N-terminal ectodomain of FLT1 and inhibited secretion of the isoforms of sFLT1. The shed FLT1 ectodomain can bind VEGF and PlGF and inhibit VEGF-induced vascular tube formation thus confirming that it is functionally equivalent to the alternately spliced and secreted sFLT1 isoforms.
机译:FLT1及其可溶形式(sFLT1)作为同一基因的替代转录物出现,而sFLT1可以拮抗血管内皮生长因子(VEGF)对其同源受体的作用。我们调查了VEGF和蛋白激酶C(PKC)激活对sFLT1丰度的影响。我们证明了VEGF通过VEGFR2和PKC刺激血管内皮细胞中的sFLT1和FLT1 mRNA和蛋白水平。使用具有N和C末端抗原决定簇标签的FLT1表达载体,我们显示PKC激活增加了FLT1裂解为N末端细胞外片段和C末端细胞内片段的裂解,裂解发生在跨膜结构域附近。贩运和糖基化抑制剂布雷菲德菌素,莫能菌素和衣霉素实质上减少了FLT1 N端胞外域的切割和释放,并抑制了sFLT1同工型的分泌。脱落的FLT1胞外域可结合VEGF和PlGF并抑制VEGF诱导的血管形成,因此证实其在功能上等同于交替剪接和分泌的sFLT1同工型。

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